AU2012241142B2

AU2012241142B2 - Use of genetically modified organisms to generate biomass degrading enzymes

Info

Publication number: AU2012241142B2
Application number: AU2012241142A
Authority: AU
Inventors: Stephen Mayfield; Michael Mendez; Bryan O'neill; Yan Poon
Original assignee: Scripps Research Institute; Sapphire Energy Inc
Current assignee: Scripps Research Institute; Sapphire Energy Inc
Priority date: 2007-06-01
Filing date: 2012-10-12
Publication date: 2013-03-14
Anticipated expiration: 2028-05-30
Also published as: AU2012241142A1

Abstract

The present invention provides a method and compositions for high throughput screening of genetically modified photosynthetic organisms for plasmic state. The present invention provides methods of producing one or more proteins, including biomass degrading enzymes in a plant. Also provided are the methods of producing biomass degradation pathways in alga cells, particularly in the chloroplast. Single enzymes or multiple enzymes may be produced by the methods disclosed. The methods disclosed herein allow for the production of biofuel, including ethanol.

Description

Regulation 3.2 AUSTRALIA Patents Act 1990 COMPLETE SPECIFICATION STANDARD PATENT Invention Title: Use of genetically modified organisms to generate biomass degrading enzymes The following statement is a full description of this invention, including the best method of performing it known to us: USE OF GENETICALLY MODIFIED ORGANISMS TO GENERATE BIOMASS DEGRADING ENZYMES CROSS-REFERENCE [0001] This application claims priority to and the benefit of the following U.S. Provisional Applications: USSN 60/941,452, filed June 1, 2007, entitled of "USE OF PHOTOSYNTHETIC ORGANISMS TO GENERATE BIOFUELS" by Mayfield et al; USSN 61/070,384, filed March 20, 2008, entitled "USE OF GENETICALLY MODIFIED ORGANISMS TO GENERATE BIOMASS DEGRADING ENZYMES" by Mayfield et al.; and USSN 61/070,437 filed March 20, 2008, entitled "HIGH THROUGHPUT SCREENING OF GENETICALLY MODIFIED PHOTOSYNTHETIC ORGANISMS" by Mayfield et al. Each of these prior applications is incorporated herein by reference. INCORPORATION BY REFERENCE [0002] All publications and patent applications mentioned in this specification are herein incorporated by reference to the same extent as if each individual publication or patent application was specifically and individually indicated to be incorporated by reference. BACKGROUND OF THE INVENTION [0003] Fuel is becoming increasingly more expensive. Also, fuel refinery is associated with the generation of pollutants and global warming. There is an increasing need in the industry to find cheaper, safer, and more environmentally unharmful ways to generate fuels. The development of means to produce fuel from biological material is an essential component of the future energy landscape. One of the most important elements in the production of fuel from biologic materials is the ability to digest or reduce certain molecular structures, such as cellulose, to molecular species recognizable as substrate for fuel generating processes, such as fermentation. (00041 Molecular biology and genetic engineering hold promise for the production of large quantities of biologically active molecules that can be used to produce such fuels. For example, production of enzymes capable of breaking down organic materials into fuels hold promise to address the increasing needs for alternative fuels. A primary advantage of using genetic engineering techniques for producing such enzymes is that the methods allow for the generation of large amounts of a desired protein. In many cases, the only other way to obtain sufficient quantities of biological materials from non-engineered secretion sources is by purifying the naturally occurring biological material from cells of an organism that produce the agent. Thus, prior to the advent of genetic engineering, enzymes capable of degrading organic materials could only be isolated by growing the organism, typically a bacterial or fungal species, in large quantities and extracting the protein. Such procedures are often complex and economically prohibitive for use in fuel production. (0005] Although genetic engineering provides a means to produce large amounts of a biological material, particularly proteins and nucleic acids, there are limitations to currently available methods. Bacteria provide an environment suitable to the production of such enzymes; however, byproducts produced by some bacteria would contaminate fuel sources. Thus, even where bacteria can be used to produce the biological material, additional steps such as purification or refining may be required to obtain biologically active material and/or bio-fuel. Furthermore, the use of non-photosynthetic systems requires the addition of costly sugar or other organic carbon sources to feed the recombinant organism. Additionally, there is typically a large capital investment associated with building fermenters.

[0006] Recombinant proteins also can be produced in eukaryotic cells, including, for example, fungi, insect cells and mammalian cells, which may provide the necessary environment to process an expressed protein into a biologically active agent. However, these systems typically suffer from the same cost prohibitions (sugar/organic carbon sources and fermenters). Thus, a need exists for methods to conveniently produce enzymes that are biologically active, can produce large quantities of enzymes and/or provide a host organism which is compatible with production of degradative enzymes. SUMMARY OF THE INVENTION [0007] Presented herein are compositions and methods for the production of biomass degrading enzymes and biofuels. The inventions disclosed herein provide novel methods for the production of biomass degrading enzymes, typically in genetically modified photosynthetic organisms such as algae and cyanobacteria. Also presented herein are compositions and methods for transforming photosynthetic organisms and methods of screening transformants. [0008] Accordingly, one aspect of the present invention provides a vector comprising a nucleic acid encoding a biomass degrading enzyme and a promoter configured for expression of the nucleic acids in a non vascular photosynthetic organism. Vectors of the present invention may contain nucleic acids encoding more than one biomass degrading enzyme and, in other instances, may contain nucleic acids encoding polypeptides which covalently link biomass degrading enzymes. Biomass degrading enzymes may include cellulolytic enzymes, hemicellulolytic enzymes and ligninolytic enzymes. More specifically, the biomass degrading enzymes may be exo-p-glucanase, endo-p-glucanase, 0-glucosidase, endoxylanase, or lignase. Nucleic acids encoding the biomass degrading enzymes may be derived from fungal or bacterial sources, for example, those encoding exo-$-glucanase in Trichoderma viride, exo-o-glucanase in Trichoderna reesel, exo-o-glucanase in Aspergillus aculeatus, endo-o-glucanase in Trichoderma reesei, endo-p-glucanase in Aspergillus niger, 0 glucosidase in Trichoderma reesei, $-glucosidase in Aspergillus niger endoxylanase in Trichoderma reesei, and endoxylanase in Aspergillus niger. Other nucleic acids encoding biomass degrading enzymes may be homologous to the genes from these organisms [0009] A vector of the present invention may also contain a selectable marker, allowing for direct screening of transformed organisms. The vectors of the present invention may be capable of stable transformation of multiple photosynthetic organisms, including, but not limited to, photosynthetic bacteria (including cyanobacteria), cyanophyta, prochlorophyta, rhodophyta, chlorophyta, heterokontophyta, tribophyta, glaucophyta, chlorarachniophytes, euglenophyta, euglenoids, haptophyta, chrysophyta, cryptophyta, cryptomonads, dinophyta, dinoflagellata, pyrmnesiophyta, bacillariophyta, xanthophyta, eustigmatophyta, raphidophyta, phaeophyta, and phytoplankton. Other vectors of the present invention are capable of stable transformation of C. reinhardtii, D. salina or H. pluvalis. Still other vectors contain nucleic acids which are biased to an organism's (e.g., C. reinhardiii) codon preference. Specific vectors of the present invention contain sequences provided herein (SEQ ID NO. 19, SEQ ID NO. 20, SEQ ID NO. 21, SEQ ID NO. 22, SEQ ID NO. 23, SEQ ID NO. 24, SEQ ID NO. 25, SEQ ID NO. 26, or SEQ ID NO. 27). [0010] Host cells comprising the vectors of the present invention are also provided. In some instances, the host cell is a non-vascular photosynthetic organism, for example, an organism classified as photosynthetic bacteria (including cyanobacteria), cyanophyta, prochlorophyta, rhodophyta, chlorophyta, heterokontophyta, tribophyta, glaucophyta, chlorarachniophytes, euglenophyta, euglenoids, haptophyta, chrysophyta, cryptophyta, cryptomonads, dinophyta, dinoflagellata, pyrmnesiophyta, bacillariophyta, xanthophyta, eustigmatophyta, raphidophyta, phaeophyta, and phytoplankton. A host cell of the present invention may also be a microalga species including, but not limited to, C. reinhardtii, D. salina or H. pluvalis. In other instances, the host cell may be one or more cells of a multicellular photosynthetic organism. For some embodiments, the host cell may be grown in the absence of light and/or in the presence of an organic carbon source. [0011] The present invention also provides compositions containing one or more exogenous biomass degrading enzymes derived from one or more non-vascular photosynthetic organisms. In some instances, these compositions may also contain elements of the non-vascular photosynthetic organisms. The ratio (w/w) of enzymes to elements of the organisms may be at least 1:10, or the elements may be found only in trace amounts. Some of the compositions comprise at least one of the following enzymes: exo-f-glucanase, endo-f3 glucanase, p-glucosidase, endoxylanase, and/or lignase; where the enzyme(s) is isolated from one or more of the following organisms: C. reinhardtii, D. salina, H. pluvalis, photosynthetic bacteria (including cyanobacteria), cyanophyta, prochlorophyta, rhodophyta, chlorophyta, heterokontophyta, tribophyta, glaucophyta, chlorarachniophytes, euglenophyta, euglenoids, haptophyta, chrysophyta, cryptophyta, cryptomonads, dinophyta, dinoflagellata, pyrmnesiophyta, bacillariophyta, xanthophyta, eustigmatophyta, raphidophyta, phaeophyta, and phytoplankton. For some embodiments, the organism may be grown in the absence of light and/or in the presence of an organic carbon source. [0012] The present invention also provides a composition containing a plurality of vectors each of which encodes a different biomass degrading enzyme and a promoter for expression of said biomass degrading enzymes in a chloroplast. Such compositions may contain multiple copies of a particular vector encoding a particular enzyme. In some instances, the vectors will contain nucleic acids encoding cellulolytic, hemicellulolytic and/or ligninolytic enzymes. More specifically, the plurality of vectors may contain vectors capable of expressing exo-D-glucanase, endo-D-glucanase, D-glucosidase, endoxylanase and/or lignase. Some of the vectors of this embodiment are capable of insertion into a chloroplast genome and such insertion can lead to disruption of the photosynthetic capability of the transformed chloroplast. Insertion of other vectors into a chloroplast genome does not disrupt photosynthetic capability of the transformed chloroplast. Some vectors provide for expression of biomass degrading enzymes which are sequestered in a transformed chloroplast. Still other vectors may contain specific sequences provided herein (SEQ ID NO. 19, SEQ ID NO. 20, SEQ ID NO. 21, SEQ ID NO. 22, or SEQ ID NO. 23, SEQ ID NO. 24, SEQ ID NO. 25, SEQ ID NO. 26, or SEQ ID NO. 27). The present invention also provides an algal cell containing the vector compositions described above and specifically provides C. reinhardtii, D. salina or H. pluvalis cells containing the vector compositions. For some embodiments, the cell may be grown in the absence of light and/or in the presence of an organic carbon source. [0013] Another vector of the present invention encodes a plurality of distinct biomass degrading enzymes and a promoter for expression of the biomass degrading enzymes in a non-vascular photosynthetic organism. The biomass degrading enzymes may be one or more of cellulollytic, hemicellulolytic or ligninolytic enzymes. In some vectors, the plurality of distinct biomass degrading enzymes is two or more of exo-p-glucanase, endo D-glucanase, D-glucosidase, lignase and endoxylanase. In some embodiments, the plurality of enzymes is operatively linked. In other embodiments, the plurality of enzymes is expressed as a functional protein complex. Insertion of some vectors into a host cell genome does not disrupt photosynthetic capability of the organism. Vectors encoding a plurality of distinct enzymes, may lead to production of enzymes which are sequestered in a chloroplast of a transformed organism. The present invention also provides an algal cell or cyanobacterial cell transformed with a vector encoding a plurality of distinct enzymes. In some instances, the algal cell is C. reinhardtii, D. salina or H. pluvalis. In other instances, the cyanobacterial cell is a species of the genus Synechocystis or the genus Synechococcus or the genus Athrospira. For some embodiments, the organism may be grown in the absence of light and/or in the presence of an organic carbon source. [0014] Yet another aspect of the present invention provides a genetically modified chloroplast producing one or more biomass degrading enzymes. Such enzymes may be cellulolytic, hemicellulolytic or ligninolytic enzymes, and more specifically, may be an exo-o-glucanase, an endo-p-glucanase, a -glucosidase, an endoxylanase, a lignase and/or combinations thereof. The one or more enzymes are be sequestered in the chloroplast in some embodiments. The present invention also provides photosynthetic organisms containing the genetically modified chloroplasts of the present invention. [0015] Yet another aspect provides a method for preparing a biomass-degrading enzyme. This method comprises the steps of (1) transforming a photosynthetic, non-vascular organism to produce or increase production of said biomass-degrading enzyme and (2) collecting the biomass-degrading enzyme from said transformed organism. Transformation may be conducted with a composition containing a plurality of different vectors encoding different biomass degrading enzymes. Transformation may also be conducted with a vector encoding a plurality of distinct biomass degrading enzymes. Any or all of the enzymes may be operatively linked to each other. In some instances, a chloroplast is transformed. This method of the invention may have one or more additional steps, including: (a) harvesting transformed organisms; (b) drying transformed organisms; (c) harvesting enzymes from a cell medium; (d) mechanically disrupting transformed organisms; or (e) chemically disrupting transformed organisms. The method may also comprise further purification of an enzyme through performance liquid chromatography. In some instances the transformed organism is an alga or a photosynthetic bacteria, e.g., cyanobacteria. For some embodiments, the organism may be grown in the absence of light and/or in the presence of an organic carbon source. [0016] Still another method of the present invention allows for preparing a biofuel. One step of this method includes treating a biomass with one or more biomass degrading enzymes derived from a photosynthetic, non vascular organism for a sufficient amount of time to degrade at least a portion of said biomass. The biofuel produced may be ethanol. The enzymes of this method may contain at least traces of said photosynthetic non vascular organism from which they are derived. Additionally, the enzymes useful for some embodiments of this method include cellulolytic, hemicellulolytic and ligninolytic enzymes. Specific enzymes useful for some aspects of this method include exo-o-glucanase, endo-p-glucanase, p-glucosidase, endoxylanase, and/or lignase. The organisms of this method may include photosynthetic bacteria (including cyanobacteria), cyanophyta, prochlorophyta, rhodophyta, chlorophyta, heterokontophyta, tribophyta, glaucophyta, chlorarachniophytes, euglenophyta, euglenoids, haptophyta, chrysophyta, cryptophyta, cryptomonads, dinophyta, dinoflagellata, pyrmnesiophyta, bacillariophyta, xanthophyta, eustigmatophyta, raphidophyta, phaeophyta, and phytoplankton. Other organisms used for this method are microalgae including, but not limited to C. reinhardrii, D. salina and H. pluvalis. For some embodiments, the organism may be grown in the absence of light and/or in the presence of an organic carbon source. Multiple types of biomass including agricultural waste, paper mill waste, corn stover, wheat stover, soy stover, switchgrass, duckweed, poplar trees, woodchips, sawdust, wet distiller grain, dray distiller grain, human waste, newspaper, recycled paper products, or human garbage may be treated with this method of the invention. Biomass may also be derived from a high-cellulose content organism, such as switchgrass or duckweed. The enzyme(s) used in this method may be liberated from the organism and this liberation may involve chemical or mechanical disruption of the cells of the organism. In an alternate embodiment, the enzyme(s) are secreted from the organism and then collected from a culture medium. The treatment of the biomass may involve a fermentation process, which may utilize a microorganism other than the organism which produced the enzyme(s). In some instances the non-vascular photosynthetic organism may be added to a saccharification tank. This method of the invention may also comprise the step of collecting the biofuel. Collection may be performed by distillation. In some instances, the biofuel is mixed with another fuel. [00171 An additional method of the present invention provides for making at least one biomass degrading enzyme by transforming a chloroplast to make a biomass degrading enzyme. The biomass degrading enzyme may be a cellulolytic enzyme, a hemicellulolytic enzyme, or a ligninolytic enzyme, and specifically may be exo-o-glucanase, endo-p-glucanase, P-glucosidase, endoxylanase, or lignase. In some instances, the biomass degrading enzyme is sequestered in the transformed chloroplast. The method may further involve disrupting, via chemical or mechanical means, the transformed chloroplast to release the biomass degrading enzyme(s). In some instances, multiple enzymes will be produced by a transformed chloroplast. The biomass degrading enzymes may be of fungal or bacterial origin, for example, exo-D-glucanase, endo-o-glucanase, $-glucosidase, endoxylanase, lignase, or a combination thereof. [0018] Yet another method of the present invention provides for screening a transformed non-vascular photosynthetic organism, by amplifying a first nucleic acid sequence from a chloroplast of said organism and amplifying a second nucleic acid sequence from said chloroplast of said organism and determining the plasmic state of said organism based on results from amplification of said first sequence and second sequence. In some instances the first and second amplifying step is performed simultaneously. The first nucleic acid sequence may be an endogenous chloroplast genome sequence and the second nucleic acid sequence may be at least partially from an exogenous nucleic acid. In some instances, a third nucleic acid sequence from the chloroplast may be amplified as a control. This third nucleic acid sequence may be a wild-type sequence that remains intact after integration of exogenous nucleic acid(s). Where this third nucleic acid is amplified, such amplification may be performed concurrently with the first or second amplifying step, or all three amplifications may be performed concurrently. For amplifications of this method, the specific primers provided herein - SEQ ID NO. 1, SEQ ID NO. 2, SEQ ID NO. 3, SEQ ID NO. 4, SEQ ID NO. 5, SEQ ID NO. 6, SEQ ID NO. 7, SEQ ID NO. 8, SEQ ID NO. 9, SEQ ID NO. 10, SEQ ID NO. 11, SEQ ID NO. 12, SEQ ID NO. 13, SEQ ID NO. 14, or SEQ ID NO. 15 - may be utilized. Amplification of the first and/or second nucleic acid may utilize more than thirty cycles of PCR. In some instances, determining the plasmic state is performed by visual analysis of products from the amplifying steps. One or more amplifications may be performed using real-time or quantitative PCR. [0019] The plasmic state determined by this method may be homoplasmy and the organism tested may be a microalga, specifically, one of the microalga species C. reinhardtii, D. salina or H. pluvalis. In this method, the organism may contain an exogenous nucleic acid which contains a gene of interest and a selectable marker. The gene of interest may encode a biomass degrading enzyme, for example a cellulolytic, hemicellulolytic or lignolytic enzyme. Specifically, the biomass degrading enzyme may be exo-$-glucanase, endo-$-glucanase, D-glucosidase, endoxylanase or lignase. Additionally, the exogenous nucleic acid may be one of the nucleic acids specifically provided herein - SEQ ID NO. 19, SEQ ID NO. 20, SEQ ID NO. 21, SEQ ID NO. 22, SEQ ID NO. 23, SEQ ID NO. 24, SEQ ID NO. 25, SEQ ID NO. 26, SEQ ID NO. 27, SEQ ID NO. 28, SEQ ID NO. 29, SEQ ID NO. 30, or SEQ ID NO. 31.

[00201 The present invention also provides a non-vascular photosynthetic organism containing a homoplasmic chloroplast population, where the chloroplast population comprises an exogenous nucleic acid and where the homoplasmic state of the chloroplast population is determined by at least two different PCR reactions. In some instances, the chloroplast population is more than one chloroplast. The non-vascular photosynthetic organism may be a microalga, specifically one of the species C. reinhardtii, D. salina or H. pluvalis. The organism may be screened using at least two different PCR reactions performed simultaneously. These PCR reactions may utilize one of the specific primers disclosed herein - SEQ ID NO. 1, SEQ ID NO. 2, SEQ ID NO. 3, SEQ ID NO. 4, SEQ ID NO. 5, SEQ ID NO. 6, SEQ ID NO. 7, SEQ ID NO. 8, SEQ ID NO. 9, SEQ ID NO. 10, SEQ ID NO. 11, SEQ ID NO. 12, SEQ ID NO. 13, SEQ ID NO. 14, or SEQ ID NO. 15. The PCR reactions may utilize more than thirty cycles. [0021] The organism may contain an exogenous nucleic acid comprising at least one gene of interest and a selectable marker. This gene may encode a biomass degrading enzyme, specifically a cellulolytic, hemicellulolytic or ligninolytic enzyme. Even more specifically, the biomass degrading enzyme may be exo P-glucanase, endo-@-glucanase, P-glucosidase, endoxylanase or lignase. The exogenous nucleic acid present in this organism of the present invention may be on of the nucleic acids specifically described herein - SEQ ID NO. 19, SEQ ID NO. 20, SEQ ID NO. 21, SEQ ID NO. 22, SEQ ID NO. 23, SEQ ID NO. 24, SEQ ID NO. 25, SEQ ID NO. 26, SEQ ID NO. 27, SEQ ID NO. 28, SEQ ID NO. 29, SEQ ID NO. 30, or SEQ ID NO. 31. [0022] Another method is provided herein for producing a genetically-modified homoplasmic non-vascular photosynthetic organism. This method involves transforming. t least one chloroplast of the organism with an exogenous nucleic acid, amplifying a first nucleic acid sequence and a second nucleic acid sequence, and determining the plasmic state of the organism based on results from the amplifying step. The first and second nucleic acid sequences may be within the chloroplast genome. Additionally, the first nucleic acid sequence may be an endogenous chloroplast sequence. The second nucleic acid sequence may be at least partially from the exogenous nucleic acid. This method may also involve amplifying a third nucleic acid sequence from the chloroplast as a control. In some instances the third nucleic acid is a wild-type sequence that remains intact after integration of an exogenous nucleic acid. This method may involve PCR using one of the specifically disclosed primers herein - SEQ ID NO. 1, SEQ ID NO. 2, SEQ ID NO. 3, SEQ ID NO. 4, SEQ ID NO. 5, SEQ ID NO. 6, SEQ ID NO. 7, SEQ ID NO. 8, SEQ ID NO. 9, SEQ ID NO. 10, SEQ ID NO. 11, SEQ ID NO. 12, SEQ ID NO. 13, SEQ ID NO. 14, or SEQ ID NO. 15. Amplification of the first and second nucleic acid sequences may utilize more than thirty cycles of PCR. The determination of plasmic state using this method may involve visual analysis of the products of the amplifying step(s). (0023] The plasmic state determined by this method may be homoplasmy and the organism may be a microalga, specifically one of the species C. reinhardtii, D. salina or H. pluvalis. The exogenous nucleic acid may contain at least one gene of interest and a selectable marker. In some instances, the gene of interest encodes a biomass degrading enzyme, specifically a cellulolytic, hemicellulolytic or ligninolytic enzyme. Even more specifically the biomass degrading enzyme may be exo-@-glucanase, endo-@-glucanase, 0 glucosidase, endoxylanase or lignase. Moreover, the exogenous nucleic acid may be one specifically described herein - SEQ ID NO. 19, SEQ ID NO. 20, SEQ ID NO. 21, SEQ ID NO. 22, SEQ ID NO. 23, SEQ ID NO. 24, SEQ ID NO. 25, SEQ ID NO. 26, SEQ ID NO. 27, SEQ ID NO. 28, SEQ ID NO. 29, SEQ ID NO. 30, or SEQ ID NO. 31. [0024] Another embodiment of the present invention is a kit for determining plasmic state of a genetically modified non-vascular photosynthetic organism. Such a kit may contain amplification primer(s) for amplifying a first nucleic acid sequence of a chloroplast genome corresponding to an endogenous sequence and amplification primer(s) for amplifying a second nucleic acid sequence of a chloroplast genome that is an introduced or non-naturally occurring sequence. A kit may also contain a PCR buffer and/or amplification primer(s) for amplifying a control nucleic acid sequence. A kit may contain one or more of the PCR primers specifically disclosed herein - SEQ ID NO. 1, SEQ ID NO. 2, SEQ ID NO. 3, SEQ ID NO. 4, SEQ ID NO. 5, SEQ [D NO. 6, SEQ ID NO. 7, SEQ ID NO. g, SEQ ID NO. 9, SEQ ID NO. 10, SEQ ID NO. 11, SEQ ID NO. 12, SEQ ID NO. 13, SEQ ID NO. 14. or SEQ ID NO. 15. The primer(s) for amplifying a first nucleic acid sequence in a kit of the present invention, may bind to at least a portion of a psbA 5'UTR, a psbA coding sequence, an psbC 5' UTR, a psbD 5' UTR, an atpA 5' UTR, or a 3HB locus. In some instances, at least one of the primer(s) for amplifying a second nucleic acid sequence will bind to at least a portion of a sequence encoding a biomass degrading enzyme, such as a cellulolytic, hemicellulolytic or ligninolytic enzyme. Specific biomass degrading enzymes encoded by the second nucleic acid may be exo-p-glucanase, endo-$ glucanase, S-glucosidase, endoxylanase or lignase. The primers may amplify at least a portion of one or more of the sequences specifically disclosed herein - SEQ ID NO. 19, SEQ ID NO. 20, SEQ ID NO. 21, SEQ ID NO. 22, SEQ ID NO. 23, SEQ ID NO. 24, SEQ ID NO. 25, SEQ ID NO. 26, SEQ ID NO. 27, SEQ ID NO. 28, SEQ ID NO. 29, SEQ ID NO. 30, or SEQ ID NO. 31. Additionally, the kit may contain instructions for use. [0024a] The present invention also provides a method for determining endoxylanase activity in a eukaryotic non-vascular photosynthetic organism, comprising obtaining a eukaryotic non-vascular photosynthetic organism having an exogenous nucleotide sequence encoding an endoxylanase; lysing the organism to obtain a lysate; adding an endoxylanase substrate to the lysate; and determining the endoxylanase activity. [0024b] The present invention also provides a method for determining endoxylanase activity in a eukaryotic non-vascular photosynthetic organism, comprising obtaining a eukaryotic non-vascular photosynthetic organism having an exogenous nucleotide sequence encoding an endoxylanase and an epitope tag; lysing the organism to obtain a lysate; clarifying the lysate to produce a clarified lysate; isolating the endoxylanase using the epitope tag; adding an endoxylanase substrate to the isolated endoxylanase; and determining the endoxylanase activity.

SUMMARY OF THE FIGURES [0025] The novel features of the invention are set forth with particularity in the appended claims. A better understanding of the features and advantages of the present invention will be obtained by reference to the following detailed description that sets forth illustrative embodiments, in which the principles of the invention are utilized, and the accompanying drawings of which: [0026] Figure 1 illustrates transformation of alga cells, selection, confirmation, and scaling of production of enzymes. [0027] Figure 2 illustrates two constructs for insertion of a gene into a chloroplast genome. [0028] Figure 3 illustrates primer pairs for PCR screening of transformants and expected band profiles for wild-type, heteroplasmic and homoplasmic strains. [0029] Figure 4 illustrates results from PCR screening and Western blot analysis of endo-p3-glucanase transformed C. reinhardtii clones. [0030] Figure 5 illustrates results from PCR screening and Western blot analysis of exo-p-glucanase transformed C. reinhardtii clones. [00311 Figure 6 illustrates results from PCR screening and Western blot analysis of P-glucosidase transformed C. reinhardrii clones. _7 A- [0032] Figure 7 illustrates results from PCR screening and Western blot analysis of endoxylanase transformed C. reinhardili clones. [0033) Figure 8 illustrates determination of the level of endo-p-glucanase protein produced by transformed C. reinhardili clones. [0034] Figure 9 is a graphic representation of an embodiment of the present invention, showing generalized constructs for insertion of multiple genes into a chloroplast genome. [00351 Figure 10 illustrates results from PCR screening and Western blot analysis of endo-p-glucanase transformed C. reinhardtii clones. [0036] Figure 11 illustrates results from PCR screening and Western blot analysis of p-glucosidase transformed C. reinhardtii clones. [0037] Figure 12 is a graphic representation of two exogenous DNA constructs for insertion into a chloroplast genome. [0038] Figure 13 is a graphic representation of two exogenous DNA constructs for insertion into a cyanobacterial genome. [0039] Figure 14 illustrates results from PCR screening and Western blot analysis of endo-p-glucanase transformed C. reinhardtii clones. [0040] Figure 15 illustrates results from PCR screening and Western blot analysis of endoxylanase transformed C. reinhardtii clones. [0041] Figure 16 illustrates results from PCR screening and Western blot analysis of exo-3-glucanase transformed C. reinhardtii clones. [0042] Figure 17 illustrates activity of bacterially-produced biomass degrading enzymes. DETAILED DESCRIPTION OF THE INVENTION [0043] Technical and scientific terms used herein have the meanings commonly understood by one of ordinary skill in the art to which the instant invention pertains, unless otherwise defined. Reference is made herein to various materials and methodologies known to those of skill in the art. Standard reference works setting forth the general principles of recombinant DNA technology include Sambrook et al., "Molecular Cloning: A Laboratory Manual", 2d ed., Cold Spring Harbor Laboratory Press, Plainview, N.Y., 1989; Kaufman et al., eds., "Handbook of Molecular and Cellular Methods in Biology and Medicine", CRC Press, Boca Raton, 1995; and McPherson, ed., "Directed Mutagenesis: A Practical Approach", IRL Press, Oxford, 1991. Standard reference literature teaching general methodologies and principles of yeast genetics useful for selected aspects of the invention include: Sherman et al. "Laboratory Course Manual Methods in Yeast Genetics", Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y., 1986 and Guthrie et al., "Guide to Yeast Genetics and Molecular Biology", Academic, New York, 1991. [0044] Where a range of values is provided, it is understood that each intervening value, to the tenth of the unit of the lower limit unless the context clearly dictates otherwise, between the upper and lower limits of that range is also specifically disclosed. Each smaller range between any stated value or intervening value in a stated range and any other stated or intervening value in that stated range is encompassed. The upper and lower limits of these smaller ranges can independently be included or excluded in the range, and each range where either, neither or both limits are included in the smaller ranges is also encompassed, subject to any specifically excluded limit in the stated range. Where the stated range includes one or both of the limits, ranges excluding either or both of those included limits are also included. [0045] The present invention relates to the production of enzymes, e.g., biomass degrading enzymes, by genetically modified organisms. Another aspect of the present invention relates to compositions and methods for using biologic material to create products, such as ethanol, using biomass degrading enzymes produced by photosynthetic microorganisms, such as, but not limited to, algae. Typically, photosynthetic organisms do not possess all of the necessary enzymes to degrade biomass. The present invention takes advantage of the ability to introduce exogenous nucleic acids into algal cells, and particularly into the chloroplasts of those cells. One advantage of using molecular biology and genetic engineering to create enzyme-expressing and/or enzymatic pathway-expressing algal strains is the potential for the production of large quantities of active enzymes. (0046] One approach to construction of a genetically manipulated strain of alga is diagramed as a flow chart in FIG. 1. As can be seen, alga cells (e.g., Chlanydomonas reinhardti, Dunaliella salina, Henatococcus pluvalis) are transformed with a nucleic acid which encodes a gene of interest, typically a biomass degrading enzyme. In some embodiments, a transformation may introduce nucleic acids into any plastid of the host alga cell (e.g., chloroplast). Transformed cells are typically plated on selective media following introduction of exogenous nucleic acids. This method may also comprise several steps for screening. Initially, a screen of primary transformants is typically conducted to determine which clones have proper insertion of the exogenous nucleic acids. Clones which show the proper integration may be patched and re-screened to ensure genetic stability. Such methodology ensures that the transformants contain the genes of interest. In many instances, such screening is performed by polymerase chain reaction (PCR); however, any other appropriate technique known in the art may be utilized. Many different methods of PCR are known in the art (e.g., nested PCR, real time PCR). For any given screen, one of skill in the art will recognize that PCR components may be varied to achieve optimal screening results. For example, magnesium concentration may need to be adjusted upwards when PCR is performed on disrupted alga cells as many such organisms have magnesium chelators. In such instances, magnesium concentration may need to be adjusted upward, or downward (compared to the standard concentration in commercially available PCR kits) by 0.1, 0.2,0.3, 0.4, 0.5, 0.6, 0.7, 0.8, 0.9, 1.0, 1.1, 1.2, 1.3, 1.4, 1.5, 1.6, 1.7, 1.8, 1.9, or 2.0 mM. Thus, after adjusting, final magnesium concentration in a PCR reaction may be, for example 0.7, 0.8, 0.9, 1.0, 1.1, 1.2, 1.3, 1.4, 1.5, 1.6, 1.7, 1.8, 1.9, 2.0, 2.1, 2.2, 2.3, 2.4, 2.5, 2.6, 2.7, 2.8, 2.9, 3.0, 3.1, 3.2, 3.3, 3.4, 3.5 mM or higher. Particular examples are utilized in the examples described herein; however, one of skill in the art will recognize that other PCR techniques may be substituted for the particular protocols described. Following screening for clones with proper integration of exogenous nucleic acids, typically clones are screened for the presence of the encoded protein. Protein expression screening typically is performed by Western blot analysis and/or enzyme activity assays. [0047] Following confirmation of nucleic acid integration and/or protein expression, selected clones may be scaled up for production of biofuels through biomass degradation, first in smaller volumes of 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, 20, 21, 22, 23, 24, 25, 26, 27, 28, 29, 30, 31, 32, 33, 34, 35, 36, 37, 38, 39, 40, 41, 42, 43, 44, 45, 46, 47, 48, 49, 50, 51, 52, 53, 54, 55, 56, 57, 58, 59, 60 61, 62, 63, 64, 65, 66, 67, 68, 69, 70, 71, 72,73, 74, 75, 76, 77, 78, 79, 80, 81, 82, 83, 84, 85, 86, 87, 88, 89, 90, 91, 92, 93, 94, 95, 96, 97, 98, 99, 100 or more liters. Following initial scaling up, larger scale degradation of biomass may be performed in larger quantities. One example of a partially closed bioreactor system is shown in FIG. 1, step 6. However, growth of the transformed strains for biomass degradation and/or biofuel production can also be accomplished in man-made structures such as ponds, aqueducts, reservoirs and/or landfills. Alternately, the strains can also be grown directly in naturally occurring bodies of water, e.g., in ocean, sea, lakes, or rivers. In some cases, transformed strains are grown near ethanol production plants or other facilities. Alternately, the biomass degrading cells may be grown near regions (e.g., electrical generating plants, concrete plants, oil refineries, other industrial facilities, cities, highways, etc.) generating CO2. As such, the methods disclosed herein further contemplate business methods for selling carbon credits to ethanol plants or other facilities or regions generating CO 2 while making or catalyzing the production of fuels by growing one or more of the modified organisms described herein near the ethanol production plant. [0048] The present invention contemplates making biomass degrading enzymes by transforming host cells (e.g., alga cells such as C. reinhardtii, D. salina, H. pluvalis and cyanobacterial cells) and/or organisms comprising host cells with nucleic acids encoding one or more different biomass degrading enzymes (e.g., cellulolytic enzymes, hemicellulolytic enzymes, xylanases, lignases and cellulases). In some embodiments, a single enzyme may be produced. For example, a cellulase which breaks down pretreated cellulose fragments into double glucose molecules (cellobiose) or a cellulase which splits cellobiose into glucose, may be produced. [0049] Some host cells may be transformed with multiple genes encoding one or more enzymes. For example, a single transformed cell may contain exogenous nucleic acids encoding an entire biodegradation pathway. One example of a pathway might include genes encoding an exo-fl-glucanase (acts on the cellulose end chain), an endo-1-glucanase (acts on the interior portion of a cellulose chain), P-glucosidase (avoids reaction inhibitors by / degrades cellobiose), and endoxylanase (acts on hemicellulose cross linking). Such cells transformed with entire pathways and/or enzymes extracted from them, can degrade certain components of biomass. Constructs may contain multiple copies of the same gene, and/or multiple genes encoding the same enzyme from different organisms, and/or multiple genes with mutations in one or more parts of the coding sequences. [0050] Alternately, biomass degradation pathways can be created by transforming host cells with the individual enzymes of the pathway and then combining the cells producing the individual enzymes. This approach allows for the combination of enzymes to more particularly match the biomass of interest by altering the relative ratios of the multiple transformed strains. For example, two times as many cells expressing the first enzyme of a pathway may be added to a mix where the first step of the reaction pathway is the limiting step. [0051] Following transformation with enzyme-encoding constructs, the host cells and/or organisms are grown. The biomass degrading enzymes may be collected from the organisms/cells. Collection may be by any means known in the art, including, but not limited to concentrating cells, mechanical or chemical disruption of cells, and purification of enzymes from cell cultures and/or cell lysates. Cells and/or organisms can be grown and then the enzyme(s) collected by any means. One method of extracting the enzyme is by harvesting the host cell or a group of host cells and then drying the host cell(s). The enzyme(s) from the dried host cell(s) are then harvested by crushing the cells to expose the enzyme. The whole product of crushed cells is then used to degrade biomass. Many methods of extracting proteins from intact cells are well known in the art, and are also contemplated herein (e.g., introducing an exogenous nucleic acid construct in which an enzyme-encoding sequence is operably linked to a sequence encoding a secretion signal - excreted enzyme is isolated from the growth medium). Following extraction of the protein from the cells/organisms and/or the surrounding medium, the protein may be purified from the crude extract such that the enzyme may comprise 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19,20, 30, 40, 50,60, 70, 80, 90,95, 99 percent or higher of the total protein. Purification steps include, but are not limited to, using HPLC, affinity columns, and antibody-based purification methods. [0052] Extracting and utilizing the biomass-degrading enzyme can also be accomplished by expressing a vector containing nucleic acids that encode a biomass production-modulation molecule in the host cell. In this embodiment, the host cell produces the biomass, and also produces a biomass-degrading enzyme. The biomass-degrading enzyme can then degrade the biomass produced by the host cell. In some instances, vector used for the production of a biomass-degrading enzyme may not be continuously active. Such vectors can comprise one or more activatable promoters and one or more biomass-degrading enzymes. Such promoters activate the production of biomass-degrading enzymes, for example, after the biomass has grown to sufficient density or reached certain maturity. [0053] A method of the invention can be performed by introducing a recombinant nucleic acid molecule into a chloroplast, wherein the recombinant nucleic acid molecule includes a first polynucleotide, which encodes at least one polypeptide (i.e., 1, 2, 3, 4, or more). In some embodiments, a polypeptide is operatively linked to a second, third, fourth, fifth, sixth, seventh, eighth, ninth, tenth and/or subsequent polypeptide. For example, several enzymes in a biodegradation pathway may be linked, either directly or indirectly, such that products produced by one enzyme in the pathway, once produced, are in close proximity to the next enzyme in the pathway. [0054] For transformation of chloroplasts, one major benefit of the present invention is the utilization of a recombinant nucleic acid construct which contains both a selectable marker and one or more genes of interest. Typically, transformation of chloroplasts is performed by co-transformation of chloroplasts with two constructs: one containing a selectable marker and a second containing the gene(s) of interest. Screening of such transformants is laborious and time consuming for multiple reasons. First, the time required to grow some transformed organisms is lengthy. Second, transformants must be screened both for presence of the selectable marker and for the presence of the gene(s) of interest. Typically, secondary screening for the gene(s) of interest is performed by Southern blot (see, e.g. PCT/US2007/072465). [00551 Constructs of the current invention (FIG. 2, FIG. 9 and FIG. 12), allow for a PCR-based screening method in which transformants can be screened using a combination of primers specific for the insert and wild-type sequences (FIG. 3, lanes: G - gene specific reaction; C - control reaction; WT - wild type reaction; M - multiplex). This methodology provides a rapid screening process and advances over older techniques. For example, selection of transformants receiving unlinked markers inherently yields a lower percentage of clones with the transgenes. Because of this, the likelihood of obtaining homoplasmic lines from a primary transformation is low. By linking the marker and the gene(s) of interest, the likelihood of obtaining transgenic clones with the transgene, especially homoplasmic clones, is improved on the first pass. Specific PCR protocols for screening transformants are detailed in the Examples below, but one of skill in the art will recognize that these protocols may be altered to provide quantitative analysis of transformants. For example, different ratios of primers for a particular reaction may be utilized to compare insert copy number to a control reaction. Such variation may be performed where the multiplex reactions (FIG. 3, row M) are run concurrently or separately. [0056] Determination of insert copy number may be important in some embodiments where an optimal level of expression of the exogenous gene(s) of interest is, in part, determined by gene copy number. For example, transformation of an alga host cell (e.g., C. reinhardtii, D. salina, H. pluvalis) which results in incorporation of the exogenous nucleic acid in less than half of the copies of the chloroplast genomes in a cell may yield little or no detectable expression of the gene(s) of interest. Alternately, incorporation of exogenous nucleic acid in all the copies of the chloroplast genomes in a cell may yield little or no detectable expression of the gene(s) of interest where there are few initial copies of the genome (e.g., quantitative PCR analysis will allow for exclusion of homoplasmic clones which have low insert copy number, and thus may not have sufficiently high production of the gene and/or polypeptide of interest). In other embodiments, there may be an optimum level of incorporation of exogenous nucleic acid. In some instances, exogenous DNA may encode a protein which, whether through transcriptional, translational, or other control mechanisms, is optimally produced when it is present in a particular range of copy number. Thus, determining the copy number of such exogenous DNA, for example by quantitative PCR, may allow selection and/or production of transformed organisms which produce protein(s) of interest at an efficient level. [0057] Additionally, recombinant nucleic acid molecules of the present invention may be operatively linked to a second and/or subsequent nucleotide sequence. For example, the nucleotide sequences encoding enzymes of a biodegradation pathway may be operatively linked such that expression of these sequences may be controlled with a single inducing stimulus or controlled by a single transcriptional activator. Such systems are similar to bacterial operons (e.g., the Escherischia coli Lac operon). However, these groupings of operatively linked nucleotide sequences in the present invention are synthetic and designed to function in plant plastids, preferably are incorporated into the chloroplast genome. [0058] As used herein, the term "operatively linked" means that two or more molecules are positioned with respect to each other such that they act as a single unit and affect a function attributable to one or both molecules or a combination thereof. For example, a polynucleotide encoding a polypeptide can be operatively linked to a transcriptional or translational regulatory element, in which case the element confers its regulatory effect on the polynucleotide similarly to the way in which the regulatory element would affect a polynucleotide sequence with which it normally is associated with in a cell. A first polynucleotide coding sequence also can be operatively linked to a second (or more) coding sequence such that a chimeric polypeptide can be expressed from the operatively linked coding sequences. The chimeric polypeptide produced from such a construct can be a fusion protein, in which the two (or more) encoded peptides are translated into a single polypeptide, i.e., are covalently bound through a peptide bond, either directly or with a short spacer region. [00591 In chloroplasts, regulation of gene expression generally occurs after transcription, and often during translation initiation. This regulation is dependent upon the chloroplast translational apparatus, as well as nuclear-encoded regulatory factors (see Barkan and Goldschmidt-Clermont, Biochemie 82:559-572, 2000; Zerges, Biochenie 82:583-601, 2000). The chloroplast translational apparatus generally resembles that in bacteria; chloroplasts contain 70S ribosomes; have mRNAs that lack 5 caps and generally do not contain 3' poly-adenylated tails (Harris et al., Microbiol. Rev. 58:700-754, 1994); and translation is inhibited in chloroplasts and in bacteria by selective agents such as chloramphenicol.

[0060] Some methods of the present invention take advantage of proper positioning of a ribosome binding sequence (RBS) with respect to a coding sequence. It has previously been noted that such placement of an RBS results in robust translation in plant chloroplasts (see U.S. Application 2004/0014174, incorporated herein by reference), and that polypeptides that an advantage of expressing polypeptides in chloroplasts is that the polypeptides do not proceed through cellular compartments typically traversed by polypeptides expressed from a nuclear gene and, therefore, are not subject to certain post-translational modifications such as glycosylation. As such, the polypeptides and protein complexes produced by some methods of the invention can be expected to be produced without such post-translational modification. [0061] The following discussion is provided by way of background only and applicant does not intend the disclosed invention to be limited, either in scope, or by theory, to the disclosure of mechanisms of chloroplast gene regulation. In chloroplasts, ribosome binding and proper translation start site selection are thought to be mediated, at least in part, by cis-acting RNA elements. One example of a potential regulator has been identified within the 5'UTR's of chloroplast mRNAs (Alexander et al., Nucl. Acids Res. 26:2265-2272, 1998; Hirose and Sugiura, EMBO J. 15:1687-1695, 1996; Mayfield et al., J. Cell Biol. 127:1537-1545, 1994; Sakamoto et al., Plant J. 6:503-512, 1994, each of which is incorporated herein by reference). These elements may interact with nuclear-encoded factors. (0062] Many chloroplast mRNAs contain elements resembling prokaryotic RBS elements (Bonham-Smith and Bourque, Nucl. Acids Res. 17:2057-2080, 1989; Ruf and Kossel, FEBS Lett. 240:41-44, 1988, each of which is incorporated herein by reference). However, the functional utility of these RBS sequences in chloroplast translation has been unclear as several studies have shown differing effects of these elements on translation (Betts and Spremulli, J. Biol. Chem. 269:26456-26465, 1994; Hirose et al., FEBS Lett. 430:257 260, 1998; Fargo et al., Mol. Gen. Genet. 257:271-282, 1998; Koo and Spremulli, J. Biol. Chem. 269:7494 7500, 1994; Rochaix, Plant Mol. Biol. 32:327-341, 1996). Interpretation of these results has been complicated by the lack of a consensus for chloroplast RBS elements, and because the mutations generated to study these putative RBS sequences may have altered the context of other important sequences within the 5'UTR. [0063] Some aspects (e.g., vectors) of the present invention may include an RBS. Such RBSs can be chemically synthesized, or can be isolated from a naturally occurring nucleic acid molecule (e.g., isolation from a chloroplast gene). In addition, to an RBS, embodiments with a 5'UTR can include transcriptional regulatory elements such as a promoter. As with RBSs utilized for the present invention, a 5'UTR may be chemically synthesized, or can be isolated from a naturally occurring nucleic acid molecule. Non-limiting examples of 5'UTRs which may be used for the present invention include, but art not limited to, an atpA 5'UTR; a psbC 5'UTR, a psbD 5'UTR, a psbA 5'UTR, a rbcL 5'UTR and/or a 16S rRNA 5'UTR. A ribonucleotide sequence may further include an initiation codon, (e.g., an AUG codon), operatively linked to an RBS. Initiation codons may be endogenous (e.g., naturally occurring in a cloned gene) or can be synthetic (e.g., inserted in a linker polypeptide or PCR primer). [0064] An isolated ribonucleotide sequence may be obtained by any method known in the art, including, but not limited to being chemically synthesized, generated using an enzymatic method, (e.g., generated from a DNA or RNA template using a DNA dependent RNA polymerase or an RNA dependent RNA polymerase). A DNA template encoding the ribonucleotide of the invention can be chemically synthesized, can be isolated from a naturally occurring DNA molecule, or can be derived from a naturally occurring DNA sequence that is modified to have the required characteristics.

[0065] The term "polynucleolide" or "nucleotide sequence" or "nucleic acid molecule" is used broadly herein to mean a sequence of two or more deoxyribonucleotides or ribonucleotides that are linked together by a phosphodiester bond. As such, the terms include RNA and DNA, which can be a gene or a portion thereof, a cDNA, a synthetic polydeoxyribonucleic acid sequence, or the like, and can be single stranded or double stranded, as well as a DNAIRNA hybrid. Furthermore, the terms as used herein include naturally occurring nucleic acid molecules, which can be isolated from a cell, as well as synthetic polynucleotides, which can be prepared, for example, by methods of chemical synthesis or by enzymatic methods such as by the polymerase chain reaction (PCR). It should be recognized that the different terms are used only for convenience of discussion so as to distinguish, for example, different components of a composition, except that the term "synthetic polynucleotide" as used herein refers to a polynucleotide that has been modified to reflect chloroplast codon usage. [0066] In general, the nucleotides comprising a polynucleotide are naturally occurring deoxyribonucleotides, such as adenine, cytosine, guanine or thymine linked to 2'-deoxyribose, or ribonucleotides such as adenine, cytosine, guanine or uracil linked to ribose. Depending on the use, however, a polynucleotide also can contain nucleotide analogs, including non-naturally occurring synthetic nucleotides or modified naturally occurring nucleotides. Nucleotide analogs are well known in the art and commercially available, as are polynucleotides containing such nucleotide analogs (Lin et al., Nucl. Acids Res. 22:5220-5234, 1994; Jellinek et al., Biochemistry 34:11363-11372, 1995; Pagratis et al., Nature Biotechnol. 15:68-73, 1997). Generally, a phosphodiester bond links the nucleotides of a polynucleotide of the present invention, however other bonds, including a thiodiester bond, a phosphorothioate bond, a peptide-like bond and any other bond known in the art may be utilized to produce synthetic polynucleotides (Tam et al.,.Nucl. Acids Res. 22:977T986, 1994; Ecker and Crooke, BioTechnology 13:351360, 1995). [0067] A polynucleotide comprising naturally occurring nucleotides and phosphodiester bonds can be chemically synthesized or can be produced using recombinant DNA methods, using an appropriate polynucleotide as a template. In comparison, a polynucleotide comprising nucleotide analogs or covalent bonds other than phosphodiester bonds generally are chemically synthesized, although an enzyme such as T7 polymerase can incorporate certain types of nucleotide analogs into a polynucleotide and, therefore, can be used to produce such a polynucleotide recombinantly from an appropriate template (Jellinek et al., supra, 1995). Polynucleotides useful for practicing a method of the present invention may be isolated from any organism. Typically, the biodegradative enzymes utilized in practicing the present invention are encoded by nucleotide sequences from bacteria or fungi. Non-limiting examples of such enzymes and their sources are shown in Table I. Such polynucleotides may be isolated and/or synthesized by any means known in the art, including, but not limited to cloning, sub-cloning, and PCR. [0068] One or more codons of an encoding polynucleotide can be biased to reflect chloroplast codon usage. Most amino acids are encoded by two or more different (degenerate) codons, and it is well recognized that various organisms utilize certain codons in preference to others. Such preferential codon usage, which also is utilized in chloroplasts, is referred to herein as "chloroplast codon usage". The codon bias of Chlamydozonas reinhardtii has been reported. See U.S. Application 2004/0014174. [0069] The term "biased," when used in reference to a codon, means that the sequence of a codon in a polynucleotide has been changed such that the codon is one that is used preferentially in the target which the bias is for, e.g., alga cells, chloroplasts, or the like. A polynucleotide that is biased for chloroplast codon usage can be synthesized de novo, or can be genetically modified using routine recombinant DNA techniques, for example, by a site directed mutagenesis method, to change one or more codons such that they are biased for chloroplast codon usage. Chloroplast codon bias can be variously skewed in different plants, including, for example, in alga chloroplasts as compared to tobacco. Generally, the chloroplast codon bias selected reflects chloroplast codon usage of the plant which is being transformed with the nucleic acids of the present invention. For example, where C. reinhardtii is the host, the chloroplast codon usage is biased to reflect alga chloroplast codon usage (about 74.6% AT bias in the third codon position). [00701 One method of the invention can be performed using a polynucleotide that encodes a first polypeptide and at least a second polypeptide. As such, the polynucleotide can encode, for example, a first polypeptide and a second polypeptide; a first polypeptide, a second polypeptide, and a third polypeptide; etc. Furthermore, any or all of the encoded polypeptides can be the same or different. The polypeptides expressed in chloroplasts of the microalga C. reinhardtil may be assembled to form functional polypeptides and protein complexes. As such, a method of the invention provides a means to produce functional protein complexes, including, for example, dimers, trimers, and tetramers, wherein the subunits of the complexes can be the same or different (e.g., homodimers or heterodimers, respectively). [0071] The term "recombinant nucleic acid molecule" is used herein to refer to a polynucleotide that is manipulated by human intervention. A recombinant nucleic acid molecule can contain two or more nucleotide sequences that are linked in a manner such that the product is not found in a cell in nature. In particular, the two or more nucleotide sequences can be operatively linked and, for example, can encode a fusion polypeptide, or can comprise an encoding nucleotide sequence and a regulatory element. A recombinant nucleic acid molecule also can be based on, but manipulated so as to be different, from a naturally occurring polynucleotide, (e.g. biased for chloroplast codon usage, insertion of a restriction enzyme site, insertion of a promoter, insertion of an origin of replication). A recombinant nucleic acid molecule may further contain a peptide tag (e.g., His-6 tag), which can facilitate identification of expression of the polypeptide in a cell. Additional tags include, for example: a FLAG epitope, a c-myc epitope; biotin; and glutathione S-transferase. Such tags can be detected by any method known in the art (e.g., anti-tag antibodies, streptavidin). Such tags may also be used to isolate the operatively linked polypeptide(s), for example by affinity chromatography. Composition: [0072] Nucleic acids [0073] The compositions herein comprise nucleic acids which encode one or more different biomass degrading enzymes and/or one or more different biomass-production modulating agent and vectors of such nucleic acids. The nucleic acids can be heterologous to a photosynthetic host cell to which they are inserted. The vector can include one or a plurality of copies of the nucleic acids which encode the biomass degrading enzymes and/or one or a plurality of copies of the nucleic acids which encode the biomass-production modulating agents. When using a plurality of copies, at least 2, 3, 4, 5, 6 7, 8, 9, or 10 copies of the nucleic acids (e.g., encoding a single biomass degrading enzyme) can be inserted into a single vector. This allows for an increased level of their production in the host cell. [0074] A recombinant nucleic acid molecule useful in a method of the invention can be contained in a vector. Furthermore, where the method is performed using a second (or more) recombinant nucleic acid molecules, the second recombinant nucleic acid molecule also can be contained in a vector, which can, but need not, be the same vector as that containing the first recombinant nucleic acid molecule. The vector can be any vector useful for introducing a polynucleotide into a chloroplast and, preferably, includes a nucleotide sequence of chloroplast genomic DNA that is sufficient to undergo homologous recombination with chloroplast genomic DNA, for example, a nucleotide sequence comprising about 400 to 1500 or more substantially contiguous nucleotides of chloroplast genomic DNA. Chloroplast vectors and methods for selecting regions of a chloroplast genome for use as a vector are well known (see, for example, Bock, J. Mol. Biol. 312:425-438, 2001; see, also, Staub and Maliga, Plant Cell 4:39-45, 1992; Kavanagh et al., Genetics 152:1111-1122, 1999, each of which is incorporated herein by reference). [0075] In some instances, such vectors include promoters. Promoters useful for the present invention may come from any source (e.g., viral, bacterial, fungal, protist, animal). The promoters contemplated herein can be specific to photosynthetic organisms, non-vascular photosynthetic organisms, and vascular photosynthetic organisms (e.g., algae, flowering plants). As used herein, the term "non-vascular photosynthetic organism," refers to any macroscopic or microscopic organism, including, but not limited to, algae, cyanobacteria and photosynthetic bacteria, which does not have a vascular system such as that found in higher plants. In some instances, the nucleic acids above are inserted into a vector that comprises a promoter of a photosynthetic organism, e.g., algae. The promoter can be a promoter for expression in a chloroplast and/or other plastid. In some instances, the nucleic acids are chloroplast based. Examples of promoters contemplated for insertion of any of the nucleic acids herein into the chloroplast include those disclosed in US Application No. 2004/0014174. The promoter can be a constitutive promoter or an inducible promoter. A promoter typically includes necessary nucleic acid sequences near the start site of transcription, (e.g., a TATA element). [0076] A "constitutive" promoter is a promoter that is active under most environmental and developmental conditions. An "inducible" promoter is a promoter that is active under environmental or developmental regulation. Examples of inducible promoters/regulatory elements include, for example, a nitrate-inducible promoter (Back et al, Plant Mol. Biol. 17:9 (1991)), or a light-inducible promoter, (Feinbaum et al, Mol Gen. Genet. 226:449 (1991); Lam and Chua, Science 248:471 (1990)), or a heat responsive promoter (Muller et al., Gene 111: 165-73 (1992)). [0077] The entire chloroplast genome of C. reinhardtii is available to the public on the world wide web, at the URL "biology.duke.edu/chlamy-genome/- chloro.html" (see "view complete genome as text file" link and "maps of the chloroplast genome" link), each of which is incorporated herein by reference (J. Maul, J. W. Lilly, and D. B. Stem, unpublished results; revised Jan. 28, 2002; to be published as GenBank Acc. No. AF396929). Generally, the nucleotide sequence of the chloroplast genomic DNA is selected such that it is not a portion of a gene, including a regulatory sequence or coding sequence, particularly a gene that, if disrupted due to the homologous recombination event, would produce a deleterious effect with respect to the chloroplast, for example, for replication of the chloroplast genome, or to a plant cell containing the chloroplast. In this respect, the website containing the C. reinhardiji chloroplast genome sequence also provides maps showing coding and non-coding regions of the chloroplast genome, thus facilitating selection of a sequence useful for constructing a vector of the invention. For example, the chloroplast vector, p322, which was used in experiments disclosed herein, is a clone extending from the Eco (Eco RI) site at about position 143.1 kb to the Xho (Xho I) site at about position 148.5 kb (see, world wide web, at the URL "biology.duke.edu/chamy-genome/chloro.html", and clicking on "maps of the chloroplast genome" link, and "140-150 kb" link; also accessible directly on world wide web at URL "biology.duke.edu/chlam y/chloro/chlorol40.html"; see, also, Example 1).

[0078] A vector utilized in the practice of the invention also can contain one or more additional nucleotide sequences that confer desirable characteristics on the vector, including, for example, sequences such as cloning sites that facilitate manipulation of the vector, regulatory elements that direct replication of the vector or transcription of nucleotide sequences contain therein, sequences that encode a selectable marker, and the like. As such, the vector can contain, for example, one or more cloning sites such as a multiple cloning site, which can, but need not, be positioned such that a heterologous polynucleotide can be inserted into the vector and operatively linked to a desired element. The vector also can contain a prokaryote origin of replication (ori), for example, an E. coli ori or a cosmid ori, thus allowing passage of the vector in a prokaryote host cell, as well as in a plant chloroplast, as desired. [00791 A regulatory element, as the term is used herein, broadly refers to a nucleotide sequence that regulates the transcription or translation of a polynucleotide or the localization of a polypeptide to which it is operatively linked. Examples include, but are not limited to, an RBS, a promoter, enhancer, transcription terminator, an initiation (start) codon, a splicing signal for intron excision and maintenance of a correct reading frame, a STOP codon, an amber or ochre codon, an IRES. Additionally, a cell compartmentalization signal (i.e., a sequence that targets a polypeptide to the cytosol, nucleus, chloroplast membrane or cell membrane). Such signals are well known in the art and have been widely reported (see, e.g., U.S. Pat. No. 5,776,689). [0080] A vector or other recombinant nucleic acid molecule may include a nucleotide sequence encoding a reporter polypeptide or other selectable marker. The term "reporter" or "selectable marker" refers to a polynucleotide (or encoded polypeptide) that confers a detectable phenotype. A reporter generally encodes a detectable polypeptide, for example, a green fluorescent protein or an enzyme such as luciferase, which, when contacted with an appropriate agent (a particular wavelength of light or luciferin, respectively) generates a signal that can be detected by eye or using appropriate instrumentation (Giacomin, Plant Sci. 116:59-72, 1996; Scikantha, J. Bacteriol. 178:121, 1996; Gerdes, FEBS Lett. 389:44-47, 1996; see, also, Jefferson, EMBO J. 6:3901-3907, 1997, fl-glucuronidase). A selectable marker generally is a molecule that, when present or expressed in a cell, provides a selective advantage (or disadvantage) to the cell containing the marker, for example, the ability to grow in the presence of an agent that otherwise would kill the cell. [0081] A selectable marker can provide a means to obtain prokaryotic cells or plant cells or both that express the marker and, therefore, can be useful as a component of a vector of the invention (see, for example, Bock, supra, 2001). Examples of selectable markers include, but are not limited to, those that confer antimetabolite resistance, for example, dihydrofolate reductase, which confers resistance to methotrexate (Reiss, Plant Physiol. (Life Sci. Adv.) 13:143-149, 1994); neomycin phosphotransferase, which confers resistance to the aminoglycosides neomycin, kanamycin and paromycin (Herrera-Estrella, EMBO J. 2:987-995, 1983), hygro, which confers resistance to hygromycin (Marsh, Gene 32:481-485, 1984), trpB, which allows cells to utilize indole in place of tryptophan; hisD, which allows cells to utilize histinol in place of histidine (Hartman, Proc. Nail. Acad. Sci., USA 85:8047, 1988); mannose-6-phosphate isomerase which allows cells to utilize mannose (WO 94/20627); ornithine decarboxylase, which confers resistance to the ornithine decarboxylase inhibitor, 2 (difluoromethyl)-DL-ornithine (DFMO; McConlogue, 1987, In: Current Communications in Molecular Biology, Cold Spring Harbor Laboratory ed.); and deaminase from Aspergillus terreus, which confers resistance to Blasticidin S (Tamura, Biosci. Biotechnol. Biochem. 59:2336-2338, 1995). Additional selectable markers include those that confer herbicide resistance, for example, phosphinothricin acetyltransferase gene, which confers resistance to phosphinothricin (White et al., Nuc. Acids Res. 18:1062, 1990; Spencer et al., Theor. Apple. Genet. 79:625-631, 1990), a mutant EPSPV-synthase, which confers glyphosate resistance (Hinchee et al., BioTechnology 91:915-922, 1998), a mutant acetolactate synthase, which confers imidazolione or sulfonylurea resistance (Lee et al., EMBO J. 7:1241-1248, 1988), a mutant psbA, which confers resistance to atrazine (Smeda et al., Plant Physiol. 103:911-917, 1993), or a mutant protoporphyrinogen oxidase (see U.S. Pat. No. 5,767,373), or other markers conferring resistance to an herbicide such as glufosinate. Selectable markers include polynucleotides that confer dihydrofolate reductase (DHFR) or neomycin resistance for eukaryotic cells and tetracycline; ampicillin resistance for prokaryotes such as E. coli; and bleomycin, gentamycin, glyphosate, hygromycin, kanamycin, methotrexate, phleomycin, phosphinotricin, spectinomycin, streptomycin, sulfonamide and sulfonylurea resistance in plants (see, for example, Maliga et al., Methods in Plant Molecular Biology, Cold Spring Harbor Laboratory Press, 1995, page 39). [00821 Reporter genes have been successfully used in chloroplasts of higher plants, and high levels of recombinant protein expression have been reported. In addition, reporter genes have been used in the chloroplast of C. reinhardtii, but, in most cases very low amounts of protein were produced. Reporter genes greatly enhance the ability to monitor gene expression in a number of biological organisms. In chloroplasts of higher plants, p-glucuronidase (uidA, Staub and Maliga, EMBO J. 12:601-606, 1993), neomycin phosphotransferase (nptlI, Carrer et al., Mol. Gen. Genet. 241:49-56, 1993), adenosyl-3-adenyltransf- erase (aadA, Svab and Maliga, Proc. Nail. Acad. Sci., USA 90:913-917, 1993), and the Aequorea victoria GFP (Sidorov et al., Plant J. 19:209-216, 1999) have been used as reporter genes (Heifetz, Biochemie 82:655-666, 2000). Each of these genes has attributes that make them useful reporters of chloroplast gene expression, such as ease of analysis, sensitivity, or the ability to examine expression in situ. Based upon these studies, other heterologous proteins have been expressed in the chloroplasts of higher plants such as Bacillus thuringiensis Cry toxins, conferring resistance to insect herbivores (Kota et al., Proc. Nail. Acad. Sci., USA 96:1840-1845, 1999), or human somatotropin (Staub et al., Nat. Biotechnol. 18:333-338, 2000), a potential biopharmaceutical. Several reporter genes have been expressed in the chloroplast of the eukaryotic green alga, C. reinhardtii, including aadA (Goldschmidt-Clermont, Nucl. Acids Res. 19:4083-4089 1991; Zerges and Rochaix, Mol. Cell Biol. 14:5268-5277, 1994), uidA (Sakamoto et al., Proc. Nail. Acad. Sci., USA 90:477 501, 19933, Ishikura et al., J. Biosci. Bioeng. 87:307-314 1999), Renilla luciferase (Minko et al., Mol. Gen. Genet. 262:421-425, 1999) and the amino glycoside phosphotransferase from Acinetobacter baumanii, aphA6 (Bateman and Purton, Mol. Gen. Genet 263:404-410, 2000). [0083] In some instances, the vectors of the present invention will contain elements such as an E. coli or S. cerevisiae origin of replication. Such features, combined with appropriate selectable markers, allows for the vector to be "shuttled" between the target host cell and the bacterial and/or yeast cell. The ability to passage a shuttle vector of the invention in a secondary host may allow for more convenient manipulation of the features of the vector. For example, a reaction mixture containing the vector and putative inserted polynucleotides of interest can be transformed into prokaryote host cells such as E. coli, amplified and collected using routine methods, and examined to identify vectors containing an insert or construct of interest. If desired, the vector can be further manipulated, for example, by performing site directed mutagenesis of the inserted polynucleotide, then again amplifying and selecting vectors having a mutated polynucleotide of interest. A shuttle vector then can be introduced into plant cell chloroplasts, wherein a polypeptide of interest can be expressed and, if desired, isolated according to a method of the invention.

[0084] A polynucleotide or recombinant nucleic acid molecule of the invention, can be introduced into plant chloroplasts using any method known in the art. A polynucleotide can be introduced into a cell by a variety of methods, which are well known in the art and selected, in part, based on the particular host cell. For example, the polynucleotide can be introduced into a plant cell using a direct gene transfer method such as electroporation or microprojectile mediated (biolistic) transformation using a particle gun, or the "glass bead method," or by pollen-mediated transformation, liposome-mediated transformation, transformation using wounded or enzyme-degraded immature embryos, or wounded or enzyme-degraded embryogenic callus (Potrykus, Ann. Rev. Plant. Physiol. Plant Mol. Biol. 42:205-225, 1991). [00851 The term "exogenous" is used herein in a comparative sense to indicate that a nucleotide sequence (or polypeptide) being referred to is from a source other than a reference source, or is linked to a second nucleotide sequence (or polypeptide) with which it is not normally associated, or is modified such that it is in a form that is not normally associated with a reference material. For example, a polynucleotide encoding an biomass degrading enzyme is heterologous with respect to a nucleotide sequence of a plant chloroplast, as are the components of a recombinant nucleic acid molecule comprising, for example, a first nucleotide sequence operatively linked to a second nucleotide sequence, as is a mutated polynucleotide introduced into a chloroplast where the mutant polynucleotide is not normally found in the chloroplast. [0086] Plastid transformation is a routine and well known method for introducing a polynucleotide into a plant cell chloroplast (see U.S. Pat. Nos. 5,451,513, 5,545,817, and 5,545,818; WO 95/16783; McBride et al., Proc. Natl. Acad. Sci., USA 91:7301-7305, 1994). In some embodiments, chloroplast transformation involves introducing regions of chloroplast DNA flanking a desired nucleotide sequence, allowing for homologous recombination of the exogenous DNA into the target chloroplast genome. In some.instances one to 1.5 kb flanking nucleotide sequences of chloroplast genomic DNA may be used. Using this method, point mutations in the chloroplast 16S rRNA and rpsl2 genes, which confer resistance to spectinomycin and streptomycin, can be utilized as selectable markers for transformation (Svab et al., Proc. Natl. Acad. Sci., USA 87:8526-8530, 1990), and can result in stable homoplasmic transformants, at a frequency of approximately one per 100 bombardments of target leaves. [0087] Microprojectile mediated transformation also can be used to introduce a polynucleotide into a plant cell chloroplast (Klein et al., Nature 327:70-73, 1987). This method utilizes microprojectiles such as gold or tungsten, which are coated with the desired polynucleotide by precipitation with calcium chloride, spermidine or polyethylene glycol. The microprojectile particles are accelerated at high speed into a plant tissue using a device such as the BIOLISTIC PD-1000 particle gun (BioRad; Hercules Calif.). Methods for the transformation using biolistic methods are well known in the art (see, e.g.; Christou, Trends in Plant Science 1:423-431, 1996). Microprojectile mediated transformation has been used, for example, to generate a variety of transgenic plant species, including cotton, tobacco, corn, hybrid poplar and papaya. Important cereal crops such as wheat, oat, barley, sorghum and rice also have been transformed using microprojectile mediated delivery (Duan et al., Nature Biotech. 14:494-498, 1996; Shimamoto, Curr. Opin. Biotech. 5:158-162, 1994). The transformation of most dicotyledonous plants is possible with the methods described above. Transformation of monocotyledonous plants also can be transformed using, for example, biolistic methods as described above, protoplast transformation, electroporation of partially permeabilized cells, introduction of DNA using glass fibers, the glass bead agitation method, and the like.

[0088] Transformation frequency may be increased by replacement of recessive rRNA or r-protein antibiotic resistance genes with a dominant selectable marker, including, but not limited to the bacterial aadA gene (Svab and Maliga, Proc. Natl. Acad. Sci., USA 90:913-917, 1993). Approximately 15 to 20 cell division cycles following transformation are generally required to reach a homoplastidic state. It is apparent to one of skill in the art that a chloroplast may contain multiple copies of its genome, and therefore, the term "homoplasmic" or "homoplasmy" refers to the state where all copies of a particular locus of interest are substantially identical. Plastid expression, in which genes are inserted by homologous recombination into all of the several thousand copies of the circular plastid genome present in each plant cell, takes advantage of the enormous copy number advantage over nuclear-expressed genes to permit expression levels that can readily exceed 10% of the total soluble plant protein. [0089] The methods of the present invention are exemplified using the microalga, C. reinhardtii. The use of microalgae to express a polypeptide or protein complex according to a method of the invention provides the advantage that large populations of the microalgae can be grown, including commercially (Cyanotech Corp.; Kailua-Kona HI), thus allowing for production and, if desired, isolation of large amounts of a desired product. However, the ability to express, for example, functional mammalian polypeptides, including protein complexes, in the chloroplasts of any plant allows for production of crops of such plants and, therefore, the ability to conveniently produce large amounts of the polypeptides. Accordingly, the methods of the invention can be practiced using any plant having chloroplasts, including, for example, macroalgae, for example, marine algae and seaweeds, as well as plants that grow in soil, for example, corn (Zea mays), Brassica sp. (e.g., B. napus, B. rapa, B. juncea), particularly those Brassica species useful as sources of seed oil, alfalfa (Medicago sativa), rice (Oryza sativa), rye (Secale cereale), sorghum (Sorghum bicolor, Sorghum vulgare), millet (e.g., pearl millet (Pennisetum glaucum), proso millet (Panicum miliaceum), foxtail millet (Setaria italica), finger millet (Eleusine coracana)), sunflower (Helianthus annuus), safflower (Carthamus tinctorius), wheat (Triticum aestivum), soybean (Glycine max), tobacco (Nicotiana tabacum), potato (Solanum tuberosum), peanuts (Arachis hypogaea), cotton (Gossypium barbadense, Gossypium hirsutum), sweet potato (Ipomoea batatus), cassaya (Manihot esculenta), coffee (Cofea spp.), coconut (Cocos nucifera), pineapple (Ananas coinosus), citrus trees (Citrus spp.), cocoa (Theobroma cacao), tea (Camellia sinensis), banana (Musa spp.), avocado (Persea ultilane), fig (Ficus casica), guava (Psidium guajava), mango (Mangifera indica), olive (Olea europaea), papaya (Carica papaya), cashew (Anacardium occidentale), macadamia (Macadamia integrifolia), almond (Prunus amygdalus), sugar beets (Beta vulgaris), sugar cane (Saccharum spp.), oats, duckweed (Lemna), barley, tomatoes (Lycopersicon esculentumn), lettuce (e.g., Lactuca sativa), green beans (Phaseolus vulgaris), lima beans (Phaseolus limensis), peas (Lathyrus spp.), and members of the genus Cucunis such as cucumber (C. sativus), cantaloupe (C. cantalupensis), and musk melon (C. melo). Ornamentals such as azalea (Rhododendron spp.), hydrangea (Macrophylla hydrangea), hibiscus (fHibiscus rosasanensis), roses (Rosa spp.), tulips (Tulipa spp.), daffodils (Narcissus spp.), petunias (Petunia hybrida), carnation (Dianthus caryophyllus), poinsettia (Euphorbia pulcherrima), and chrysanthemum are also included. Additional ornamentals useful for practicing a method of the invention include impatiens, Begonia, Pelargonium, Viola, Cyclamen, Verbena, Vinca, Tagetes, Primula, Saint Paulia, Agertum, Amaranthus, Antihirrhinum, Aquilegia, Cineraria, Clover, Cosmo, Cowpea, Dahlia, Datura, Delphinium, Gerbera, Gladiolus, Gloxinia, Hippeastrum, Mesembryanthemum, Salpiglossos, and Zinnia. Conifers that may be employed in practicing the present invention include, for example, pines such as loblolly pine (Pinus taeda), slash pine (Pinus elliotii), ponderosa pine (Pinus ponderosa), lodgepole pine (Pinus contorta), and Monterey pine (Pinus radiata), Douglas-fir (Pseudotsuga menziesii); Western hemlock (Tsuga ultilane); Sitka spruce (Picea glauca); redwood (Sequoia senipervirens); true firs such as silver fir (Abies amabilis) and balsam fir (Abies balsamea); and cedars such as Western red cedar (Thuja plicata) and Alaska yellow-cedar (Chamnaecyparis nootkatensis). [00901 Leguminous plants useful for practicing a method of the invention include beans and peas. Beans include guar, locust bean, fenugreek, soybean, garden beans, cowpea, mung bean, lima bean, fava bean, lentils, chickpea, etc. Legumes include, but are not limited to, A rachis, e.g., peanuts, Vicia, e.g., crown vetch, hairy vetch, adzuki bean, mung bean, and chickpea, Lupinus, e.g., lupine, trifolium, Phaseolus, e.g., common bean and lima bean, Pisum, e.g., field bean, Melilotus, e.g., clover, Medicago, e.g., alfalfa, Lotus, e.g., trefoil, lens, e.g., lentil, and false indigo. Preferred forage and turf grass for use in the methods of the invention include alfalfa, orchard grass, tall fescue, perennial ryegrass, creeping bent grass, and redtop. Other plants useful in the invention include Acacia, aneth, artichoke, arugula, blackberry, canola, cilantro, clementines, escarole, eucalyptus, fennel, grapefruit, honey dew, jicama, kiwifruit, lemon, lime, mushroom, nut, okra, orange, parsley, persimmon, plantain, pomegranate, poplar, radiata pine, radicchio, Southern pine, sweetgum, tangerine, triticale, vine, yams, apple, pear, quince, cherry, apricot, melon, hemp, buckwheat, grape, raspberry, chenopodium, blueberry, nectarine, peach, plum, strawberry, watermelon, eggplant, pepper, cauliflower, Brassica, e.g., broccoli, cabbage, ultilan sprouts, onion, carrot, leek, beet, broad bean, celery, radish, pumpkin, endive, gourd, garlic, snapbean, spinach, squash, turnip, ultilane, chicory, groundnut and zucchini. Thus, the compositions contemplated herein include host organisms comprising any of the above nucleic acids. The host organism can be any chloroplast-containing organism. [0091) The term "plant" is used broadly herein to refer to a eukaryotic organism containing plastids, particularly chloroplasts, and includes any such organism at any stage of development, or to part of a plant, including a plant cutting, a plant cell, a plant cell culture, a plant organ, a plant seed, and a plantlet. A plant cell is the structural and physiological unit of the plant, comprising a protoplast and a cell wall. A plant cell can be in the form of an isolated single cell or a cultured cell, or can be part of higher organized unit, for example, a plant tissue, plant organ, or plant. Thus, a plant cell can be a protoplast, a gamete producing cell, or a cell or collection of cells that can regenerate into a whole plant. As such, a seed, which comprises multiple plant cells and is capable of regenerating into a whole plant, is considered plant cell for purposes of this disclosure. A plant tissue or plant organ can be a seed, protoplast, callus, or any other groups of plant cells that is organized into a structural or functional unit. Particularly useful parts of a plant include harvestable parts and parts useful for propagation of progeny plants. A harvestable part of a plant can be any useful part of a plant, for example, flowers, pollen, seedlings, tubers, leaves, stems, fruit, seeds, roots, and the like. A part of a plant useful for propagation includes, for example, seeds, fruits, cuttings, seedlings, tubers, rootstocks, and the like. [0092] A method of the invention can generate a plant containing chloroplasts that are genetically modified to contain a stably integrated polynucleotide (Hager and Bock, Appl. Microbiol. Biotechnol. 54:302-310, 2000). Accordingly, the present invention further provides a transgenic (transplastomic) plant, e.g. C. reinhardtii, which comprises one or more chloroplasts containing a polynucleotide encoding one or more heterologous polypeptides, including polypeptides that can specifically associate to form a functional protein complex.

[00931 In some instances, transformants and/or transplastomic plants comprising a recombinant polynucleotide encoding a single enzyme of a particular biodegradative pathway (e.g., the cellulosic pathway), may be combined with transformants comprising recombinant polynucleotides encoding the other enzymes of the biodegradative pathway. For example, where a biochemical pathway utilizes four enzymes to produce a product from a substrate, four transformant lines may be combined to provide the enzymes of that pathway. Such combinations may contain as many transformant lines as is necessary to comprise a mixture of cells producing the entire enzyme pathway, or a portion thereof. Additionally, such combinations may comprise different ratios of cells of the different transformants. For example, where one enzyme of a degradative pathway is the rate limiting step in the pathway, a combination of cells may contain 2, 3, 4, 5, 6, 7, 8, 9, 10 times or higher numbers of cells producing the rate limiting enzyme. One of skill in the art will recognize that multiple combinations of ratios of transformants may be achieved through simple methods (e.g., weighing dried tranformants and combining). Alternately, individual enzymes may be isolated from the transformants (e.g., "cracking" algal transformants to isolate sequestered enzymes) and then combined following isolation. Such approaches may allow for tailoring of enzyme concentrations to different biomass or other substrate materials which may contain different relative ratios of substrates or other components. [0094] In some instances, a protein produced by a transgenic organism of the present invention is isolated after it is produced. Therefore, the present invention also contemplates a method of producing a heterologous polypeptide or protein complex in a chloroplast or in a transgenic plant which may include a step of isolating an expressed polypeptide or protein complex from the plant cell chloroplasts. As used herein, the term "isolated" or "substantially purified" means that a polypeptide or polynucleotide being referred to is in a form that is relatively free of proteins, nucleic acids, lipids, carbohydrates or other materials with which it is naturally associated. An isolated polypeptide (or polynucleotide) may constitute at least 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, 20, 21, 22, 23, 24, 25, 26, 27, 28, 29, 30, 31, 32, 33, 34, 35, 36, 37, 38, 39, 40, 41, 42, 43, 44, 45, 46, 47, 48, 49, 50, 51, 52, 53, 54, 55, 56, 57, 58, 59, 60 61, 62, 63, 64, 65, 66, 67, 68, 69, 70, 71, 72,73, 74, 75, 76, 77, 78, 79, 80, 81, 82, 83, 84, 85, 86, 87, 88, 89, 90, 91, 92, 93, 94, 95, 96, 97, 98, 99, or 100 percent of a sample. [00951 A polypeptide or protein complex can be isolated from chloroplasts using any method suitable for the particular polypeptide or protein complex, including, for example, salt fractionation methods and chromatography methods such as an affinity chromatography method using a ligand or receptor that specifically binds the polypeptide or protein complex. A determination that a polypeptide or protein complex produced according to a method of the invention is in an isolated form can be made using well known methods, for example, by performing electrophoresis and identifying the particular molecule as a relatively discrete band or the particular complex as one of a series of bands. Accordingly, the present invention also provides an isolated polypeptide or protein complex produced by a method of the invention. In some instances, an enzyme of the present invention may be produced but sequestered in the chloroplast. In such embodiments, access to the active enzyme may be had upon "cracking" the cells containing the enzyme (e.g., using mechanical, chemical, and/or biological means to disrupt the cell wall). The timing of such cracking may be planned to occur at the time the enzyme(s) produced by the cells are to be utilized to perform their enzymatic capabilities. In other instances, the enzyme may be secreted by the host cell. In such instances, the enzyme may be collected directly from the culture medium of the organism. Enzymes present in such media may be used directly, without purification, may be dried (e.g., air dried, lyophilized), and/or may be subjected to purification by any means known in the art (e.g., affinity chromatography, high performance liquid chromatography). [0096] Examples of biomass-degrading enzymes and the nucleic acids that encode those enzymes are shown in Table I. Non-limiting examples of biomass-degrading enzymes include: cellulolytic enzymes, hemicellulolytic enzymes, pectinolytic enzymes, xylanases, ligninolytic enzymes, cellulases, cellobiases, softening enzymes (e.g., endopolygalacturonase), amylases, lipases, proteases, RNAses, DNAses, inulinase, lysing enzymes, phospholipases, pectinase, pullulanase, glucose isomerase, endoxylanase, beta-xylosidase, alpha-L-arabinofuranosidase, alpha-glucoronidase, alpha-galactosidase, acetylxylan esterase, and feruloyl esterase. Examples of genes that encode such enzymes include, but are not limited to, amylases, cellulases, hemicellulases, (e.g., 0-glucosidase, endocellulase, exocellulase), exo-p-glucanase, endo-D-glucanase and xylanse (endoxylanase and exoxylanse). Examples of ligninolytic enzymes include, but are not limited to, lignin peroxidase and manganese peroxidase from Phanerochaete chryososporium. One of skill in the art will recognize that these enzymes are only a partial list of enzymes which could be used in the present invention. Table 1. Examples of Biomass-degrading enzymes # Target (family) Source AA NCBI prot. ID Exo-@-glucanase 1. CBH 1 (7) Trichoderma 514 AAQ76092 viride 2. CBH I (6) T. reesei 471 AAA72922 3. CBH 1 (7) Aspergillus 540 BAA25183 aculeatus Endo-@-glucanase 4. EG 1 (7) T. reesei 459 AAA34212 5. EG III (5) T. reesei 218 AAA34213 6. EG V (45) T. reesei 242 CAA83846 7. EGL A (12) A. niger 239 CAA11964 D-glucosidase 8. BGL 1 (3) T. reesei 744 AAA18473 9. BGL II (1) T. reesei 466 BAA74959 10. BGL 1 (3) A. niger 860 ABG46337 Endoxylanase 11. XYN I (11) T. reesei 222 CAA49293 12. XYN II (11) T. reesei 229 CAA49294 [0097] Biomass-production modulating agents include agents that increase biomass production in an organism, e.g., photosynthetic organism. [00981 Host cells/organism [0099] The present invention also contemplates a host cell transformed with one or more of the nucleic acids herein. In preferred embodiments, the host cell is photosynthetic. In some cases, the host cell is photosynthetic and non-vascular. In other cases, the host cell is photosynthetic and vascular. The host cell can be eukaryotic or prokaryotic. [00100] The host cell is transfected with a vector described herein (e.g., a vector comprising one or more biomass degrading enzymes and/or one or more biomass-production modulating agents). The vector may contain a plastid promoter or a nucleic promoter for transfecting a chloroplast or other plastid of the host cell. The vector may also encode a fusion protein or agent that selectively targets the vector product to the chloroplast or other plastid. Transfection of a host cell can occur using any method known in the art. [00101] A host organism is an organism comprising a host cell. In preferred embodiments, the host organism is photosynthetic. A photosynthetic organism is one that naturally photosynthesizes (has a plastid) or that is genetically engineered or otherwise modified to be photosynthetic. In some instances, a photosynthetic organism may be transformed with a construct of the invention which renders all or part of the photosynthetic apparatus inoperable. In some instances it is non-vascular and photosynthetic. The host cell can be prokaryotic. Examples of some prokaryotic organisms of the present invention include, but are not limited to cyanobacteria (e.g., Synechococcus, Synechocystis, Athrospira). The host organism can be unicellular or multicellular. In most embodiments, the host organism is eukaryotic (e.g. green algae). Examples of organisms contemplated herein include, but are not limited to, rhodophyta, chlorophyta, heterokontophyta, tribophyta, glaucophyta, chlorarachniophytes, euglenoids, haptophyta, cryptomonads, dinoflagellata, and phytoplankton. [001021 A host organism may be grown under conditions which permit photosynthesis, however, this is not a requirement (e.g., a host organism may be grown in the absence of light). In some instances, the host organism may be genetically modified in such a way that photosynthetic capability is diminished and/or destroyed (see examples below). In growth conditions where a host organism is not capable of photosynthesis (e.g., because of the absence of light and/or genetic modification), typically, the organism will be provided with the necessary nutrients to support growth in the absence of photosynthesis. For example, a culture medium in (or on) which an organism is grown, may be supplemented with any required nutrient, including an organic carbon source, nitrogen source, phosphorous source, vitamins, metals, lipids, nucleic acids, micronutrients, or an organism-specific requirement. Organic carbon sources includ any source of carbon which the host organism is able to metabolize including, but not limited to, acetate, simple carbohydrates (e.g., glucose, sucrose, lactose), complex carbohydrates (e.g., starch, glycogen), proteins, and lipids. One of skill in the art will recognize that not all organisms will be able to sufficiently metabolize a particular nutrient and that nutrient mixtures may need to be modified from one organism to another in order to provide the appropriate nutrient mix. 100103] A host organism can be grown on land, e.g., ponds, aqueducts, landfills, or in closed or partially closed bioreactor systems. The host organisms herein can also be grown directly in water, e.g., in ocean, sea, on lakes, rivers, reservoirs, etc. In embodiments where algae are mass-cultured, the algae can be grown in high density photobioreactors Methods of mass-culturing algae are known. For example, algae can be grown in high density photobioreactors (see, e.g., Lee et al, Biotech. Bioengineering 44:1161-1167, 1994) and other bioreactors (such as those for sewage and waste water treatments) (e.g., Sawayama et al, AppL. Micro. Biotech., 41:729-731, 1994). Additionally, algae may be mass-cultured to remove heavy metals (e.g., Wilkinson, Biotech. Letters, 11:861-864, 1989), hydrogen (e.g., U.S. Patent Application Publication No. 20030162273), and pharmaceutical compounds [00104] In some cases, host organism(s) are grown near ethanol production plants or other facilities or regions (e.g., electrical generating plants, concrete plants, oil refineries, other industrial facilities, cities, highways, etc.) generating CO 2 . As such, the methods herein contemplate business methods for selling carbon credits to ethanol plants or other facilities or regions generating CO 2 while making or catalyzing the production of fuels by growing one or more of the modified organisms described herein near the ethanol production plant. [00105] Biomass [001061 As used herein, "biomass" is any organic material. In some instances, biomass is substantially free or free of starch and simple sugars. Biomass can be broken down into starch or simple sugars that can be subsequently utilized for the production of fuel. Any cellulosic or lignocellulosic material and materials comprising cellulose, hemicellulose, lignin, starch, oligosaccharides and/or monosaccharides are also considered to be biomass. Biomass may also comprise additional components, such as protein and/or lipid. Biomass may be derived from a single source, or biomass can comprise a mixture derived from more than one source; for example, biomass could comprise a mixture of corn cobs and corn stover, or a mixture of grass and leaves. Biomass includes, but is not limited to, bioenergy crops, agricultural residues, municipal solid waste, industrial solid waste, sludge from paper manufacture, yard waste, wood and forestry waste. Examples of biomass include, but are not limited to, corn grain, corn cobs, crop residues such as corn husks, corn stover, grasses, wheat, wheat straw, barley, barley straw, hay, rice straw, switchgrass, waste paper, sugar cane bagasse, sorghum, soy, components obtained from milling of grains, trees, branches, roots, leaves, wood chips, sawdust, paper, shrubs and bushes, vegetables, fruits, flowers and animal manure. [001071 Agricultural waste is one form of biomass used for the production of fuel. Non-limiting examples of agricultural waste include corn stover, wheat stover, and soy stover. Another source of biomass in this invention is a high cellulose content organism. A high cellulose content organism is an organism whose weight is at least 30% or more attributable to biomass that is substantially free of starch or simple sugars. High cellulose content organism(s) can be selectively grown in large quantities to produce biomass, which can be degraded with biomass-degrading enzyme(s) of this invention to create starch and simple sugars. Examples of high cellulose content organisms include, but are not limited to: willow, duckweed, sugarbeets, and switchgrass. [00108] A third example of biomass comprises organisms that are genetically modified to have an increased cellulose or biomass. Such organisms are optionally photosynthetic and may comprise a host cell incorporating a vector that encodes a biomass production-modulating agent. In some instances, the same vector can encode both a biomass production-modulating agent and a biomass-degrading enzyme. In some instances, the vector encoding the biomass production-modulating agent and the vector encoding the biomass degrading enzyme are separate. [00109) Fuel Production [00110] The present invention relates to methods of producing a biofuel. Such methods comprise expressing a gene encoding a biomass-degrading enzyme in a photosynthetic organism (e.g., non-vascular). The method further comprises utilizing the biomass-degrading enzyme and breaking down biomass with the enzyme. To produce a biofuel, the method may further involve refining the degraded biomass. The final product (e.g., ethanol) may then be mixed with one or more other biofuels. [00111] The invention relates to a method of producing a biofuel comprising expressing a vector or vectors encoding a biomass-degrading enzyme, a biomass-degrading enzymatic pathway, and/or a biomass production-modulating agent in photosynthetic organism (e.g., non-vascular). In this embodiment, the host cell comprising the vector could then both make and degrade its own biomass. The method can comprise extracting only the product of the biomass degradation. In this manner, the enzyme would not have to be extracted to use for the creation of a biofuel. The production of the biofuel may further involve refining the product of the breaking down of the biomass. The production of biofuel may also involve the utilization of saccharification tanks. Such devices are well known in the art, see, for example U.S. Patent Nos. 5,114,491; 5,534,075; and 5,559,031 (each of which is herein incorporated by reference). [00112] In some embodiments, the biofuel is ethanol or other biologically produced alcohols. The refining may include a fermentation step to produce ethanol from products of biomass degradation including starch and simple sugars. Thus, refining may include using microorganisms which are capable of fermenting starch, simple sugars, and/or biomass materials, including, but not limited to Saccharonyces cerevisiae and Zymononas mobilis. [00113] The following examples merely illustrate the invention disclosed herein, but do not limit it. [00114] Examples Example 1. Production of Endo-p-glucanase in C. reinhardii [00115] In this example a nucleic acid encoding endo-p-glucanase from T. reesei was introduced into C. reinhardtii. Transforming DNA (SEQ ID NO. 20, Table 4) is shown graphically in FIG. 2A. In this instance the segment labeled "Transgene" is the endo-p-glucanase encoding gene (SEQ ID NO. 16, Table 3), the segment labeled "psbA 5' UTR" is the 5' UTR and promoter sequence for the psbA gene from C. reinhardtii, the segment labeled "psbA 3' UTR" contains the 3' UTR for the psbA gene from C. reinhardtii, and the segment labeled "Selection Marker" is the kanamycin resistance encoding gene from bacteria, which is regulated by the 5' UTR and promoter sequence for the atpA gene from C. reinhardiii and the 3' UTR sequence for the rbcL gene from from C. reinhardtii. The transgene cassette is targeted to the psbA loci of C. reinhardtii via the segments labeled "5' Homology" and "3' Homology," which are identical to sequences of DNA flanking the psbA locus on the 5' and 3' sides, respectively. All DNA manipulations carried out in the construction of this transforming DNA were essentially as described by Sambrook et al., Molecular Cloning: A Laboratory Manual (Cold Spring Harbor Laboratory Press 1989) and Cohen et al., Meth. Enzymol. 297, 192-208, 1998. [00116] For these experiments, all transformations were carried out on C. reinhardtii strain 137c (mt+). Cells were grown to late log phase (approximately 7 days) in the presence of 0.5 mM 5-fluorodeoxyuridine in TAP medium (Gorman and Levine, Proc. Nail. Acad. Sci., USA 54:1665-1669, 1965, which is incorporated herein by reference) at 23*C under constant illumination of 450 Lux on a rotary shaker set at 100 rpm. Fifty ml of cells were harvested by centrifugation at 4,000xg at 23"C for 5 min. The supernatant was decanted and cells resuspended in 4 ml TAP medium for subsequent chloroplast transformation by particle bombardment (Cohen et al., supra, 1998). All transformations were carried out under kanamycin selection (150 jig/ml) in which resistance was conferred by the gene encoded by the segment in Figure 2 labeled "Selection Marker." (Chlamydomonas Stock Center, Duke University). [00117) PCR was used to identify transformed strains. For PCR analysis, 106 algae cells (from agar plate or liquid culture) were suspended in 10 mM EDTA and heated to 95'C for 10 minutes, then cooled to near 23'C. A PCR cocktail consisting of reaction buffer, MgCI2, dNTPs, PCR primer pair(s) (Table 2 and shown graphically in FIG. 3A), DNA polymerase, and water was prepared. Algae lysate in EDTA was added to provide template for reaction. Magnesium concentration is varied to compensate for amount and concentration of algae lysate in EDTA added. Annealing temperature gradients were employed to determine optimal annealing temperature for specific primer pairs. [001181 To identify strains that contain the endo-p-glucanase gene, a primer pair was used in which one primer anneals to a site within the psbA 5'UTR (SEQ ID NO. 1) and the other primer anneals within the endo p-glucanase coding segment (SEQ ID NO. 3). Desired clones are those that yield a PCR product of expected size. To determine the degree to which the endogenous gene locus is displaced (heteroplasmic vs. homoplasmic), a PCR reaction consisting of two sets of primer pairs were employed (in the same reaction). The first pair of primers amplifies the endogenous locus targeted by the expression vector and consists of a primer that anneals within the psbA 5'UTR (SEQ ID NO. 8) and one that anneals within the psbA coding region (SEQ ID NO. 9). The second pair of primers (SEQ ID NOs. 6 and 7) amplifies a constant, or control region that is not targeted by the expression vector, so should produce a product of expected size in all cases. This reaction confirms that the absence of a PCR product from the endogenous locus did not result from cellular and/or other contaminants that inhibited the PCR reaction. Concentrations of the primer pairs are varied so that both reactions work in the same tube; however, the pair for the endogenous locus is 5X the concentration of the constant pair. The number of cycles used was >30 to increase sensitivity. The most desired clones are those that yield a product for the constant region but not for the endogenous gene locus. Desired clones are also those that give weak-intensity endogenous locus products relative to the control reaction. [00119] Results from this PCR on 96 clones were determined and the results are shown in FIG. 4. Figure 4A shows PCR results using the transgene-specific primer pair. As can be seen, multiple transformed clones are positive for insertion of the exo-p-glucanase gene (e.g. numbers 1-14). Figure 4B shows the PCR results using the primer pairs to differentiate homoplasmic from heteroplasnic clones. As can be seen, multiple transformed clones are either homoplasmic or heteroplasmic to a degree in favor of incorporation of the transgene (e.g. numbers 1-14). Unnumbered clones demonstrate the presence of wild-type psbA and, thus, were not selected for further analysis. Table 2. PCR primers. SEQ ID Use Sequence NO. 1. psbA 5' UTR forward primer GTGCTAGGTAACTAACGTTTGAT T 2. Exo-p-glucanase reverse primer AACCTTCCACGTTAGCTTGA 3. Endo-P-glucanase reverse primer GCATTAGTTGGACCACCTTG 4. pl-glucosidase reverse primer ATCACCTGAAGCAGGTTTGA 5. Endoxylanase reverse primer GCACTACCTGATGAAAAATAACC 6. Control forward primer CCGAACTGAGGTTGGGTTTA 7. Control reverse primer GGGGGAGCGAATAGGATTAG 8. psbA 5' UTR forward primer (wild-type) GGAAGGGGACGTAGGTACATAAA 9. psbA 3' reverse primer (wild-type) TTAGAACGTGTTTTGTTCCCAAT 10. psbC 5' UTR forward primer TGGTACAAGAGGATTTTTGTTGTT II. psbD 5' UTR forward primer AAATTTAACGTAACGATGAGTTG 12. arpA 5' UTR forward primer CCCCTTACGGGCAAGTAAAC SEQ ID Use Sequence NO. 13. 3HB forward primer (wild-type) CTCGCCTATCGGCTAACAAG 14. 3HB forward primer (wild-type) CACAAGAAGCAACCCCTTGA [00120] To ensure that the presence of the endo-p-glucanase-encoding gene led to expression of the endo-fp glucanase protein, a Western blot was performed. Approximately 1x10 8 algae cells were collected from TAP agar medium and suspended in 0.5 ml of lysis buffer (750 mM Tris, pH=8.0, 15% sucrose, 100 mM beta mercaptoethanol). Cells were lysed by sonication (5x30sec at 15% power). Lysate was mixed 1:1 with loading buffer (5% SDS, 5% beta-mercaptoethanol, 30% sucrose, bromophenol blue) and proteins were separated by SDS-PAGE, followed by transfer to PVDF membrane. The membrane was blocked with TBST + 5% dried, nonfat milk at 23*C for 30 min, incubated with anti-FLAG antibody (diluted 1:1,000 in TBST + 5% dried, nonfat milk) at 4*C for 10 hours, washed three times with TBST, incubated with horseradish-linked anti-mouse antibody (diluted 1:10,000 in TBST + 5% dried, nonfat milk) at 23*C for 1 hour, and washed three times with TBST. Proteins were visualized with chemiluminescent detection. Results from multiple clones (FIG. 4C) show that expression of the endo-o-glucanase gene in C. reinhardtii cells resulted in production of the protein. [00121] Cultivation of C. reinhardtii transformants for expression of endo-f-glucanase was carried out in liquid TAP medium at 23*C under constant illumination of 5,000 Lux on a rotary shaker set at 100 rpm, unless stated otherwise. Cultures were maintained at a density of 1x10 7 cells per ml for at least 48 hr prior to harvest. [00122] To determine if the endo-o-glucanase produced by transformed alga cells was functional, endo-0 glucanase activity was tested using a filter paper assay (Xiao et al., Biotech. Bioengineer. 88, 832-37, 2004). Briefly, 500 ml of algae cell culture was harvested by centrifugation at 4000xg at 4*C for 15 min. The supernatant was decanted and the cells resuspended in 10 ml of lysis buffer (100 mM Tris-HCI, pH=8.0, 300 mM NaCl, 2% Tween-20). Cells were lysed by sonication (10x30sec at 35% power). Lysate was clarified by centrifugation at 14,000xg at 4'C for 1 hour. The supernatant was removed and incubated with anti-FLAG antibody-conjugated agarose resin at 4'C for 10 hours. Resin was separated from the lysate by gravity filtration and washed 3x with wash buffer ((100 mM Tris-HCI, pH=8.0, 300 mM NaCI, 2% Tween-20). Endo p-glucanase was eluted by incubation of the resin with elution buffer (TBS, 250 ug/ml FLAG peptide). Results from Western blot analysis of samples collect after each step (FIG. 4D) show that the endo-p-glucanase protein was isolated. A 20 pl aliquot of diluted enzyme was added into wells containing 40 pl of 50 mM NaAc buffer and a filter paper disk. After 60 minutes incubation at 50*C, 120 p1 of DNS was added to each reaction and incubated at 95"C for 5 minutes. Finally, a 36 pl aliquot of each sample was transferred to the wells of a flat-bottom plate containing 160 pl water. The absorbance at 540 nm was measured. The results for two transformed strains indicated that the isolated enzyme was functional (absorbance of 0.33 and 0.28). Example 2. Production of Exo-p-glucanase in C. reinhardtii [00123] In this example a nucleic acid encoding exo-J-glucanase from T. viride was introduced into C. reinhardtii. Transforming DNA (SEQ ID NO. 19, Table 4) is shown graphically in FIG. 2A. In this instance the segment labeled "Transgene" is the exo-p-glucanase encoding gene (SEQ ID NO. 15, Table 3), the segment labeled "psbA 5' UTR" is the 5' UTR and promoter sequence for the psbA gene from C. reinhardiii, the segment labeled "psbA 3' UTR" contains the 3' UTR for the psbA gene from C. reinhardtii, and the segment labeled "Selection Marker" is the kanamycin resistance encoding gene from bacteria, which is regulated by the 5' UTR and promoter sequence for the atpA gene from C. reinhardrii and the 3' UTR sequence for the rbcL gene from from C. reinhardtii. The transgene cassette is targeted to the psbA loci of C. reinhardtii via the segments labeled "5' Homology" and "3' Homology," which are identical to sequences of DNA flanking the psbA locus on the 5' and 3' sides, respectively. All DNA manipulations carried out in the construction of this transforming DNA were essentially as described by Sambrook et al., Molecular Cloning: A Laboratory Manual (Cold Spring Harbor Laboratory Press 1989) and Cohen et al., Meth. Enzynol. 297, 192-208, 1998. [00124) For these experiments, all transformations were carried out on C. reinhardtii strain 137c (mt+). Cells were grown to late log phase (approximately 7 days) in the presence of 0.5 mM 5-fluorodeoxyuridine in TAP medium (Gorman and Levine, Proc. Natl. A cad. Sci., USA 54:1665-1669, 1965, which is incorporated herein by reference) at 23*C under constant illumination of 450 Lux on a rotary shaker set at 100 rpm. Fifty ml of cells were harvested by centrifugation at 4,000xg at 23*C for 5 min. The supernatant was decanted and cells resuspended in 4 ml TAP medium for subsequent chloroplast transformation by particle bombardment (Cohen et al., supra, 1998). All transformations were carried out under kanamycin selection (150 pg/ml), in which resistance was conferred by the gene encoded by the segment in Figure 2 labeled "Selection Marker." (Chlamydomonas Stock Center, Duke University). [00125] PCR was used to identify transformed strains. For PCR analysis, 106 algae cells (from agar plate or liquid culture) were suspended in 10 mM EDTA and heated to 95*C for 10 minutes, then cooled to near 23'C. A PCR cocktail consisting of reaction buffer, MgCI2, dNTPs, PCR primer pair(s) (Table 2 and shown graphically in FIG. 3A), DNA polymerase, and water was prepared. Algae lysate in EDTA.was added to.. provide template for reaction. Magnesium concentration is varied to compensate for amount and concentration of algae lysate in EDTA added. Annealing temperature gradients were employed to determine optimal annealing temperature for specific primer pairs. [00126] To identify strains that contain the exo-o-glucanase gene, a primer pair was used in which one primer anneals to a site within the psbA 5'UTR (SEQ ID NO. 1) and the other primer anneals within the exo-s glucanase coding segment (SEQ ID NO. 2). Desired clones are those that yield a PCR product of expected size. To determine the degree to which the endogenous gene locus is displaced (heteroplasmic vs. homoplasmic), a PCR reaction consisting of two sets of primer pairs were employed (in the same reaction). The first pair of primers amplifies the endogenous locus targeted by the expression vector and consists of a primer that anneals within the psbA 5'UTR (SEQ ID NO. 8) and one that anneals within the psbA coding region (SEQ ID NO. 9). The second pair of primers (SEQ ID NOs. 6 and 7) amplifies a constant, or control region that is not targeted by the expression vector, so should produce a product of expected size in all cases. This reaction confirms that the absence of a PCR product from the endogenous locus did not result from cellular and/or other contaminants that inhibited the PCR reaction. Concentrations of the primer pairs are varied so that both reactions work in the same tube; however, the pair for the endogenous locus is 5X the concentration of the constant pair. The number of cycles used was >30 to increase sensitivity. The most desired clones are those that yield a product for the constant region but not for the endogenous gene locus. Desired clones are also those that give weak-intensity endogenous locus products relative to the control reaction.

[00127] Results from this PCR on 96 clones were determined and the results are shown in FIG. 5. Figure 5A shows PCR results using the transgene-specific primer pair. As can be seen, multiple transformed clones are positive for insertion of the endo-p-glucanase gene (e.g. numbers 1-14). Figure 4B shows the PCR results using the primer pairs to differentiate homoplasmic from heteroplasmic clones. As can be seen, multiple transformed clones are either homoplasmic or heteroplasmic to a degree in favor of incorporation of the transgene (e.g. numbers 1-14). Unnumbered clones demonstrate the presence of wild-type psbA and, thus, were not selected for further analysis. [00128] To. ensure that the presence of the exo-p-glucanase-encoding gene led to expression of the exo-p glucanase protein, a Western blot was performed. Approximately Ix108 algae cells were collected from TAP agar medium and suspended in 0.5 ml of lysis buffer (750 mM Tris, pH=8.0, 15% sucrose, 100 mM beta mercaptoethanol). Cells were lysed by sonication (5x30sec at 15% power). Lysate was mixed 1:1 with loading buffer (5% SDS, 5% beta-mercaptoethanol, 30% sucrose, bromophenol blue) and proteins were separated by SDS-PAGE, followed by transfer to PVDF membrane. The membrane was blocked with TBST + 5% dried, nonfat milk at 23*C for 30 min, incubated with anti-FLAG antibody (diluted 1:1,000 in TBST + 5% dried, nonfat milk) at 4"C for 10 hours, washed three times with TBST, incubated with horseradish-linked anti-mouse antibody (diluted 1:10,000 in TBST + 5% dried, nonfat milk) at 23*C for 1 hour, and washed three times with TBST. Proteins were visualized with chemiluminescent detection. Results from multiple clones (FIG. SC) show that expression of the exo-p-glucanase gene in C. reinhardrii cells resulted in production of the protein. [00129] Cultivation of C. reinhardtii transformants for expression of endo-pl-glucanase was carried out in liquid TAP medium at 23*C under constant illumination of 5,000 Lux on a rotary shaker set at 100 rpm, unless stated otherwise. Cultures were maintained at a density of Ix107 cells per ml for at least 48 hr prior to harvest. [00130] To determine if the exo-p-glucanase produced by transformed alga cells was functional, exo-p glucanase activity was tested using a filter paper assay (Xiao et al., Biotech. Bioengineer. 88, 832-37, 2004). Briefly, 500 ml of algae cell culture was harvested by centrifugation at 4000xg at 4*C for 15 min. The supernatant was decanted and the cells resuspended in 10 ml of lysis buffer (100 mM Tris-HCI, pH=8.0, 300 mM NaCl, 2% Tween-20). Cells were lysed by sonication (10x30sec at 35% power). Lysate was clarified by centrifugation at 14,000xg at 4'C for 1 hour. The supernatant was removed and incubated with anti-FLAG antibody-conjugated agarose resin at 4'C for 10 hours. Resin was separated from the lysate by gravity filtration and washed 3x with wash buffer (100 mM Tris-HCl, pH=8.0, 300 mM NaCl, 2% Tween-20). Exo-p glucanase was eluted by incubation of the resin with elution buffer (TBS, 250 ug/ml FLAG peptide). Results from Western blot analysis of samples collect after each step (FIG. 5D) show that the exo- -glucanase protein was isolated. A 20 pl aliquot of diluted enzyme was added into wells containing 40 pl of 50 mM NaAc buffer and a filter paper disk. After 60 minutes incubation at 50*C, 120 pl of DNS was added to each reaction and incubated at 95*C for 5 minutes. Finally, a 36 pi aliquot of each sample was transferred to the wells of a flat bottom plate containing 160 pl water. The absorbance at 540 nm was measured. The results for two transformed strains indicated that the isolated enzyme was functional (absorbance of 0.20 and 0.45). Example 3. Production of 3-glucosidase in C. reinhardii [00131] In this example a nucleic acid encoding p-glucosidase from T. reesei was introduced into C. reinhardrii. Transforming DNA (SEQ ID NO. 21, Table 4) is shown graphically in FIG. 2A. The amino acid sequence encoded by this gene is shown in Table 3. In this instance the segment labeled "Transgene" is the pglucosidase encoding gene (SEQ ID NO. 17, Table 3), the segment labeled "psbA 5' UTR" is the 5' UTR and promoter sequence for the psbA gene from C. reinhardtii, the segment labeled "psbA 3' UTR" contains the 3' UTR for the psbA gene from C. reinhardtii, and the segment labeled "Selection Marker" is the kanamycin resistance encoding gene from bacteria, which is regulated by the 5' UTR and promoter sequence for the arpA gene from C. reinhardtii and the 3' UTR sequence for the rbcL gene from from C. reinhardiii. The transgene cassette is targeted to the psbA loci of C. reinhardtii via the segments labeled "5' Homology" and "3' Homology," which are identical to sequences of DNA flanking the psbA locus on the 5' and 3' sides, respectively. All DNA manipulations carried out in the construction of this transforming DNA were essentially as described by Sambrook et al., Molecular Cloning: A Laboratory Manual (Cold Spring Harbor Laboratory Press 1989) and Cohen et al., Meth. Enzymol. 297, 192-208, 1998. [00132] For these experiments, all transformations were carried out on C. reinhardiii strain 137c (mt+). Cells were grown to late log phase (approximately 7 days) in the presence of 0.5 mM 5-fluorodeoxyuridine in TAP medium (Gorman and Levine, Proc. Natd. Acad. Sci., USA 54:1665-1669, 1965, which is incorporated herein by reference) at 23*C under constant illumination of 450 Lux on a rotary shaker set at 100 rpm. Fifty ml of cells were harvested by centrifugation at 4,000xg at 23*C for 5 min. The supernatant was decanted and cells resuspended in 4 ml TAP medium for subsequent chloroplast transformation by particle bombardment (Cohen et al., supra, 1998). All transformations were carried out under kanamycin selection (150 pg/ml), in which resistance was conferred by the gene encoded by the segment in Figure 2 labeled "Selection Marker." (Chlamydomonas Stock Center, Duke University). [001331 PCR was used to identify transformed strains. For PCR analysis, 106 algae cells (from agar plate or liquid culture) were suspended in 10 mM EDTA and heated to 95'C for 10 minutes, then cooled to near 23'C. A PCR cocktail consisting of reaction buffer, MgCI2, dNTPs, PCR primer pair(s) (Table 2 and shown graphically in FIG. 3A), DNA polymerase, and water was prepared. Algae lysate in EDTA was added to provide template for reaction. Magnesium concentration is varied to compensate for amount and concentration of algae lysate in EDTA added. Annealing temperature gradients were employed to determine optimal annealing temperature for specific primer pairs. [00134] To identify strains that contain the p-glucosidase gene, a primer pair was used in which one primer anneals to a site within the psbA 5'UTR (SEQ ID NO. 1) and the other primer anneals within the p glucosidase coding segment (SEQ ID NO. 4). Desired clones are those that yield a PCR product of expected size. To determine the degree to which the endogenous gene locus is displaced (heteroplasmic vs. homoplasmic), a PCR reaction consisting of two sets of primer pairs were employed (in the same reaction). The first pair of primers amplifies the endogenous locus targeted by the expression vector and consists of a primer that anneals within the psbA 5'UTR (SEQ ID NO. 8) and one that anneals within the psbA coding region (SEQ ID NO. 9). The second pair of primers (SEQ ID NOs. 6 and 7) amplifies a constant, or control region that is not targeted by the expression vector, so should produce a product of expected size in all cases. This reaction confirms that the absence of a PCR product from the endogenous locus did not result from cellular and/or other contaminants that inhibited the PCR reaction. Concentrations of the primer pairs are varied so that both reactions work in the same tube; however, the pair for the endogenous locus is 5X the concentration of the constant pair. The number of cycles used was >30 to increase sensitivity. The most desired clones are those that yield a product for the constant region but not for the endogenous gene locus.

Desired clones are also those that give weak-intensity endogenous locus products relative to the control reaction. [00135] Results from this PCR on 96 clones were determined and the results are shown in FIG. 6. Figure 6A shows PCR results using the transgene-specific primer pair. As can be seen, multiple transformed clones are positive for insertion of the endo-p-glucanase gene (e.g. numbers 1-9). Figure 6B shows the PCR results using the primer pairs to differentiate homoplasmic from heteroplasmic clones. As can be seen, multiple transformed clones are either homoplasmic or heteroplasmic to a degree in favor of incorporation of the transgene (e.g. numbers 1-9). Unnumbered clones demonstrate the presence of wild-type psbA and, thus, were not selected for further analysis. [00136] To ensure that the presence of the -glucosidase-encoding gene led to expression of the p-glucosidase protein, a Western blot was performed. Approximately Ix 108 algae cells were collected from TAP agar medium and suspended in 0.5 ml of lysis buffer (750 mM Tris, pH=8.0, 15% sucrose, 100 mM beta mercaptoethanol). Cells were lysed by sonication (5x30sec at 15% power). Lysate was mixed 1:1 with loading buffer (5% SDS, 5% beta-mercaptoethanol, 30% sucrose, bromophenol blue) and proteins were separated by SDS-PAGE, followed by transfer to PVDF membrane. The membrane was blocked with TBST + 5% dried, nonfat milk at 23*C for 30 min, incubated with anti-FLAG antibody (diluted 1:1,000 in TBST + 5% dried, nonfat milk) at 4*C for 10 hours, washed three times with TBST, incubated with horseradish-linked anti-mouse antibody (diluted 1:10,000 in TBST + 5% dried, nonfat milk) at 23*C for 1 hour, and washed three times with TBST. Proteins were visualized with chemiluminescent detection. Results from multiple clones (FIG. 6C) show that expression of the 0-glucosidase gene in C. reinhardtii cells resulted in production of the protein. [001371 To determine if the p-glucosidase produced by transformed alga cells was functional, p-glucosidase activity was tested using an enzyme function assay. Briefly, 500 ml of algae cell culture was harvested by centrifugation at 4000xg at 4*C for 15 min. The supernatant was decanted and the cells resuspended in 10 ml of lysis buffer (100 mM Tris-HCl, pH=8.0, 300 mM NaCl, 2% Tween-20). Cells were lysed by sonication (10x30sec at 35% power). Lysate was clarified by centrifugation at 14,00Oxg at 4'C for 1 hour. The supernatant was removed and incubated with anti-FLAG antibody-conjugated agarose resin at 4'C for 10 hours. Resin was separated from the lysate by gravity filtration and washed 3x with wash buffer ((100 mM Tris-HCl, pH=8.0, 300 mM NaCl, 2% Tween-20). s-glucosidase was eluted by incubation of the resin with elution buffer (TBS, 250 ug/ml FLAG peptide). Western blot analysis of samples collect after each step (FIG. 6D) show that the p-glucosidase protein was isolated. For each sample tested, 50 p1 of p-Nitrophenyl-/3-D glucoside (substrate), 90 Vl of 0.1 M sodium acetate buffer (pH 4.8), and 10 pl enzyme was added to a microplate well. The reaction was incubated at 50'C for one hour and then the reaction was stopped with a glycine buffer. The absorbance of the liberated p-nitrophenol was measured at 430 nm. The results for two transformed strains indicated that the isolated enzyme was functional (absorbance of 0.157 and 0.284). Example 4. Production of Endoxylanase in C. reinhardtii [00138] In this example a nucleic acid encoding endoxylanase from T. reesei was introduced into C. reinhardtii. Transforming DNA (SEQ ID NO. 22, Table 4) is shown graphically in FIG. 2A. The amino acid sequence encoded by this gene is shown in Table 3. In this instance the segment labeled "Transgene" is the endoxylanase encoding gene (SEQ ID NO. 18, Table 3), the segment labeled "psbA 5' UTR" is the 5' UTR and promoter sequence for the psbA gene from C. reinhardtii, the segment labeled "psbA 3' UTR" contains the 3' UTR for the psbA gene from C. reinhardtii, and the segment labeled "Selection Marker" is the kanamycin resistance encoding gene from bacteria, which is regulated by the 5' UTR and promoter sequence for the atpA gene from C. reinhardii and the 3' UTR sequence for the rbcL gene from from C. reinhardtii. The transgene cassette is targeted to the psbA loci of C. reinhardiji via the segments labeled "5' Homology" and "3' Homology," which are identical to sequences of DNA flanking the psbA locus on the 5' and 3' sides, respectively. All DNA manipulations carried out in the construction of this transforming DNA were essentially as described by Sambrook et al., Molecular Cloning: A Laboratory Manual (Cold Spring Harbor Laboratory Press 1989) and Cohen et al., Meih. Enzymol. 297, 192-208, 1998. [00139] For these experiments, all transformations were carried out on C. reinhardtii strain 137c (mt+). Cells were grown to late log phase (approximately 7 days) in the presence of 0.5 mM 5-fluorodeoxyuridine in TAP medium (Gorman and Levine, Proc. NatL. Acad. Sci., USA 54:1665-1669, 1965, which is incorporated herein by reference) at 23*C under constant illumination of 450 Lux on a rotary shaker set at 100 rpm. Fifty ml of cells were harvested by centrifugation at 4,000xg at 23"C for 5 min. The supernatant was decanted and cells resuspended in 4 ml TAP medium for subsequent chloroplast transformation by particle bombardment (Cohen et al., supra, 1998). All transformations were carried out under kanamycin selection (150 pg/ml), in which resistance was conferred by the gene encoded by the segment in Figure 2 labeled "Selection Marker." (Chlamydomonas Stock Center, Duke University). [00140] PCR was used to identify transformed strains. For PCR analysis, 106 algae cells (from agar plate or liquid culture) were suspended in 10 mM EDTA and heated to 95'C for 10 minutes, then cooled to near 23'C. A PCR cocktail consisting of reaction buffer, MgCl2, dNTPs, PCR primer pair(s) (Table 2 and shown graphically in FIG. 3A), DNA polymerase, and water was prepared. Algae lysate in EDTA was added to provide template for reaction. Magnesium concentration is varied to compensate for amount and concentration of algae lysate in EDTA added. Annealing temperature gradients were employed to determine optimal annealing temperature for specific primer pairs. [001411 To identify strains that contain the endoxylanase gene, a primer pair was used in which one primer anneals to a site within the psbA 5'UTR (SEQ ID NO. 1) and the other primer anneals within the endoxylanase coding segment (SEQ ID NO. 5). Desired clones are those that yield a PCR product of expected size. To determine the degree to which the endogenous gene locus is displaced (heteroplasmic vs. homoplasmic), a PCR reaction consisting of two sets of primer pairs were employed (in the same reaction). The first pair of primers amplifies the endogenous locus targeted by the expression vector and consists of a primer that anneals within the psbA 5'UTR (SEQ ID NO. 8) and one that anneals within the psbA coding region (SEQ ID NO. 9). The second pair of primers (SEQ ID NOs. 6 and 7) amplifies a constant, or control region that is not targeted by the expression vector, so should produce a product of expected size in all cases. This reaction confirms that the absence of a PCR product from the endogenous locus did not result from cellular and/or other contaminants that inhibited the PCR reaction. Concentrations of the primer pairs are varied so that both reactions work in the same tube; however, the pair for the endogenous locus is 5X the concentration of the constant pair. The number of cycles used was >30 to increase sensitivity. The most desired clones are those that yield a product for the constant region but not for the endogenous gene locus. Desired clones are also those that give weak-intensity endogenous locus products relative to the control reaction.

[00142] Results from this PCR on 96 clones were determined and the results are shown in FIG. 7. Figure 7A shows PCR results using the transgene-specific primer pair. As can be seen, multiple transformed clones are positive for insertion of the endo-p-glucanase gene (e.g. numbers 1-9). Figure 7B shows the PCR results using the primer pairs to differentiate homoplasmic from heteroplasmic clones. As can be seen, multiple transformed clones are either homoplasmic or heteroplasmic to a degree in favor of incorporation of the transgene (e.g. numbers 1-9). Unnumbered clones demonstrate the presence of wild-type psbA and, thus, were not selected for further analysis. [00143] To ensure that the presence of the endoxylanase-encoding gene led to expression of the endoxylanase protein, a Western blot was performed. Approximately lx108 algae cells were collected from TAP agar medium and suspended in 0.5 ml of lysis buffer (750 mM Tris, pH=8.0, 15% sucrose, 100 mM beta mercaptoethanol). Cells were lysed by sonication (5x30sec at 15% power). Lysate was mixed 1:1 with loading buffer (5% SDS, 5% beta-mercaptoethanol, 30% sucrose, bromophenol blue) and proteins were separated by SDS-PAGE, followed by transfer to PVDF membrane. The membrane was blocked with TBST + 5% dried, nonfat milk at 23*C for 30 min, incubated with anti-FLAG antibody (diluted 1:1,000 in TBST + 5% dried, nonfat milk) at 4*C for 10 hours, washed three times with TBST, incubated with horseradish-linked anti-mouse antibody (diluted 1:10,000 in TBST + 5% dried, nonfat milk) at 23*C for 1 hour, and washed three times with TBST. Proteins were visualized with chemiluminescent detection. Results from multiple clones (FIG. 7C) show that expression of the endoxylanase gene in C. reinhardtii cells resulted in production of the protein. [00144] To determine if the endoxylanase produced by transformed alga cells was functional, endoxylanase activity was tested using an enzyme function assay. Briefly, 500 ml of algae cell culture was harvested by centrifugation at 4000xg at 4*C for 15 min. The supernatant was decanted and the cells resuspended in 10 ml of lysis buffer (100 mM Tris-HCI, pH=8.0, 300 mM NaCl, 2% Tween-20). Cells were lysed by sonication (10x30sec at 35% power). Lysate was clarified by centrifugation at 14,000xg at 4'C for I hour. The supernatant was removed and incubated with anti-FLAG antibody-conjugated agarose resin at 4'C for 10 hours. Resin was separated from the lysate by gravity filtration and washed 3x with wash buffer ((100 mM Tris-HCI, pH=8.0, 300 mM NaCl, 2% Tween-20). Endoxylanase was eluted by incubation of the resin with elution buffer (TBS, 250 ug/mI FLAG peptide). Results from Western blot analysis of samples collect after each step (FIG. 7D) show that the Endoxylanase protein was isolated. To test for enzyme function, 0.5 ml aliquots of diluted enzyme preparation were added to glass test tubes and equilibrated at 40'C for 5 minutes. A Xylazyme AX test tablet (Megazyme) was added to initiate the reaction. After 30 minutes, the reaction was terminated by adding 10 ml Trizma base solution with vigorous stirring. The tubes were incubated at room temperature for 5 minutes and the reaction was stirred again. The reaction was then filtered through a Whatman No. 1 (9 cm) filter circle. The filtrate was then clarified by microcentrifugation. The absorbance of the filtrate was measured at 590 nm. The results indicate that, for crude enzyme extracts from two different clones, endoxylanase activity was present (absorbance of 0.974 and 0.488). Example 5. Determination of level of protein expression in a C. reinhardtii strain producing exogneous endo-p-glucanase. [001451 Western blot analysis of proteins was done as follows. Approximately lx108 algae cells were collected from liquid cultures growing in TAP medium at 23*C under constant illumination of 5,000 Lux on a rotary shaker set at 100 rpm. Cells were suspended in 0.5 ml of lysis buffer (750 mM Tris, pH=8.0, 15% sucrose, 100 mM beta-mercaptoethanol) and lysed by sonication (5x30sec at 15% power). Lysates were centrifuged at 14,000 RPM for 15 minutes at 4'C and the supernatant was collected. Total soluble protein concentrations were determined using BioRad's protein assay reagent. The sample concentrations were then normalized to one another. The FLAG control protein was a FLAG tagged bacterial alkaline phosphatase protein standard (Sigma-Aldrich, St. Louis, Mo). Lysate was mixed 1:1 with loading buffer (5% SDS, 5% beta-mercaptoethanol, 30% sucrose, bromophenol blue) and proteins were separated by SDS-PAGE, followed by transfer to PVDF membrane. The membrane was blocked with TBST + 5% dried, nonfat milk at 23*C for 30 min, incubated with anti-FLAG antibody (diluted 1:1,000 in TBST + 5% dried, nonfat milk) at 4"C for 10 hours, washed three times with TBST, incubated with horseradish-linked anti-mouse antibody (diluted 1:10,000 in TBST + 5% dried, nonfat milk) at 23"C for 1 hour, and washed three times with TBST. Proteins were visualized with chemiluminescent detection. [00146] To ascertain the level of cellulase accumulating in the transformants under different growth conditions, we carried out the titration shown in FIG. 8. Five, ten and twenty pg of total protein from a transformant expressing endo-B-glucanase (BD5-26) were separated along with 10, 50, 100 and 200 ug of a control protein. Both proteins contain the FLAG epitope tag on their carboxy terminus, thus a direct comparison can be made between the two proteins to determine expression levels. A comparison of the signal intensity between the 5 ug samples form either 24 or 48 hours growth, show a signal greater than the 50 ng control peptide and close in intensity to the 100 ng sample. A 1% total protein expression level would equal 1/100 or 50 ng of a 5 ug sample. The intensity here shows a signal equal to a level of twice that, or 100 ng in the 5 ug sample which is equal to 2% of total protein. Table 3. Amino Acid Sequences of Cellulolytic Enzymes. SEQ Sequence Source LD NO. 15 MVPYRKLAVISAFLATARAQSACTLQSETHPPLTWQKCSSGGTCTQQTGSVVIDANWRWTHATNSSTNCYDGNTWSST Exo- LCPDNErCAKNCCLDGAAYASTYGVTrSGNSLSIGFVTQSAQKNVGARLYLMASDTTYQEFTLLGNEFSFDVDVSQLPC glucanase GLNGALYFVSMDADGGfVSKYFNTAGAKYGTGYCDSQCPTDLKFNGQANVEGWEPSSNNANTGIGGHGSCCSEMD.w from T EANSISEALTPHPCTrVGQEICEGDGCGGTYSDNRYGGTCDPDGCDWDPYRLGNTSFYGPGSSFrLDlrKKLTVVTQFET viride SGAINRYYVQNGVTFQQPNAELGSYSGNGLNDDYCTAEEAEFGGSSFSDKGGLTQFKKATSGGMVLVMSLWDDYYAN MLWLDSTYPTNETSSTPGAVRGSCSTSSGVPAQVESQSPNAKVTFSNIKFGPIGSTGDPSGGNPPGGNPPGT1TIRPATIT GSSPGPTQSHYGQCGGIGYSGPTVCASGTTCQVLNPYYSQCLGTGENLYFQGSGGGGSDYKDDDDKGTG 16 MVPNKSVAPLLLAASILYGGAVAQQTVWGQCGGIGWSGPTNCAPGSACSTLNPYYAQCIPGATrTSTRPPSGPTTrRA Endo- TSTSSSTPPTSSGVRFAGVNIAGFDFGCTrDGTCVTSKVYPPLKNFGSNNYPDGGQMQHFVNEDGMTIFRLPVGWQYLV glucanase NNNLGGNLDSTSISKYDQLVQGCLSLGAYCIVDIHNYARWNGGIIGQGGPTNAQFrSLWSQLASKYASQSRVWFGIMNEP rrom T. HDVNINTWAATVQEVVTARNAGATSQFISLPGNDWQSAGAFISDGSAAALSQVTNPDGSTrNLFDVHKYLDSDNSGTHA reesei ECTrNNIDGAFSPLATWLRQNNRQAILTETGGGNVQSCIQDMCQQIQYLNQNSDVYLGYVGWGAGSFDSTYVLTETPTSSG NSWTDTSLVSSCLARKGTGENLYFQGSGGGGSDYKDDDDKGTG 17 MVPLPKDFQWGFATAAYQEGAVDQDGRGPSIWDTFCAQPGKIADGSSGVTACDSYNRTAEDIALLKSLGAKSYRFSISWS p-gluco RIlPEGGRGDAVNQAGIDHYVKFVDDLLDAGITPFITLFHWDLPEGLHQRYGGLLNRTEFPLDFENYARVMFRALPKVRNWI sidase TFNEPLCSAIPGYGSGTFAPGRQSTSEPWTVGHNILVAHGRAVKAYRDDFKPASGDGQIGIVLNGDFrYPWDAADPADKEA from T. AERRLEFFrAWFADPIYLGDYPASMRKQLGDRLPTFTPEERALVHGSNDFYGMNHYTSNYIRHRSSPASADDTVGNVDVLFT reesei NKQGNCIGPETQSPWLRPCAAGFRDFLVWISKRYGYPPIYVTENGTSIKGESDLPKEKILEDDFRVKYYNEYIRAMVTAVELD GVNVKGYFAWSLMDNFEWADGYVTRFGVTYVDYENGQKRFPKKSAKSLKPLFDELIAAAGTGENLYFQGSGGGGSDYKDD DDKGTG 18 MVPVSFTSLLAASPPSRASCRPAAEVESVAVEKRQTEQPGTGYNNGYFYSYWNDGHGGVTYTNGPGGQFSVNWSNSGNFVG Endo GKGWQPGTKNKVINFSGSYNPNGNSYLSVYGWSRNPLIEYYIVENFGTYNPSTGATKLGEVTSDGSVYDIYRTQRVNQPSIIG xylanase TATFYQYWSVRRNHRSSGSVNTANHFNAWAQQGLTLGTMDYQIVAVEGYFSSGSASITVSGTGENLYQGSGGGGSDYKDD from T. DDKGTG reesei Example 6. Construction of a C. reinhardtii strain transformed with multiple biodegradative enzyme encoding genes [00147] In this example a strain containing multiple biomass degrading (BD) enzyme-encoding genes using two separate constructs is described. One of skill in the art will realize that such an approach is provided merely by way of example. Transformation of a strain with a single construct containing all the genes of interest is performed generally as described in prior examples. An example of constructs which could be used to transform such a strain is shown in FIG. 9. As can be seen in the figure, two polynucleotides are constructed for the delivery of multiple genes into a host alga cell. The upper construct contains three enzyme-coding sequences (FIG. 9 BD-5, BD- 1, and BD-9). The lower construct contains three enzyme coding sequences (FIG. 9 BD-2, BD-4, and BD-l 1). The numbers used in this figure are meant only to indicate that different enzymes are encoded by each gene. In some instances, the genes encode different enzymes in one or more biomass degrading pathways. In other instances, one or more of the genes encode the same enzyme, but one may be a mutated form or some may be from multiple organisms. Both constructs contain terminal regions which have homology to the C. reinhardtii genome to facilitate integration into the chloroplast genome. Proper transformation, integration, protein production and protein function is analyzed as described above. [00148] Each construct contains a selectable marker (FIG. 9 Marker I and Marker II). The C. reinhardtii cells are transformed as described above. Introduction of the two constructs can be by co-transformation with both constructs. In such instances, potential transformants are selected by growth on TAP medium supplemented with substances which will select for the presence of both markers (e.g., streptomycin and kanamycin resistance). [00149] The genes of both constructs may be placed under control of a single transcriptional control, in essence introducing a synthetic operon ("chloroperon") into the chloroplasts of the alga cells. Such an approach allows for an entire pathway to be engineered into a chloroplast. Alternately, the separate constructs may be placed under control of different transcriptional regulators. Additionally, each gene so introduced may be placed under control of different transcriptional regulators. Example 7. Construction of a C. reinhardtii strain transformed with a construct that does not disrupt photosynthetic capability [00150] In this example a nucleic acid encoding endo-p-glucanase from T. reesei was introduced into C. reinhardtii. Transforming DNA (SEQ ID NO. 30, Table 4) is shown graphically in FIG. 2B. In this instance the segment labeled "Transgene" is the endo--glucanase encoding gene (SEQ ID NO. 16, Table 3), the segment labeled 5' UTR is the 5' UTR and promoter sequence for the psbD gene from C. reinhardtii, the segment labeled 3' UTR contains the 3' UTR for the psbA gene from C. reinhardtii, and the segment labeled "Selection Marker" is the kanamycin resistance encoding gene from bacteria, which is regulated by the 5' UTR and promoter sequence for the atpA gene from C. reinhardtii and the 3' UTR sequence for the rbcL gene from C. reinhardiii. The transgene cassette is targeted to the 3HB locus of C. reinhardtii via the segments labeled "5' Homology" and "3' Homology," which are identical to sequences of DNA flanking the 3HB locus on the 5' and 3' sides, respectively. All DNA manipulations carried out in the construction of this transforming DNA were essentially as described by Sambrook et al., Molecular Cloning: A Laboratory Manual (Cold Spring Harbor Laboratory Press 1989) and Cohen et al., Meth. Enzymol. 297, 192-208, 1998.

[00151] For these experiments, all transformations were carried out on C. reinhardtii strain 137c (mt+). Cells were grown to late log phase (approximately 7 days) in the presence of 0.5 mM 5-fluorodeoxyuridine in TAP medium (Gorman and Levine, Proc. Nat!. Acad. Sci., USA 54:1665-1669, 1965, which is incorporated herein by reference) at 23 0 C under constant illumination of 450 Lux on a rotary shaker set at 100 rpm. Fifty ml of cells were harvested by centrifugation at 4,000xg at 23*C for 5 min. The supernatant was decanted and cells resuspended in 4 ml TAP medium for subsequent chloroplast transformation by particle bombardment (Cohen et al., supra, 1998). All transformations were carried out under kanamycin selection (100 pg/ml), in which resistance was conferred by the gene encoded by the segment in Figure 2B labeled "Selection Marker." (Chlamydomonas Stock Center, Duke University). [00152] PCR was used to identify transformed strains. For PCR analysis, 106 algae cells (from agar plate or liquid culture) were suspended in 10 mM EDTA and heated to 95*C for 10 minutes, then cooled to near 23'C. A PCR cocktail consisting of reaction buffer, MgCI2, dNTPs, PCR primer pair(s) (Table 2 and shown graphically in FIG. 3B), DNA polymerase, and water was prepared. Algae lysate in EDTA was added to provide template for reaction. Magnesium concentration is varied to compensate for amount and concentration of algae lysate in EDTA added. Annealing temperature gradients were employed to determine optimal annealing temperature for specific primer pairs. [00153] To identify strains that contain the endo-p-glucanase gene, a primer pair was used in which one primer anneals to a site within the psbD 5'UTR (SEQ ID NO. 11) and the other primer anneals within the endo-p-glucanase coding segment (SEQ ID NO. 3). Desired clones are those that yield a PCR product of expected size. To determine the degree to which the endogenous gene locus is displaced (heteroplasmic vs. homoplasmic), a PCR reaction consisting of two sets of primer pairs were employed (in the same reaction). The first pair of primers amplifies the endogenous locus targeted by the expression vector (SEQ ID NOs. 13 and 14). The second pair of primers (SEQ ID NOs. 6 and 7) amplifies a constant, or control region that is not targeted by the expression vector, so should produce a product of expected size in all cases. This reaction confirms that the absence of a PCR product from the endogenous locus did not result from cellular and/or other contaminants that inhibited the PCR reaction. Concentrations of the primer pairs are varied so that both reactions work in the same tube; however, the pair for the endogenous locus is 5X the concentration of the constant pair. The number of cycles used was >30 to increase sensitivity. The most desired clones are those that yield a product for the constant region but not for the endogenous gene locus. Desired clones are also those that give weak-intensity endogenous locus products relative to the control reaction. [00154] Results from this PCR on 96 clones were determined and the results are shown in FIG. 14. Figure 14A shows PCR results using the transgene-specific primer pair. As can be seen, multiple transformed clones are positive for insertion of the endo-p-glucanase gene (e.g. numbers 1, 4, and 14). Figure 14B shows the PCR results using the primer pairs to differentiate homoplasmic from heteroplasmic clones. As can be seen, multiple transformed clones are either homoplasmic or heteroplasmic to a degree in favor of incorporation of the transgene (e.g. numbers 1, 4, and 14). Unnumbered clones demonstrate the presence of wild-type psbA and, thus, were not selected for further analysis. [001551 To ensure that the presence of the endo-p-glucanase-encoding gene led to expression of the endo-p glucanase protein, a Western blot was performed. Approximately lx108 algae cells were collected from TAP agar medium and suspended in 0.5 ml of lysis buffer (750 mM Tris, pH=8.0, 15% sucrose, 100 mM beta mercaptoethanol). Cells were lysed by sonication (5x30sec at 15% power). Lysate was mixed 1:1 with loading buffer (5% SDS, 5% beta-mercaptoethanol, 30% sucrose, bromophenol blue) and proteins were separated by SDS-PAGE, followed by transfer to PVDF membrane. The membrane was blocked with TBST + 5% dried, nonfat milk at 23*C for 30 min, incubated with anti-FLAG antibody (diluted 1:1,000 in TBST + 5% dried, nonfat milk) at 4*C for 10 hours, washed three times with TBST, incubated with horseradish-linked anti-mouse antibody (diluted 1:10,000 in TBST + 5% dried, nonfat milk) at 23*C for 1 hour, and washed three times with TBST. Proteins were visualized with chemiluminescent detection. Results from multiple clones (FIG. 14C) show that expression of the endo-p-glucanase gene in C. reinhardrii cells resulted in production of the protein. [00156] Similar results were seen (FIG. 15) with a similar construct containing the endoxylanase gene from T. reesei (SEQ ID NO. 31, Table 4). The construct containing the endoxylanase gene is depicted in FIG. 2B. In this instance the segment labeled "Transgene" is the endoxylanase encoding gene (SEQ ID NO. 18, Table 3), the segment labeled 5' UTR is the 5' UTR and promoter sequence for the psbD gene from C. reinhardiji, the segment labeled 3' UTR contains the 3' UTR for the psbA gene from C. reinhardtii, and the segment labeled "Selection Marker" is the kanamycin resistance encoding gene from bacteria, which is regulated by the 5' UTR and promoter sequence for the atpA gene from C. reinhardiii and the 3' UTR sequence for the rbcL gene from from C. reinhardiii. The transgene cassette is targeted to the 3HB locus of C. reinhardtii via the segments labeled "5' Homology" and "3' Homology," which are identical to sequences of DNA flanking the 3HB locus on the 5' and 3' sides, respectively. All DNA manipulations carried out in the construction of this transforming DNA were essentially as described by Sambrook et al., Molecular Cloning: A Laboratory Manual (Cold Spring Harbor Laboratory Press 1989) and Cohen et al., Meth. Enzymol. 297, 192-208, 1998. [001571 FIG. 15A shows PCR using the gene-specific primer pair. As can be seen, multiple transformed clones are positive for insertion of the endoxylanase gene. Figure 15B shows the PCR results using the primer pairs to differentiate homoplasmic from heteroplasmic clones. As can be seen, multiple transformed clones are either homoplasmic or heteroplasmic to a degree in favor of incorporation of the transgene. Unnumbered clones demonstrate the presence of wild-type psbA and, thus, were not selected for further analysis. Western blot analysis demonstrating protein expression is demonstrated in FIG. 15C. [00158] Similar results were seen (FIG. 16) with a similar construct containing the exo-p-glucanase gene from T. viride (SEQ ID NO. 29, Table 4). The construct containing the exo-p-glucanase gene is depicted in FIG. 2B. In this instance the segment labeled "Transgene" is the exo-p-glucanase encoding gene (SEQ ID NO. 15, Table 3), the segment labeled 5' UTR is the 5' UTR and promoter sequence for the psbD gene from C. reinhardtii, the segment labeled 3' UTR contains the 3' UTR for the psbA gene from C. reinhardtii, and the segment labeled "Selection Marker" is the kanamycin resistance encoding gene from bacteria, which is regulated by the 5' UTR and promoter sequence for the atpA gene from C. reinhardtii and the 3' UTR sequence for the rbcL gene from from C. reinhardtii. The transgene cassette is targeted to the 3HB locus of C. reinhardiii via the segments labeled "5' Homology" and "3' Homology," which are identical to sequences of DNA flanking the 3HB locus on the 5' and 3' sides, respectively. All DNA manipulations carried out in the construction of this transforming DNA were essentially as described by Sambrook et al., Molecular Cloning: A Laboratory Manual (Cold Spring Harbor Laboratory Press 1989) and Cohen et al., Meth. EnzymoL. 297, 192-208, 1998. [00159] FIG. 16A shows PCR using the gene-specific primer pair. As can be seen, multiple transformed clones are positive for insertion of the endoxylanase gene. Figure 16B shows the PCR results using the primer pairs to differentiate homoplasmic from heteroplasmic clones. As can be seen, multiple transformed clones are either homoplasmic or heteroplasmic to a degree in favor of incorporation of the transgene. Unnumbered clones demonstrate the presence of wild-type psbA and, thus, were not selected for further analysis. Western blot analysis demonstrating protein expression is demonstrated in FIG. 16C. Table 4. Vector Sequences SEQ ID Sequence Use NO. GCACTTCGGGGAAATGTGCGCGGAACCCCTATfTGTITATITTICTAAATACATr Exo-p CAAATATGTATCCGCTCATGAGACAATAACCCTGATAAATGCTTCAATAATATTGA glucanase AAAAGGAAGAGTATGAGTATTCAACATCCGTGTCGCCCTATrCCCITITI-GCG insertion GCATIrGCCTTCCTGTFITGCTCACCCAGAAACGCTGGTGAAAGTAAAAGATGCT cassette GAAGATCAGTTGGGTGCACGAGTGGGT-rACATCGAACTGGATCTCAACAGCGGTAA GATCCTTGAGAGTTCGCCCCGAAGAACGTITrCCAATGATGAGCAC1TTTAAAGT TCTGCTATGTGGCGCGGTATTATCCCGTATTGACGCCGGGCAAGAGCAACTCGGTC GCCGCATACACTATrCTCAGAATGACTTGGTTGAGTACTCACCAGTCACAGAAAAG BD01) CATCTTACGGATGGCATGACAGTAAGAGAATTATGCAGTGCTGCCATAACCATGAG TGATAACACTGCGGCCAACTrACTCTGACAACGATCGGAGGACCGAAGGAGCTAA CCGCTI ITIGCACAACATGGGGGATCATGTAACTCGCCTTGATCGTTGGGAACCGG AGCTGAATGAAGCCATACCAAACGACGAGCGTGACACCACGATGCCTGTAGCAAT GGCAACAACGTTGCGCAAACTATTAACTGGCGAACTACTrACTCTAGCTrCCCGGC AACAATfAATAGACTGGATGGAGGCGGATAAAGTTGCAGGACCACTTCTGCGCTCG - GCCCTTCCGGCTGGCTGGTTITATGCTGATAAATCTGGAGCCGGTGAGCGTGGGTCT CGCGGTATCATTGCAGCACTGGGGCCAGATGGTAAGCCCTCCCGTATCGTAGTITATC TACACGACGGGGAGTCAGGCAACTATGGATGAACGAAATAGACAGATCGCTGAGA TAGGTGCCTCACTGATrAAGCATTGGTAACTGTCAGACCAAGTITACTCATATATAC 1TTAGATrGATTTAAAACTfCA1TFITAATITAAAAGGATCTAGGTGAAGATCCTITr TGATAATCTCATGACCAAAATCCCTrAACGTGAGTITCGTICCACTGAGCGTCAGA CCCCGTAGAAAAGATCAAAGGATCTrCT1GAGATCClTITlCTGCGCGTAATCTG CTGCTTGCAAACAAAAAAACCACCGCTACCAGCGGTGGTGTTGCCGGATCAAG AGCTACCAACTC1 ITT-CCGAAGGTAACTGGCTTCAGCAGAGCGCAGATACCAAAT ACTGTCCTTCTAGTGTAGCCGTAGTAGGCCACCACTTCAAGAACTCTGTAGCACCG CCTACATACCTCGCTCTGCTAATCCTGTfACCAGTGGCTGCTGCCAGTGGCGATAAG TCGTGTCTrACCGGGTrGGACTCAAGACGATAGTrACCGGATAAGGCGCAGCGGTC GGGCTGAACGGGGGGTTCGTGCACACAGCCCAGCTTGGAGCGAACGACCTACACC GAACTGAGATACCTACAGCGTGAGCTATGAGAAAGCGCCACGCTrCCCGAAGGGA GAAAGGCGGACAGGTATCCGGTAAGCGGCAGGGTCGGAACAGGAGAGCGCACGAG GGAGCTTCCAGGGGGAAACGCCTGGTATCTITATAGTCCTGTCGGGTTTCGCCACCT CTGACTTGAGCGTCGAITrGTGATGCTCGTCAGGGGGGCGGAGCCTATGGAAAA ACGCCAGCAACGCGGCCTITr1 ACGGTTCCTGGCC1I1'GCTGGCCTITIGCTCACAT GTrCTTTCCTGCGTTATCCCCTGATTCTGTGGATAACCGTATACCGCCMGAGTGA GCTGATACCGCTCGCCGCAGCCGAACGACCGAGCGCAGCGAGTCAGTGAGCGAGG AAGCGGAAGAGCGCCCAATACGCAAACCGCCTCTCCCCGCGCGTTGGCCGATTCAT TAATGCAGCTGGCACGACAGGTr7CCCGACTGGAAAGCGGGCAGTGAGCGCAACG SEQ ID Sequence Use NO. ___ CAArTAATGTGAGTAGCTCACTCATAGGCACCCCAGG'ACACT~rATGCTTC CGGCTCGTATGTrGTGTGGAAnrGTGAGCGGATAACAATmCACACAGGAAACAGC TATGACCATGA'FIACGCCAAGCTCGAAATI'AACCCTCACTAAAGGGAACAAAAGCT GGAGCTCCACCGCGGTGGCGGCCGCTCTAGCACTAGTGGATCGCCCGGGCTGCAGG A ATTCcatattagataaacgatcaagcagcagaattagctttattagaacaacttgtaaag aatgatgtaccaatgccgcgcatt gtgaacaaatattaatgcttcialaaciatacatcgatgaagaacatg agtggttaac;;ngtatgatattgtaatagaiataaaggattaatataaa cctcttagacgcaatctaatgtcaacaatctgtaaatgctatttctCaatataatcccaaagatttttataatactgagacttcCaacctta cttgtttttattttgtagttacaflttcactcacgtaagacatggaatgaggcaggacgttagtcgatattta~caccttaagtttacttgc ccaataatgagcctcgtalattatgcggtcaccgcattaatcagaaaaa acttcggagtatat~tatccactaatatttatattaggcagttggcaggcaacaatataatttgtcccgtaggggacgcccgaagg ggaaggggaagaaggcagtgcctcgcctatcggctaacaagttttggagtatataaccgcctacaggtaacitaaagaacatttgtta cccgtaggggtttatacttctattgcttcttctgaacaataaaatggtttgtgtggtctgggctaggaaacttgtaacaagtgtagtgtcgcttc cgcttccctcgggacgtccccttcgggtaagtaaacttaggagtattaaatcgggacgtccccttcgtaaataatttcagtggacgtcc ccttacgggacgccagtagacgtcagtggcagttgcctcgcctatcggctaacaagttcctcggagtatataaatatagaatgtttacatact cctaagmtacttgcctcctcggagatataaatatcccgaaggggaaggaggacgccagtggcagtgtaccgccactgcctgcttcctc cttcggagtatgtaaaccccttcgggcaactaaagtttatcgcagtatataaatataggcagttggcaggcaactgccacgacgcctatttt aatactccgaaggaggcagttggcaggcaactgccactgacgtcccgtaagggtaaggggaCgtccactggcgtcccgtaaggggaag gggacgtaggtacataatgtgctaggtaactaacgtttgattttttgtggtaaaatatgtaccatgcttttaatagaagcttgaatttataaatt aaaatatttttacaatattttacggagaaattaaaactttaaaaaaattaacatATGGTACCATATCGTAAACTTGCTGT TA1TAGTGCTTTCTI'AGCTACTGCTCGTGCACAGTCAGCATGTACC1TACAATCTGA AACTCATCCTCCA7AACATGGCAAAAATGrCTCAGGAGGTACTGTACACAACA AACTGGCTCTGTAGTAATflGATGCTAACTGGCGTTGGACACATGCCACTAATAGTTC AACTAATIXJ11TATGACGGTAATACflGGTCATCAACACT!T7GTCCCGATAACGAAAC TrGTGCTAAAAATGTGTTAGATGGTGCAGCTACGC1TCAAC11'ACGGCGTTAC TACATCAGGTAACTCATATCAATnGG1TTCGTGACTCAATCAGCACAAAAAAATGT AGGCGCACGT1TATAC1TAATGGCAAGTGACACAACCTATCAAGAA1TACATrA1T AGGTAATGAGTTCAG1TTCGACGTAGATGTGAGTCAArrACCATGTGG1TI'AAATGG TGCTCTITA1TTCGTCAATGGACGCTGATGGCGGTGTAAGCAAATATCCTACTAA TACAGCAGGTGCTAAATACGGAACAGCCTAn7GTGAUrCTCAGTGTCCTCGTGA1lI' AAAGTfrATAACGGTCAAGCTAACGTGGAAGGTTGGGAACCAAGTAGTAATAATG CAAATACTGGAATTGGTGGTCACGGATC317GTTG11?CTGAAATGGATA'TIFGGGAAG CTAAT-rCAATTAGTGAAGCATrAACTCCACATCCTTGTACTACCGTTGGCCAAGAAA TrGTGAAGGCGACGGTTGCGGTGGAACATACAGTGATAACCGT7rAT3GTGGTACA TGTGATCCTGATGGCTGCGA1TGGGACCCATATCGTITAGGAAATACATC1TFIAT GGACCAGGAAGTTCATTCACATTAGATACAACTAAAAAG1TAACAGTTTfACACA GTrTCGAAACTAGCGGTGCTATrAATCG'FrATrACGTGCAAAATGGTGTAACrTPCA ACAACCAAATGCAGAATTAGG11-CTrATTCTGGTAACGGCCTrAATGACGA11'ATTG TACAGCAGAAGAAGCAGAATTI'GGTGGTAGCAGCTTCTCAGATAAAGGTGG1TAA CTCAATTCAAGAAAGCAACATCAGGTGGTATGG1TTrAGT1TATGTCATTATGGGATG ACTAT1ATGCTAATATGTlATGGTI'AGATAGTACATATCCTACAAACGAAACTTCAA GCACTCCTGGTGCTG11TCGTGGFFCATGTTCAACYTCAAGTGGTGTACCTGCTCAAG TTGAAAGCCAAAGTCCTAATGCAAAAGTAACn=AGTAATATCAAAT1GGTCCA S§E-Q ID Sequence Use NO. AnGGCTCTACAGGCGATCCTTCAGGTGGTAATCCACCAGGTGGAAATCCACCTGG CACCACTACAACACGTCGTCCTGCTACTACCACAGGTCT-CTCCTGGACCAACACA ATCTCATTACGGTCAATGTGGTGGTATrGGT-ATCAGGTCCAACTGTGTGTGCATC AGGAACTACATGTCAAG I IAAATCCATA~rATAGCCAATGTmAGGTACCGGTGA AAACTTATACTTTCAAGGCTCAGGTGGCGGTGGAAGTGAnrACAAAGATGATGATG ATAGACGTATTGctgtcatattaccacatattttaataaaac ggttaaccatacctggtttattttagttagtttaacacttttcatatatatatacttaatagctactaggcagttggcaggacg~ccccttac gggacaatgtatt~ttgttgcctgccaactgcctaatataaatattagtggactccccttccccttacgggcaagLaacttagggattLa tgctccgttaggaggcaaataaattttagtggcagtgcctCgcctatcggctaacaagtccttcggagtataat1atcctgccaactgcc gatatttatatactaggcagtggcggtaccactcgacGGATCCTACGTAATCGATGAACGATCCCAT7 TTATAACTGGTCTCAAAATACCTATAAACCCATTGTrCTTCTC1T=AGCTCTAAGAA CAATCAAMATAAATATATATrTATGCTATAATATAAATACTATATAAATAC ATT-rACCT1TATAAATACATfACCTTTI=AATTGCATGA'TrI'AATGC'7AT GCACT A1ATCTAAC-7AGAC' CrTGAA~ ATATICCTAACAAAGCAATCGGCGTCATAAAC17AGflGCUACGACGCCTGTG GACGTCCCCCCCTCCCCTrACGGGCAAGTAAACnAGGGAn=AATGCAATAAAT AAATT7GTCCTC1TCGGGCAAATGAATTITAGTAMTAAATATGACAAGGGTGAACC ATATM TACATACTCATATT M TGA M AC7 TTrAAAATTCTCGAGAAAGATrAAAAATAAACTI1AATCTIATIAT= TCI= gagatgcattatacatacgaaacttaacaaaatgtatgctg atgttattctttaatcgaaataltgaaacttttttttaagcgatctagcactttatatacaagaccacatacagtgtctctgtgaagcgaaa. atgttgagttggctctctgagaaattaaaggtgcctgaactcatcatgactttcaggatgagcagtttgaatttatgatcactaaagcgatcaat gcaaaaccaatttcagcgcttttttacagaccaagaattgcttgctatctatggaggcactcatctgttaattcaattgctattattgattg tccattcatttcaaacattgatcatcggttaaaagagtcaaattttttattgat2c~aaactcctgacgatatagatcaagatgatttKacaCLg aattatggggagaccataaaacttacctaagtctatggaatgagttaaccgagactcgtgttgaagaagattgg~tttttcatggcgatatc acggatagtaatatttLatagaaaattcaatgaatttatttagaccttggtcgtgctgggttagcagatgaattgtagatatatcctttgttg aagtctaaagtctgagacggaaatttagataaataaacgcaagatttt aaaactugatgaattgaattgaTTCCAAGCATTATCTAAAATACTCTGCAGGCACGCTAGC1TGTA CTCAAGCTCGTAACGAAGGTCGTGACC1TGCTCGTGAAGGTGGCGACGTAA1TCGT TCAGCTUGTAAATGGTCTCCAGAACTITGCTGCTGCATGTGAAGTI1GGAAAGAAArT AAATTCGAAMGATACTATrGACAAACT1TrAA1TrTAT-ITCATGATG1TTATGT GAATAGCATAAACATCGTIT!-ATI I IIATGGTG1TrrAGGTrAAATACCTAAACAT CATITACAT=AAAATTAAGTTCTAAAGrTATCTI=GmAAAT-GCCTGTGC TTrATAAATACGATGTGCCAGAAAAATAAAATCTTAGC1TI1ATTATAGAATI1A TC1TATGTAT-rATA1TTATAAG'1ATAATAAAAGiAAATAGTAACATACTAAAGCG GATGTAGCGCGT11rATCnrAACGGAAGGAA1CGGCGCCTACGTAGGATCCgatccatg ctagcaatatctgatggtactgcatttcataagtttggcctggaaaaccaccgtttcggaagtacctgtcgctttagttttatagctaaatcta aagtttctttaagtctttagctgtittaatactccacgactttCCCttacgggacaataaataatttgtccccLtcccctacgtgacgtcagtg gcagttgcctgccaactgcctccttcggagtattaaaatcctatattataactcctaagtttacttgcccaatatttatattaggcgttggcag gcaactgccactgacgtcccgaaggggaaggggaaggacgtccccttcgggtaaataaattttagtggcagtggtaccaccactgcctgc ttcctccduccccttcgggcaagtaaacttagaaaaaattatttgctgcgtagcaggttacatactcctaagittacttgcccgaaggggaa ggaggacgtccccttacgggaatataaatattagtggcagtggtacaataaataattgtatgt.acccctcgggcaactflaagtttatcg cagtatataaatatagaatgtttacatactccgaaggaggacgccagtggcagtggtaccgccactgcctgtccgcagtattaacatcctattt SEQ ID Sequence Use NO. tatactccgaaggaggcagttggcaggcaactgccactaatatttatattccgtaaggggacgtcctaatttaatactccgaaggaggca gttggcaggcaactgCcactaaaatttatttgcctcctaacggagcattaafatcccgaaggggacgtcccgaaggggaaggggaagga ggcaactgcctgcttcctccttccccitcgggcaagtaaacttagaataaatttatttgctgcgctagcaggttacatactcctaagtttacttg cccgaaggggaaggaggacgtccccttacgggaatataaatattagtggcagtggtacaataaataaattgtatgaaaccccttcgggca actaaagtttatcgrcagatataatatcggcagttggcaggcaactgccactaaattcatttgcccgaaggggacgtccactaatatttatat tcccgtaaggggacgtcccgaaggggaaggggacgtcctaaacggagcattaaaatccctaagttacttgcctaggcagttggcaggat atttatatacgatattaatacttttgctactggcacactaaaattuatttgcccgtaaggggacgtccttcggtggttatataaataatcccgtagg gggagggggagtcccgtagggggaggggagtggaggctccaacggaggttggagcttctttggtttcctaggr-attatttaaatatttttta accctagcactagaactgagattccagacggcgacccgtalagttcttcgtcccctcagctttttcacaaccaagttcgggatggattggig tgggtccaactgagcaaagagcaccaaggttaactgcatctctgtgagatgctagttaaactaagcttagcttagctcataaacgatagttac ccgcaaggggtatgtaattatattataaggtcaaaatcaaacggcctttagtatatctcggctaaagccatgctgactgtacacctgatacct atataacggcttgtctagccgcggccttagagagcactcatcttgagtttagcttcctacttagatgctttcagcagttatctatccatgcgtagc tacccagcgtttcccattggaatgagaactggtacacaatggcatgtcctttcaggtcctctcgtactatgaaaggctactctcaatgctctaa cgcctacaccggatatggaccaaactgctcacgcatgaaflttttaaagccgaataaaacttgcggtctttaaaactaacccctttactttcgta aaggcatggactatgtcttcatcctgctactgttaatggcaggagtcggcgtattatactttcccactCTCGAGGGGGGGCCCG GTACCCAATTCGCCCTATAGTGAGTCGTATTACAATTrCACTGGCCGTCG1TFACAA CGTCGTGACTGGGAAAACCCTGGCG?TACCCAACT7AATCGCCTTGCAGCACATCC CCCTrCGCCAGCTGGCGTAATAGCGAAGAGGCCCGCACCGATCGCCCTrCCCAAC AG17GCGCAGCCTGAATGGCGAATGGGACGCGCCCTGTAGCGGCGCATTAAGCGCG GCGGGTGTGGTGGTrACGCGCAGCGTGACCGCTACACTrGCCAGCGCCCTAGCGCC CGCTCCT1TCGCTJTCTrCCCTrCCmrCTCGCCACGTTCGCCGGC1TICCCCGTCAA GCTCTAAATCGGGGGCTCCC1TIAGGGTTCCGA'IMAGTGCTIACGGCACCTCGAC CCCAAAAAACTTGATTAGGGTGATGGTrCACGTAGTGGGCCATCGCCCTGATAGAC GG1TF=CGCCCTrrGACGnGGAGTCCACGTC1TIAATAGTGGACTCTrGTrCCAA ACTGGAACAACACTCAACCCTATCTCGGTCTATITC1TGATIATAAGGGATTIG CCGAT1TCGGCCTATrTGGTrAAAAAATGAGCTGA1TAACAAAAATrrAACGCGAA T1TAACAAAATA17AACGC'FrACAA1TT7AGGTG 20 GCACT=CGGGGAAATGTGCGCGGAACCCTA1rrTTmATI1 CTAAATACA1T Endo-p3 CAAATATGTATCCGCTCATGAGACAATAACCCTGATAAATGCTTCAATAATA1TGA glucanase AAAAGGAAGAGTATGAGTA1CAACA1TCCGTTCGCCCTATCCC1TF=GCG insertion GCATI=GCC11CCTG I I I IGCTCACCCAGAAACGCTGGTGAAAGTAAAAGATGCT cassette GAAGATCAG17GGGTGCACGAGTGGGTlACATCGAACTGGATCTCAACAGCGGTAA (D GATCCTTGAGAG I II IGCCCCGAAGAACGTTCCAATGATGAGCAC1TIAAAGT TCTGCTATGTGGCGCGGTATATCCCGTA11GACGCCGGGCAAGAGCAACTCGGTC

KAN

GCCGCATACACTAT-rCTCAGAATGACTrGGT-[GAGTACTCACCAGTCACAGAAAAG BD0S) CATCTTACGGATGGCATGACAGTAAGAGAATTATGCAGTGCTGCCATAACCATGAG TGATAACACTGCGGCCAAC1TACTTCTGACAACGATCGGAGGACCGAAGGAGCTAA CCGCTTGCACAACATGGGGGATCATGTAACTCGCCT-rGATCGTTGGGAACCGG AGCTGAATGAAGCCATACCAAACGACGAGCGTGACACCACGATGCCTGTAGCAAT GGCAACAACGTnGCGCAAACTATAACTGGCGAACTACTACTCTAGCTTCCCGGC AACAA1TAATAGACTGGATGG AGGCGGATAAAGTTGCAGGACCACTFCTGCGCTCG GCCC1TCCGGCTGGCTGGTFTA1TGCTGATAAATCTGGAGCCGGTGAGCGTGGGTCT CGCGGTATCATrGCAGCACTGGGGCCAGATGGTAAGCCCTCCCGTATCGTAGTTATC SEQ ID Sequence Use NO.I TACACGACGGGGAGTCAGGCAACTATGGATGAACGAAATAGACAGATCGCTGAGA TAGGTGCCTCACTGATTAAGCA1TGGTAACTGTCAGACCAAG1TT7ACT)CATATATAC TTrAGATTGA1TAAAACTTCA'TI=AA1AAAAGGATCTAGGTGAAGATCCTrTr TGATAATCTCATGACCAAAATCCCTrAACGTGAGTM~CGT'rCCACTGAGCGTCAGA CCCCGTAGAAAAGATCAAAGGATCTrC'rrGAGATCCTTIrCTGCGCGTAATCTG CTGCrrGCAAACAAAAAAACCACCGCTACCAGCGGTGG1TG1TIGCCGGATCAAG AGCTACCAACTCITI1CCGAAGGTAACTGGCTTCAGCAGAGCGCAGATACCAAAT ACTGTCCTCTAGTGTAGCCGTAGTnAGGCCACCACTCAAGAACTCTGTAGCACCG CCTACATACCTCGCTCTGCTAATCCTGTTACCAGTGGCTGCTGCCAGTGGCGATAAG TCGTGTCTrACCGGGTrGGACTCAAGACGATAGTrACCGGATAAGGCGCAGCGGTC GGGCTrGAACGGGGGG1TCGTGCACACAGCCCAGCTTGGAGCGAACGACCTACACC GAACTGAGATACCTACAGCGTGAGCTATGAGAAAGCGCCACGC1TCCCGAAGGGA GAAAGGCGGACAGGTATCCGGTAAGCGGCAGGGTCGGAACAGGAGAGCGCACGAG GGAGCTrCCAGGGGGAAACGCCTGGTATCTTrATAGTCCTGTCGGGTTrCGCCACCT CTGACTrGAGCGTCGAT1T=GTGATGCTCGTCAGGGGGGCGGAGCCTATGGAAAA ACGCCAGCAACGCGGCC1TTACGGTTCCTGGCC=IIGCTGGCCTI1GCTCACAT GTrC1TCCTGCG1TATCCCCTGATrCTGTGGATAACCGTArACCGCC1TGAGTGA GCTGATACCGCTCGCCGCAGCCGAACGACCGAGCGCAGCGAGTCAGTGAGCGAGG AAGCGGAAGAGCGCCCAATACGCAAACCGCCTCTCCCCGCGCGTTGGCCGATrCAT TAATGCAGCTGGCACGACAGGTCCCGACTGGAAAGCGGGCAGTGAGCGCAACG CAA1-rAATGTGAGTrAGCTCACTCATAGGCACCCCAGGCTACACTrATGCTTC CGGCTCGTATGTTGTGTGGAATTGTGAGCGGATAACAATITCACACAGGAAACAGC TATGACCATGA1TACGCCAAGCTCGAAATTAACCCTCACTAAAGGGAACAAAAGCT GGAGCTCCACCGCGGTGGCGGCCGCTCTAGCACTAGTGGATCGCCCGGGCTGCAGG AATTCcatatttagataaacgatttcaagcagcagaatagctttattagaacaaactgtaaagaaatgaatgtaccaatgccgcgcatt gtagaaaaaccagataattatatcaaattcgacgtalacgtgaattaaaacctgatttaacgattactggaatggcacatgcaaatccattaga agctcgagglattacaacaaaggtcagtgaatttacttttgctcaaattcatggatactaatacacgtgaaattttagaattagtaacacag cctcttagacgcaatctaatgtcaaatcaatctgtaaatgctatttcttaatataaatcccaaaiagattttttttatatactgagacttcaacactta cttgtttttattttgagttacaattcactcacgttaaagacattggaatgaggcaggacgttagtcgatattaacactcttaagtttacttgc ccaatatttatataggacgtccccttcgggtaaataaattttagtggcagtggtaccaccactgcctattttaatactccgaagcatataaatat acttcggagtatataaatatccactaatatttatattaggcagttggcaggcaacaataaataatttgtcccgaaggggacgicccgaagg ggaaggggaagaaggcagttgcctgcctatcggctaacaagttcctttggagtatataaccgcctacaggtaacttaaagaacatttgtta cccgtaggggtttataCttCtaattgcttcttctgaacaataaaatggtttgtgtggtctgggctaggaaacttgtaaCaatgtgtaggtcgcttc cgcttcccttcgggacgtccccttcgggaagtaaacttaggagtataaatcgggacgtccccttcgggtaaataaattcagggacgtcc ccttacgggacgccagtagacgtcagtggcagttgcctcgcctatcggctaacaagttcctlcggagtatataaatatagaatgttacatact cctaagttactgcctccttcggagtatataaatatcccgaagggaggaggacgccagggcagggtaccgccactgccgcttcctc cttcggagtatgtaaaccccttcgggcaactaaagtttatcgcagtatataaatataggcagttggcaggcaactgccactgacgtcctatttt aatactccgaaggaggcagtggcaggcaactgccactgacgtcccgtaagggtaaggggacgtccactggcgtcccgtaaggggaag gggacgtaggtacataaatgtgctaggtaactaacgittgat~tttgtggtataatatatgtaccatgcttttaatagaagcttgaatttataaat aaaatatttttacaatattttacggagaaattaaaactttaaaaaaattaacatATGGTACCAAACAAAAGCGTAGCAC CATTAT'rACTrGCTGCATCTATC~rATATGGTGGTGCTGTTGCTCAACAGACTG1TG GGGTCAGTGTGGTGGTATTGG'TGGTCTGGTCCTACCAAU7GTGCTCCTGGCTCAGC

ATGTAGTACC'FIAAATCCTACTATGCTCAATGTATTCCAGGTGCAACAACTATAAC

SEQ ID Sequence Use NO. AACATCAACTCGCCCTCCTTCAGGTCCAACTACAACAACTCGTGCTACTAGCAC1TC TAGCAGCACACCTCCTACATCTCTGGAGTACGTICGCTGGTGTTAATA1TGCAGG TrCGATIMGGTGTACTACCGATGGTACATGTGTrACCAGTAAAG1TATCCCCCT 1TAAAAAAT1TACTGGCTCAAACAATTATCCAGATGGCATFGGTCAAATGCAACA ClI rGTAAATGAAGATGGTATGACTATTCCG1TFACCAGTGGGCTGGCAATAC1T AGTUAACAACAA1TTAGGTGGTAACTAGATAGTACATCAATTAGTAAATATGATC AA17AGTACAAGGTrGCrrAT='~AGGTGCCTArrGTATrGTTGATArCATAA1TA TGCCCGTrGGAACGGTGGTATTATTGGTCAAGGTGGTCCAACTAATGCTCAA1TTAC ATCATTATGGAGCCAA1TAGCTTCAAAATATGCTAGTCAATCACGTGTITGG1TCGG TATrATGAATGAACCTCACGATGTGAACATAAATAC11rGGGCTGCAACTGTGCAAG AAGTAGTAACTGCTA11'CGTAATGCTGGTGCAACATCACAA11'CATTAGTTrACCAG GCAACGATTGGCAATCTGCCGGCGCTITATTrCTGACGGTAGCGCAGCTGCTC77A GTCAAGTGACTAACCCAGACGGTAGTACCACTAACTTAATAT1CGATGTACATAAA TATCflGATTCTGATAATAGCGGAACACACGCCGAATGTACCACAAATAATA11GA TGGTGCT17AGTCCTFAGCAAC1TGGTTACGTCAAAATAATCGCCAAGCCATI AACTGAAACAGGTGGTGGAAACGTGCAGAGflGTATCCAAGACATGTGTCAAC AAA TITCAGTACTTAAATCAAAACTCTGACGTGTAC1TAGGTATGTAGGT'rGGGGTGCTG GTrC1TIGATCAAC11'ATGTATrAACCGAAACCCCTACTTCTCTGGAAACTCATG GACAGACACTrCATrAGTAAGTAG1TG1TAGCTCGCAAGGGTACCGGTGAAAACT TATAC I I IAAGGCTCAGGTGGCGG1'GGAAGTGA~rACAAAGATGATGATGATAAA GGAACCGGTAATCTAGActagcttcaaCtaactctagctcaaacaactaatttttttttaaactaaataaatctggttaacc atacctggtttattttagttagtttatacacatctitcatatatatatacttlatagctaccataggcagttggcaggacgtccctacgggacaa atgtatttatgttgcctgccaactgcctaatataaatattagtggacgtCCCCttccccttacgggcaagtaaacttagggatttaatgctccgt taggaggcaaataaattttagtggcgttgcctcgccatcggctaacaagtccCtcggagtatataaatatcctgccaactgccgatatttat atactaggcagtggcggtaccactcgacGGATCCTACGTAATCGATGAATrCGATCCCAT1T1ATA ACTGGTCTCAAAATACCTATAAACCCA1GTrCTCTCTI=AGCTCTAAGAACAAT CAATJTATAAATATATITTA1TATGCTATAATATAAATACTATATAAATACATI ACC1r'IATAAATACAT=ACCI111TrAA=rGCATGATJ1TAATGCTATGCTA TC7TTATAGTCCATAAAACCTTAAAGGACCTI"CTATGGGATA1rATAT TTTCCTAACAAAGCAATCGGCGTCATAAACTIAGTTGCTTACGACGCCTGTGGACG TCCCCCCCl-rCCCCTTACGGGCAAGTAAACTTAGGGATF=AATGCAATAAATAAAT TrGTCCTCTTCGGGCAAATGAAl1TAGTA1TAAATATGACAAGGGTGAACCA'frA C1TMG1TAACAAGTGATCTrACCACTCACTATFIG1TGAA'IrAAACTTATrA AAATTCTCGAGAAAGA1I'AAAAATAAACn~nTAATC1T'A1TATTICTI 'lr~cgatggaatgcccaatatattcacaatttatcggaaacagcgttttagagccaaataaaattggtcagtcgccatcggatgtttat tcdttaatcgaaataatgaaac~ttttcttaaigcgatctagcactttatatacagagaccacatacagtctctcgtgaagcgaaaatgttga gttggctctctgagaaattaaagggcctgaactcatcatgacttttcaggatgagcagtttgaatttatgatcactaaagcgatcaatgcaaaa ccaatttcagcgctttttttaacag acaagaattgcttgctatctataaggaggcactcaatctgttaaattcaattgctattattgattgtccatt atttcaaacattgatcatcggttaaagagtcaaaattttttattgataaccaactccttgacgatatagatcaagatgattttgacactgaattatg gggagaccataaaacttacctaagtctaggaatgagttaaccgagactcgtgttgaagaaagatggttttttctatggcgatatcacggat agtaatatttatagataaattcaatgaaatttattttttagaccttggtcgtgctgggttagcagatgaatttgtagatatatcctttgttgaacgtt gcctaagagaggatgcatcggaggaaactgcgaaaatatttttaaagcatttaaaaaatgatagacctgacaaaaggaattatttttaaaact tgatgaattgaatgaTrCCAAGCAlTATCTAAAATACTrCTGCAGGCACGCTAGCTTGTACTCA S§EQ ID Sequence Use NO. _ _ _ AGCTCGTAACGAAGGTCGTGACC1TGCTCGTGAAGGTGGCGACGTAArCGflCAG CTrGTAAATGGTCTCCAGAACTGCTGCTGCATGTGAAG1TIGGAAAGAAAU7AAAT TCGAAT1TIGATACTATGACAAAC'IMAATFI1ATITrCATGATGTT7ATGTGAAT AGCATAAACATCG1TATTATGGTGMI~AGGT-AAATACCTAAACATCA1= TACATmAAAAA1TAAG1TCTAAAGTATCTITTrAAA'IMGCCTGTGCTTmAT AAATrACGATGTGCCAGAAAAATAAAATCAGCTIIAnATAGAAITATCT1' ATGTATrATAT1ATAAGT1ATAATAAAAGAAATAGTAACATACTAAAGCGGATG TAGGCGTrATCTAACGAAGGAATCGGCGCCTACGTAGGATCCgtatccagctagcaa tatctgatggtacttgcatttcataagttggcctggaataflccaccgtttcggaagtacctgtcgctCLagttttatagctaaatctaagtttcLt taagtcttttagctgtattaatactcacgactttccctacgggacataataaattgtccccttccccttacgtgacgtcagtggcagttgc ctcacgcctcggataactttrttcctattctccaataatgcgtgagacg cactgacgtcccgaaggggaaggggaaggacgtccccttgggtaaataaattttagtggcagtggtaccaccactgcctgcttcctccct ccccttcgggcaagtaaacitagaataaaattatttgctgcgctagcaggtttacatactcctaagttacttgcccgaggggaaggagga cgwccccttacgggaatataaatattagtggcagtggtacaataaataaattgtatgtaaaccccttcgggcaactaagtttatcgcagtatat aaatatagaatgttacatactccgaflggaggacgccagtggcagtggtaccgccactgcctgtccgcagtattactcctatt(atactc cgaaggaggcagtggcaggcaactgccactaatatttatatt~ccgtaaggggacgtCCtaatttaatactccgaaggaggcagttggca ggcaactgccactaaaatttatttgcctcctacggagcattaatcccgaaggggaCgtcccgaggggaaggggaggaggcaact gcctgcttcctccttccccttcgggcaagtaaacttagataaaattatttgctgcgctagcaggtttacatactcaagtttacttgcccgaa ggggaaggaggacgtcccctacgggatataaatatagtggcagtggtacaataaataaattgtatgtaaaccccttcgggcaactaag tttatcgcagtatataaatatcggcagttggcaggcaactgccactaaaatcatttgcccgaaggggacgtceactaatatttatattcccgta aggggacg!cccgaaggggaaggggacgtcctaaacggagcattaaatccctaagttactgcctaggcagttggcaggatatttatat acgatattaatacttttgctactggcacactaaaatttatttgcccgtaaggggacgtccttcggtggttatataaatatcccgtagggggagg gggatgtcccgtagggggaggggagtggaggctccaacggaggttggagcttctttggtttctaggcattattaatattttttaaccctag cactagaactgagatccagacggcgacccgtaaagtcttcagtcccctcagcttttcacaaccaagttcgggatggattggtgtgggtcc aCLgagcaaagagcaccaaggttaactgcatctctgtgagatgctagttaactaagcttagcttagctcataaacgatagtta~ccgcaag gggttatgtaattaattataaggtcaaaatcaacggcctttagatatctcggctaaagccattgctgactgtacacctgatacctatataacg gcttgtctagccgcggccttagagagcactcatctugagtttagcttcctacttagatgctttcagcagttatctatccatgcgtagctacccag cgtttcccattggaatgagaactggtacacaatggcatgtccttcaggtcctctcgtactatgaa2aggctactctcaatgctctaacgcctac accggatatggaccaaactgtctcacgcatgaaattttaaagccgaataaaacttgcggtctttaaaactaaccccttacttcgtaaggcat ggactatgtcttcatcctgctactgttaatggcaggagtcggcgtattatactttcccactCTCGAGGGGGGGCCCGCTAC CCAATTCGCCCTATAGTGAGTCGTATACAATCACTGGCCGTCG11MACAACGTC GTGACTGGGAAAACCCTGGCGTTACCCAACTITAATCGCCFIGCAGCACATCCCCCTT' TCGCCAGCTGGCGTAATAGCGAAGAGGCCCGCACCGATCGCCCTCCCAACAG11G CGCAGCCTGAATGGCGAATGGGACGCGCCCTGTAGCGGCGCArrAAGCGCGGCGG GTGTGGTGGTTACGCGCAGCGTGACCGCTACACTTGCCAGCGCCCTAGCGCCCGCT Cc I ICGCMC7CCCTCCTTCTCGCCACGTCGCCGGCTCCCCGTCAAGCTC TAAATCGGGGGCTCCC1TAGGGTI'CCGATrrAGTGCTIACGGCACCTCGACCCCA AAA AACTTGAflAGGGTGATGGflCACGTAGTGGGCCATCGCCCTGATAGA CGG1T 1TrCGCCCMGACGTGGAGTCCACGTCTrAATAGTGGACTCTTGTCCAAACTG GAACAACACTCAACCCTATCTCGGTCTArC I IIGA1TrATAAGGGATGCCGA TrrCGGCCTArrGGTrAAAAAATGAGCTGATIAACAAAAA'FflAACGCGAATflA ACAAAATATTAACGCTTACAAT-rrAGGTG 21 GCACTTCGGGGCAAATGTGCGCGGAACCCCTATrG'A'1ATmCTAAATACATr SEQ ID Sequence Use NO. CAAATATGTATCCGCTCATGAGACAATAACCCTGATAAATGCTCAATAATAT'GA P-gluco AAAAGGAAGAGTATGAGTATCAACA1TCGTGTCGCCC'ATCCCT=GCG sidase CCA1T=GCC~rCCTGrrTrGCTCACCCAGAAACGCTGGTGAAAGTAAAAGATGCT insertion GAAGATCAGTTGGGTGCACGAGTGGGTTACATCGAACTGGATCTCAACAGCGGTAA cset GATCCTTGAGAG11MCGCCCCGAAGAACG=CCAATGATGAGCAC=AAAGT TCTGCTATGTGGCGCGGTATATCCCGTATUGACGCCGGGCAAGAGCAACTCGGTC D GCCGCATACACTAUrCTCAGAATGACUTGG1GAGTACTCACCAGTCACAGAAAAG KN CATCT-ACGGATGGCATGACAGTAAGAGAATATGCAGTGCTGCCATAACCATGAG BDO9) TGATAACACTGCGGCCAACTnACTrCTGACAACGATCGGAGGACCGAAGGAGCTAA CCGCFTITMGCACAACATGGGGGATCATGTAACTCGCC~rGATCGUrGGGAACCGG AGCTGAATGAAGCCATACCAAACGACGAGCGTGACACCACGATGCCTGTAGCAAT GGCAACAACGVTGCGCAAACTATTAACTGGCGAACTACUACTCTAGCflCCCGGC AACAATnAATAGACTGGATGGAGGCGGATAAAG'ITGCAGGACCACUrCTGCGCTCG GCCCTTCCGGCTGGCTGG1TATrGCTGATAAATCTGGAGCCGGTGAGCGTGGGTCT CGCGGTATCATTGCAGCACTGGGGCCAGATGGTAAGCCCTCCCGTATCGTAGTUATC TACACGACGGGGAGTCAGGCAACTATGGATGAACGAAATAGACAGATCGCTGAGA TAGGTGCCTCACTGA1TAAGCATI'GGTAACTGTCAGACCAAGT17ACTCATATATAC T1TAGA1TGATTTAAAACTUCA1TI1AATFAAAAGGATCTAGGTGAAGATCC=~ TGATAATCTCATGACCAAAATCCCTTAACGTGAGTITCGTTCCACTGAGCGTCAGA CCCCGTAGAAAAGATCAAAGGATCTICTIGAGATCCTT1T=CTGCGCGTAATCTG CTGCTTGCAAACAAAAAAACCACCGCTACCAGCGGTGGTrGTTGCCGGATCAAG AGCTACCAACTCTCCGAAGGTAACTGGCTCAGAGAGCGCAGATACCAAAT ACTGTCCTTCTAGTGTAGCCGTAGUrAGGCCACCACTTCAAGAACTCTGTAGCACCG CC'rACATACCTCGCTCTGCTAATCCTGTTACCAGTGGCTGCTGCCAGTGGCGATAAG TCGTGTCTTACCGGGTlGGACTCAAGACGATAGrACCGGATAAGGCGCAGCGGTC GGGCTGAACGGGGGGTrCGTGCACACAGCCCAGCTTGGAGCGAACGACCTACACC GAACTGAGATACCTACAGCGTGAGCTATGAGAAAGCGCCACGCTflCCCGAAGGGA GAAAGGCGGACAGGTATCCGGTAAGCGGCAGGGTCGGAACAGGAGAGCGCACGAG GGAGCTTCCAGGGGGAAACGCCTGGTATCTMATAGTCCTGTCGGG1CGCCACCT CTGACTrGAGCGTCGATITIGTGATGCTCGTCAGGGGGGCGGAGCCTATGGAAAA ACGCCAGCAACGCGGCCTrACGGTCCTGGCCT=FGCTGGCC=GCTCACAT GT1CrCCTGCGTATCCCCTGATlCTGTGGATAACCGTAT1ACCGCCTIGAGTGA GCTGATACCGCTCGCCGCAGGCGAACGACCGAGCGCAGCGAGTCAGTGAGCGAGG AAGCGGAAGAGCGCCCAATACGCAAACCGCTCTCCCCGCGCG'rGGCCGAT-CAT TAATGCAGCTGGCACGACAGGTICCCGACTGGAAAGCGGGCAGTGAGCGCAACG CAATTAATGTGAGTAGCTCACTCATAGGCACCCCAGGCACACTATGCT'C CGGCTCGTATGTIGTGTGGAATnGTGAGCGGATAACAA1TCACACAGGAAACAGC TATGACCATGA'TTACGCCAAGCTCGAAATflAACCCTCACTAAAGGGAACAAAAGCT GGAGCTCCACCGCGGTGGCGGCCGCTCTAGCACTAGTGGATCGCCCGGGCTGCAGG AArrCcatattagataaacgatttcaagcagcagaattagctttattagaacaaacttgtaaagaatgaatgtaccaatgccgcgcatt gtagaaaaaccagataatattatcaaattcgacgtatacgtgaataaaacctgatttLacgattactggaatggcacatgcaaatccataga agctcgaggtattacaacaaaatggtcagttgaatttacttttgctcaaatcatggattactaatacacgtgaattttagaattagtaacacag ccctgccacattaacacgaagttttattatcaagttt~aatcggctacct SEQ ID Sequence Use NO. cttgttttattttttgtagttacaatlcacicacgttagacattggaaaai~tgaggcaggacgtagcgatattatar-actcttaagUtacttgc ccaatatttatattaggacgtccccttcgggtaatattttagtggcagtggtaccaccactgcctatttaatactccgagcataaatat acttcggagtatataaaatccactaatatttatattaggcagtggcaggcaacaataataaattgtcccgtaggggacgtcccgaagg ggaaggggaagaaggcagtgcctcgcctatcggctaacaagttcctttggagtatataaccgcctacaggtaacttLaagaacatttgtta cccgtaggggtttatacttctattgctttctgaacaataaatggtttgtgtggtctgggcaggaaacttgtaacaatggtagtgtcgctc cgcttcccttcgggacgtcccc~tcgggtaagtaaacttaggagtattaatcgggacgtccccttcgggtaaataatttcagtggacgtcc ccttacgggacgccagtgacgcagtggcagttgcctcgcctatcggctaacaagttccitcggagatataaatatagatgttacaact cctaagtttacttgcctccttcggagtatataaatatcccgaaggggaaggaggacgccagtggcagtggtaccgccactgcctgcttcctc aatactccgaaggaggcagttggcaggcaactgccactgacgtcccgtaagggtaaggggacgtccactggcgtcccgtaaggggaag aaaatatttttacaatattttacggagaaattaaaactttaaaaaaattaacatATGGTACCA1TACCAAAGGAT1TCCA ATGGGGTTCGCTACCGCAGCrTATCAAA11'GAAGGTGCAGTTGATCAAGATGGAC GTGGACCTTCTA1TGGGACACATTCTGTGCACAACCAGGTAAAATrGCTGATGGnr CATCAGGTGTAACAGCATGTGACTCATATAATCGTACAGCTGAAGACATI'GCACT17 TAAAATCTTTAGGTGCTAAATCATATCG1TrCTCTATCTCATGGTCAAGAATrATTCC TGAAGGTGGCCGTGGTGACGCAGTAAATCAAGCTGGTAUrGATCACTATG1TAAAT TTGTAGATGACT-YA7AGACGCAGGTATACACC1T=ATCACTA1CACTGGG ATTACCTGAAGGMIACACCAACG77ATGGTGGTCTI1AAACCGTACAGAAITIC CIMAGA I I IGAAAACTATGCAAGAGTTATGTmCGTGCACTCCCAAAGTAAGAA ACTGGATTAC1TTAATGAACC11ATGTTCTGCTATrCCTGGTIATGGTrCAGGCAC CrrrGCCCCAGGCAGACAAAGTACAAGTGAGCCCTGGACAGTGGGCCATAACATT TAGTAGCTCACGGTAGAGCTGTAAAAGCATATAGAGATGA1TCAAACCTGCTrCA GGTGATGGTCAAATAGGTATTGTGTT'AAATGGTGACTICACATATCCCTGGGATGCC GCTGATCCTGCAGATAAAGAAGCCGCTGAACGTCGCTTAGAATTTCACTGCITGG rrrGCTGACCCCATCTATC17GGTGA~rATCCTGCTrCAATGCGTAAACAATrAGGT GATCGTACCTAC=T1ACACCAGAAGAACGTGCTTAGTrCATGGTAGTAATGAC 1T'IATGGTATGAACCACTATACTrCAAACTATATrCGTCACCGTAGCTCACCCGCA AGTGCTGATGACACAGTAGGTAATGTAGATG1TrAMTACTAATAAACAAGGTAA TrGTATCGGTCCTGAAACACAGAGCCCCTGGCTTCGTCCTrGTGCAGCTGGTTrCCG TGAC1rCCTrGTATGGATAAGCAAACGTrATGGTrATCCACCAATTrATGTTACAGA AAACGGAACATCAATAAAAGGTGAAAGTGACTTACCAAAGGAAAAGA7rC1TGAA GATGATrCGTG17AAGTA1TATAACGAATACATrAGAGCTATGGTrACAGCCGTr GAArrAGATGGTGTAAATGTAAAAGGTA1TrCGCATGGTC1TAATGGATAAC1T GAATGGGCTGATGGTI'ACGnTACACG1T=GGTGTAACCTACGTTGATTACGAAAAC GGCCAAAAACGTrCCCTAAAAAGAGTGCTAAAAGmAAAACCT1TrA1TGATGA ATTAATAGCTGCTGCAGGTACCGGTGAAAAcTI'ATAC1TI'CAAGGCTCAGGTGGCG GTGGAAGTGATTACAAAGATGATGATGATAAAGGAACCGGTrAATCTAGActagcttca atatacttaatagctaccataggcagttggcaggacgtcccctacgggacaaatgtatttattgttgcctgccaactgcctaatataatatta gtggcgtcccctccccttacgggcaagtaaacttagggatttaatgctccgtaggaggcaaaaaatttagggcagtgcctcgccta tcggctaacaagttCCttCggagtatataaatatcctgccaactgccgatatttatatactaggcagtggcggtaccactcgacGGATCC TACGTAATCGATGAA1rCGATCCCATFF=ATAACTGGTCTCAAAATACCTATAAAC SEQ ID Sequence Use NO. CCATTrCTTCTC1TIAGCTCTAAGAACAATCAA11ATAAATATATIA1TATTA TGCTATAATATAAATACTATATAAATACATI1'ACC1TTATAAATACATTTACCTI' YTrMAATTGCATGA1TMAATGCTrATGCTATCTI=AIAGTCCATAAAACCT -TAAAGGACCITrCTATGGGATATATA---CCTAACAAAGCAATCGGCGTCA TAAAC1TIAGTrGCTTACGACGCCTGTGGACGTCCCCCCCTrCCCC1TACGGGCAAG TAAAC1TAGGGATMAATGCAATAAATAAA1TGTCCTC1TCGGGCAAATCAA1M TAGTATTrAAATATGACAAGGGTGAACCA11ACTI'TrGTrAACAAGTGATCTT'ACCA CTCACTA III I GT1GAATIAAACTrAMAAAATCTCGAGAAAGA1TIAAAA ATAAACT-FF=AATCITAMA II ITCTI Cgtatggaatcccatatcaacaattatc ggaaacagcgttttagagccaaataa83ttggtcagtcgccatcggatgtattctttatcgataatgaaactttttttcttagcgatcta gcactttatatacagagaccacatacagtgtctctcgtgaagcgaaatgttgagggctctctgagaattaaggtgcctgaactcatcat gactttcaggagagcagtttgatttatgacactaaagcgatcaatgcanacatttcagcgctttttttacagaccaagaattgcttgc tacaagagatatttaatatgttatatgcatatcactgtacgtaaataattt attgataaccaactccttgacgatatagatcaagatgattttgacactgaattatggggagaccataaaacttacctaagtctatggaatgagtt aaccgagactcgtgttgaagaaagattggtttttctcatggcgatatcacggatagtaatattttatagataaattcaatgaaatttatttttaga ccttggtcgtgctgggttagcagatgaattgtagatatatccttgtigaacgttgcctaagagaggatgcatcggaggaaactgcgaaaat atttttaaagcattaaaaaatgatagacctgacaaaaggaattattLtttaacttgatgttgattgaTCCAAGCATTATCT AAAATACTCTGCAGGCACGCTAGCTrGTACTCAAGCTCGTAACGAAGGTCGTGACC 11TGCTCGTGAAGGTGGCGACGTAAflCGTTCAGCTTGTAAATGGTCTCCAGAACTlG CTGCTGCATGTGAAGTI'GGAAAGAAATAAArrCGAA1TGATACTAflGACAAA CTITAAT=IA1FlrCATGATG1IATGTGAATAGCATAAACATCG TITATI TATGGTGT11'AGGTrAAATACCTAAACATCATIACATIAAAAUrAAGTTCTA AAGTATCTIMGTTTAAA1TrGCCTGTGC1TTrATAAATrACGATGTGCCAGAAAAA TAAAATCTrAGCTTrATATAGAATIATCTI1'ATGTATTrATA I II IATAAGTnAT AATAAAAGAAATAGTAACATACTAAAGCGGATGTAGCGCGTTTATCTrAACGGAAG GAATTCGGCGCCTACGTAGGATCCgtatccatgcagcaaatctgatggtacttgcaLttcataagtttggcctggat aaccaccg~tttcggaagtacctgtcgcLttaagttttatagctaatctaagtttctttaagtcttagctgattaatactccacgactttccctt acgggacaataaataaatttgtccccttccccttacggacgtcagtggcagttgcctgccaactgcctccttcggagataatcctatat tatatactcctaagtttacttgcccaataitatattaggcagttggcaggcaactgccactgacgtcccgaagggg2.aggggaaggacgtc cccttcgggtaaataaatttagtggcagggtaccaccacgcctgcttccictttcccc~cgggcaagtaaacttagaataaatttatttgc tgcgctagcaggtttacatactcctaagtttacttgcccgaaggggaaggaggacgccccttacgggatatatattagtggcagtggt acaataaataaattgtatgtaaaccccttcgggcaactaaagtttatcgcagtatataaatatagaatgttacataCtccgaggagacgcc agtggcagtggtaccgccactgcctgtccgcagtattaacatcctattttaatactccgaaggaggcagtggcaggcaactgccactaatt ttatattcccgtaaggggacgtcctaatttaatactccgaaggggcagttggcaggcaactgccactaaattatttgcctcctacggag cattaaatcccgaaggggacgtcccgaaggggaaggggaaggaggcaactgcctgcttcctccttccccttcgggcaagtacttag aataaaatattgctgcgctagcaggtttacatactcctaagtttaCttgcccgaaggggaaggaggacgccccttacgggaatataata ttagtggcagtggtacaataaataaattgtatgtaaaccccttcgggcaactaaflgtttatcgcagtatataaatatcggcagttggcaggcaa ctgccactaaaattcatttgcccgaaggggacgtccactaatattatattcccgtaaggggacgtcccgaaggggaaggggacgtcctaa acggagcattaaaatccctaagtttacttgcctaggcagttggcaggatatttatatacgatattaaactttgctactggcacactaaaattat ttgcccgtaaggggacgtccttcggtggttatataaataatcccgtagggggagggggatgtcccgtagggggaggggagtggaggctc caacggaggttggagcttcttggtttcctaggcatiatttaaatattttaaccctagcactagaactgagattccagacggcgacccgtaaa gttcttcagtcccctcagcttttcacaaccaagicgggatggattgggtgggtccaacgagcaagagcaccaaggtaacgcatctt gtgagatgctagttaaactaagctagcttagctcataaacgatagttacccgcaaggggttatgtaattatattataaggtcaaaacaaacg SEQ ID Sequence Use NO. gccttagtatatctcggctaagccattgctgactgtacaccgatccatataacggctttctagccgcggccttagagagcactcatct gagtttagcttcctacLtagatgctttcagcagttactatccatgcgtagcacccag cgtttCCCattggagaCtggtaCaCattgg catgtcctttcaggtcctctcgtactatgaaggctactctcaatgctctaacgcctacaCCggatatggacca3ctgtctcacgcatgaaat tttaaagccgaataaactgcggtctttaaaactaacccctttacttcgaaaggcatggactatgtcttcatcctgctactgttaatggcagg agtcggcgtattatactttcccactCTCGAGGGGGGGCCCGGTACCCAATrCGCCCTATAGTGAGTC GTATrACAA11'CACTGGCCGTCGT1TrACAACGTCGTGACTGGGAAAACCCTGGCGT TACCCAACTrAATCGCCITrGCAGCACATCCCCC1TrrCGCCAGCTGGCGTAATAGCGA AGAGGCCCGCACCGATCGCCC17CCCAACAGUTGCGCAGCCTGAATGGCGAATGGG ACGCGCCCTGTAGCGGCGCA1TAAGCGCGGCGGGTGTGGTGGUrACGCGCAGCGTG ACCGCTACACTrGCCAGCGCCCTAGCGCCCGCTCCCGCTTC1CCCTCCTC TCGCCACGflCGCCGGC1TTrCCCCGTCAAGCTCTAAATCGGGGGCTCCC'rTAGGGT TCGTTGG~rCGACCACCAAA~rA7GGGTG CACGTAGTGGGCCATCGCCCTGATAGACGGTrTMCGCCC11GACG17GGAGTCCA CGTfCTITAATAGTGGACTCTrCCAAACTGGAACAACACTCAACCCTATCTCGG TCTATrC1TrGA1TATAAGGGATI1GCCGATTrCGGCCTATTGGnAAAAAAATGA GCTGATIAACAAAAA11AACGCGAATI=AACAAAATAnAACGCTACAAm1A GGTG 22 GCAc1TrrcGGGGAAATGTGCGCGGAACCCCTA17TTTrATITCTAAATACAT-r Endo CAAATATGTATCCGCTCATGAGACAATAACCCTGATAAATGCTCAATAATATTGA xylanase AAAGAATTATTrACTTCGGCCC'~rCT=C insertion GCAT'TMGCC'VrCCTG1IrMGCTCACCCAGAAACGCTGGTGAAAGTAAAAGATGCT cassette GAAGATCAG7rGGGTGCACGAGTGGGT-rACATCGAACTGGATCTCAACAGCGGTAA GATCCTTGAGAGr1TCGCCCCGAAGAACGTTITrCCAATGATGAGCAC1TIAAAGT TCTGCTATGTGGCGCGGTATATCCCGTATTGACGCCGGGCAAGAGCAACTCGGTC KN GCCGCATACACTAnCTCAGAATGACTTIGGTITGAGTACTCACCAGTCACAGAAAAG B 1 CATCTTACGGATGGCATGACAGTAAGAGAATTATGCAGTGCTGCCATAACCATGAG TGATAACACTGCGGCCAACTrAC~rCTGACAACGATCGGAGGACCGAAGGAGCTAA CCGCT'-TGCACAACATGGGGGATCATGTAACTCGCCTrGATCG11'GGGAACCGG AGCTGAATGAAGCCATACCAAACGACGAGCGTGACACCACGATGCCTGTAGCAAT GGCAACAACGTTGCGCAAACTATITAACTGGCGAACTAC~rACTCTAGCTrCCCGGC AACAATTAATAGACTGGATGGAGGCGGATAAAG1TGCAGGACCACTlCTGCGCTCG GCCCTTCCGGCTGGCTGG1TAT'rGCTGATAAATCTGGAGCCGGTGAGCGTGGGTT CGCGGTATCATrGCAGCACTGGGGCCAGATGGTAAGCCCTCCCGTATCGTAGflrATC TACACGACGGGGAGTCAGGCAACTATGGATGAACGAAATAGACAGATCGCTGAGA TAGGTGCCTCACTGATTAAGCATrrGGTAACTGTCAGACCAAG1TACTCATATATAC TTrAGATrGAm1AAAACTTCA'FTAATrAAAAGGATCTAGGTGAAGATCCI= TGATAATCTCATGACCAAAATCCCTFAACGTGAGTIT1CG~rCCACTGAGCGTCAGA CCCCGTAGAAAAGATCAAAGGATCCGAGATCCIm=CGCGCGTAATCTG CTGCTTGCAAACAAAAAAACCACCCTACCAGCGGTGG1GTITGCCGGATCAAG AGCTACCAACTCTTT=CCGAAGGTAACTGGCTTCAGCAGAGCGCAGATACCAA AT ACTGTCCnTCTAGTGTAGCCGTAG11'AGGCCACCAC~CAAGAACTCTGTAGCACCG CCTACATACCTCGCTCTGCTAATCCTGUrACCAGTGGCTGCTGCCAGTGGCGATAAG

TCGTGTCTTACCGGGTGGACTCAAGACGATAGTIACCGGATAAGGCGCAGCGGTC

SEQ ID Sequence Use NO. I GGGCTGAACGGGGGGTTCGTGCACACAGCCCAGCTTGGAGCGAACGACCTACACC GAACTGAGATACCTrACAGCGTGAGCTATGAGAAAGCCCACCT-CCCGAAGGGA GAAAGGCGGACAGGTATCCGGTAAGCGGCAGGGTCGGAACAGGAGAGCGCACGAG GGAGCTrCCAGGGGAAACGCCTGGTATCATAGTCCTGTCGGGCCACCT CTGACT-rGAGCGTCGA1TTTGTGATGCTCGTCAGGGGGGCGGAGCCTATCICAAAA ACGCCAGCAACGCGGCCTACGGTCCTGGCCTrGCTGGCC=GCTCACAT GTCTrTCCTGCG17ATCCCCTGATrCTGTGGATAACCGTA11'ACCGCCMGAGTGA GCTGATACCGCTCGCCGCAGCCGAACGACCGAGCGCAGCGAGTCAGTGAGCGAGG AAGCGGAAGAGCGCCCAATACGCAAACCGCCTCTCCCCGCGCGTTGGCCGA1TCAT TAATGCAGCTGGCACGACAGGTTCCCGACTGGAAAGCGGGCAGTGAGCGCAACG CAATrAATGTGAGTrAGCTCACTCATrAGGCACCCCAGGCnTACAC'r1ATGCTTC CGGCTCGTATGflGTGTGGAATIGTGAGCGGATAACAA1MCACACAGGAAACAGC TATGACCATGA1TACGCCAAGCTCGAAATTAACCCTCACTAAAGGGAACAAAAGCT GGAGCTCCACCGCGGTGGCGGCCGCTCTAGCACTAGTGGATCGCCCGGGCTGCAGG AA17Ccatattagataaacgatttcagcagcagaattagcttattagaacaaacttgtaaagaatgagtaccaatgccgcgcatt gtagaaaaaccagataattattatcaaattcgacgatacgtgaattaaaacctgatttaacgatacggaatggcacatcgaaatccatiaga agctcgaggtattacaacaaaatggtcagttgaatttacttttgctcaaattcatggatttactaatacacgtgaatttiagaattagCtacaag cctcttagacgcaatctaagtcaaatcaatctgtaaagctattLctaatataaatcccaaaagat(tttataatactgagacttcaacactta ctugtttttattttttgtagttacaattcactcacgttaaagacattggaaaatgaggcaggacgttagtcgatatttatacactcttaagttacttgc ccaatatttatattaggacgtccccttcgggtaaataaattttagtggcagiggtaccaccactgcctattttaatactccgaagcatataatat acttcggagtatataaatatccactaatatttatattaggcagttggcaggcaacaataaataaatttgtcccgtaaggggacgtccgaagg ggaaggggaagaaggcagttgcclcgcctatcggctaacaagttcctthggagtatataaccgcctacaggtaacttaaagaacatttgtta cccgtaggggtttatacttctaattgctcttctgaacaataaaatggtttgtgtggtctgggctaggaaacttgtaaCaatgtgtagtgtcgCttc cgcttcccttcgggacgtccccttcgggtaagtaaacttaggagtattaaatcgggacgtccccttcgggtaaataaatttcagtggacgtcc ccttacgggacgccagtagacgtcagtggcagttgcctcgcctatcggctaacaagttccttcggagtatataaatatagaatgttacatac cctaagtttacttgcctccttcggagtatataaatatcccgaaggggaaggaggacgccagtggcagtggaccgccactgcctgcttcctc cttcggagtatgtaaacccttcgggcaactaaagtttatcgcagtaaaaatataggcagtggcaggcaactgccacgacgtcctatttt aatactccgaaggaggcagttggcaggcaactgccactgacgtcccgtaagggtaaggggacgtccactggcgtcccgtagggagg gggacgtaggtacataaatgtgctaggtaactaacgtttgattttttgtggtataatatatgtaccatgctttta.alagaagcttgaatttataatt aaaatatttutacaatattttacggagaaattaaaactttaaaaaaattaacatATGGTACCAGTATCT-r-CACAAGTCT TITAGCAGCATCTCCACCTTCACGTGCAAGTrGCCGTCCAGCTGCTGAAGTGGAATC AGT1TGCAGTAGAAAAACGTCAAACAATITCAACCAGGTACAGGTITACAATAACGGT ACTTIATTCT-rACTGGAATGATGGACACGGTGGTGT'TACATATACTAATGGACCTG GTGGTCAAT1AGTGTAAA'TrGGAGTAACTCAGGCAATITFGGAGGAAAAGGT TGGCAACCTGGTACAAAGAATAAGGTAATCAA1TICTCTGGTAGTTACAACCCTAA TGGTAA11TCTATIrAAGTGTATACGGTrGGAGCCGTAACCCA11'AATrGAATATTA TATTGTAGAGAACTTGGTACATACAACCCflCAACAGGTGCTACTAAAflrAGGTGA AGTrACTTCAGATGGATCAGTATGATATTTATCGTACTCAACGCGTAAATCAACC ATCTATAAn'GGAACT3CCAC1CTACCAATACTGGAGTGTAAGACGTAATCATCG T'CAAGTGGTAGTGT'TAATACAGCAAACCACTfAATGCATGGGCTCAACAAGG1TTT AACATIAGGTACAATGGACTATCAAA17GTAGCTGflGAAGGTTA1TFICATCAGG TAGTGCTTCTATCACTGTTAGCGGTACCGGTGAAAACTTATACTITCAAGGCTCAGG TGGCGGTGGAAGTGATTACAAAGATGATGATGATAAAGGAACCGG1AATCTAGAct SEQ MD Sequence Use NO. tagcttcaactaactctagctcaaa3ctttttttaaZctalta!ctggttaaccaacctggttta~ttttagtttagtttatacacactt ctcgcctatcggctaacaagttccttcggagtatataaatatcctgccaactgccgaatttatatactaggcagtggcggtaccactcgacG GATCCTACGTAATCGATGAACGATCCCAT=ATAACTGGTCTCAAAATACCTA TAAACCCATrGflCT1TCTCTI1'AGCTCTAAGAACAATCAAm'rATAAATATA17AT TATrATGCTATAATATAAATACTATATAAATACA1TACC1=ATAAATACATA CCTI1r=AATTTGCATGATI'AATGCTTATGCTATCTIA=AGTCCATAA AACCT'AAAGGACCTFTTATGGGATATrATA=~TCCTAACAAAGCAATCGG CGTCATAAACTTAGTFGCTTACGACGCCTGTGGACGTCCCCCCC7CCCCTTACGG GCAAGTAAACTAGGGATAATGCAATAAATAAATIGTCCCCGGGCAAATG AAlTIAGTATTTAAATATGACAAGGGTGAACCArACMGTlAACAAGTGATCT TACCACTCACTATFI1TTGAATAAACATAAAATTCTCGAGAAAGA I cgatctagcacttatatacagagaccacatacagtgtctctgtggcgaaagttgagttggctctctgagaaaLtaaaggtgcctgaa ttgcttgctatctataaggaggcactcaatctgttaaatcaattgctattattgattgtccattattcaacattgatcatcggttaaaagagtca aatgagttaaccgagactcgtgttgaagaaagattggtttt~tctcatggcgatltcacggatagLwLatttttatagataattcaataaattt gcgaaatatttttaaagcatttaaaaaatgaagaccgacaaaaggattattttttaaaacttgatgaattgaattgaTTCCAAGCA TTATCTAAAATACTCTGCAGGCACGCTAGCTTGTACTCAAGCTCGTAACGAAGGTCG TGACC17GCTCGTGAAGGTGGCGACGTAAFICGTTCAGCflGTAAATGGTCTCCAGA ACnrGCTGCTGCATGTGAAGTfGGAAAGAAAnTAAATCGAAT-GATACTATTGA CAAACT11.AA II IITA1TI-CATGATGTATGTGAATAGCATAAACATCGTm=A I i I IiATGGTGTTTAGGTTAAATACCTAAACATCATrACA1TITAAAA7T~AAGT TCTAAAGrATCTGTAAATGCCTGTGCTTrATAAA~ACGATGTGCCAGAA AAATAAAATCnrAGC1TrATrATAGAA11TATCTTATGTATTATAWIMATAAGT TATAATAAAAGAAATAGTAACATACTAAAGCGGATGTAGCGCG'flTATC'7AACGG ggaataaccaccgtttcggaagtacgtcgctttagttttatagctaaatctaaagtttcttLaagcttttagctgtattaaactccacgactt tcccttacgggacaataataaatttgtccccttccccttacgtgacgtcagtgcagttgcctgccaactgcctccttcggagtatatcc cgtccccttcgggtaaataaattttagggcagtggtaccaccactgcctgcttcctccttccccttcgggcaagaaactagaa~aattta tttgctgcgctagcagg(Ctacatactcctaagttacttgcccgaaggggaggaggacgtccccttacgggaatataaatattagtggcag tggtacaataaataaattgtatgtaaaccccttcgggcaactaaagtttatcgcagtatataaatatagaatgttac2actccgaaggaggac gccagtggcagtggtaccgccactgcctgtccgcagtattaacatcctattttaaactccgaagaggcagttggcaggcaactgccacta atttttcctaggctcattaatcagagcgtgagacgccaattttctcac gagcattaaaatcccgaaggggacgtcccgaggggaaggggaaggaggcaactgcctgcLtcctccttccccttcgggcaagtaaact tagaataaaatttattgctgcgctagcaggtttacatactcctaagttacttgcccgaagggaaggaggacgccccttacgggaatataa caactgccactaaaattcatttgcccgaaggggacgtccactaatatatatcccgtaaggggacgtcccgaaggggaaggggacgtcc SEQ ID Sequence Use NO. taaacggagcattaaaatccctaagtttacttgcctaggcagttggcaggatatttatatacgatattaatacttttgctactggcacactaaaatt tatttgcccgtaaggggacgtccttcggtggttatataataatcccgtagggggagggggatgtccgtagggggaggggagtggagg ctccaacggaggttggagcttctttggtttcctaggcattatttaaatattttttaaccctagcactagaactgagattccagacggcgacccgt aaagttcttcagteccctcagetttttcacaaccaagttegggatggattggtgtgggtccaaetgagcaaagagcaccaaggttaactgcat ctctgtgagatgetagttaaactaagettagettagetcataaacgatagttacccgcaaggggttatgtaattatattataaggtcnaatcaa acggcctttagtatatctcggctaaagccattgtgactgtacacctgatacctatataacggcttgtctagccgcggccttagagagcactca tettgagtttagettcctacttagatgctttcagcagttatetatccatgcgtagctacccagcgtttcccattggaatgagaaetggtacacaatt ggcatgtcctttcaggtcctctcgtactatgaaaggetactctcaatgctctaacgcctacaccggatatggaccaaactgtetcacgcatga aattttaaagccgaataaaacttgggtctttaaaactaacccctttacttcgtaaaggcatggactagtttcatcctgctactgttaatggca ggagtcggcgtattatactttcccactCTCGAGGGGGGGCCCGGTACCCA ATTCGCCCTATAGTGAG TCGTATTACAATTCACTGGCCGTCG1TITACAACGTCGTGACTGGGAAAACCCTGGC GTrACCCAACTTAATCGCCTTGCAGCACATCCCCCTTTCGCCAGCTGGCGTAATAGC GAAGAGGCCCGCACCGATCGCCCTTCCCAACAGTTGCGCAGCCTGAATGGCGAATG GGACGCGCCCTGTAGCGGCGCATTAAGCGCGGCGGGTGTGGTGGTTACGCGCAGCG TGACCGCTACACTTGCCAGCGCCCTAGCGCCCGCTCC CGCTTFCTTCCCTrCCTT TCTCGCCACGTTCGCCGGCTrCCCCGTCAAGCTCTAAATCGGGGGCTCCCmTrAGG GTTCCGATTTAGTGCTTTACGGCACCTCGACCCCAAAAAACTrGATTAGGGTGATGG TrCACGTAGTGGGCCATCGCCCTGATAGACGG I II1 I I GCCCMGACGTTGGAGTC CACGTTCTTTAATAGTGGACTCT-rGTTCCAAACTGGAACAACACTCAACCCTATCTC GGTCTATTCTITTGATTTATAAGGGATIGCCGAMCGGCCTATTGGTTAAAAAAT GAGCTGAMAACAAAAATAACGCGAAT AACAAAATATTAACGCTrACAA TT TAGGTG 23 GTGCACTCTCAGTACAATCTGCTCTGATGCCGCATAGT7AAGCCAGCCCCGACACCC p-gluco GCCAACACCCGCTGACGCGCCCTGACGGGCTTGTCTGCTCCCGGCATCCGCTTACA sidase GACAAGCTGTGACCGTCTCCGGGAGCTGCATGTGTCAGAGG=TCACCGTCATCAC insertion CGAAACGCGCGAGACGAAAGGGCCTCGTGATACGCCTA1TrATAGGTTAATGTC cassette ATGATAATAATGGTTCTrAGACGTCAGGTGGCACTITCGGGGAAATGTGCGCGG AACCCCTATFGTTATlTlCTAAATACATTCAAATATGTATCCGCTCATGAGACA

KAN

ATAACCCTGATAAATGCTfCAATAATATTGAAAAAGGAAGAGTATGAGTATTCAAC ATTTCCGTGTCGCCCTTAn-CCCITIT1TGCGGCATTGCCTTCCTGTGCTCAC rbcL CCAGAAACGCTGGTGAAAGTAAAAGATGCTGAAGATCAGTTGGGTGCACGAGTGG BDO9) GTTACATCGAACTGGATCTCAACAGCGGTAAGATCCTrGAGAGTTrfCGCCCCGAA GAACGTFTTCCAATGATGAGCACTTAAAGTTCTGCTATGTGGCGCGGTATnATCC CGTATlGACGCCGGGCAAGAGCAACTCGGTCGCCGCATACACTATTCTCAGAATGA CTFGGTrGAGTACTCACCAGTCACAGAAAAGCATCTTACGGATGGCATGACAGTAA GAGAATTATGCAGTGCTGCCATAACCATGAGTGATAACACTGCGGCCAACTTACT' CTGACAACGATCGGAGGACCGAAGGAGCTAACCGCU'I GCACAACATGGGGGA TCATGTAACTCGCCTTGATCGTGGGAACCGGAGCTGAATGAAGCCATACCAAACG ACGAGCGTGACACCACGATGCCTGTAGCAATGGCAACAACGTTGCGCAAACTATTA ACTGGCGAACTACTnACTCTAGCnrCCCGGCAACAATTAATAGACTGGATGGAGGC GGATAAAGTTGCAGGACCACTFCTGCGCTCGGCCCTCCGGCTGGCTGGTTAfTTGC TGATAAATCTGGAGCCGGTGAGCGTGGGTCTCGCGGTATCATGCAGCACTGGGGC

CAGATGGTAAGCCCTCCCGTATCGTAGTTATCTACACGACGGGGAGTCAGGCAACT

SEQ ID Sequence Use NO. ATGGATGAACGAAATAGACAGATCGCTGAGATAGGTGCCTCACTGATTAAGCATrG GTAACTGTCAGACCAAG11ACTCATATATACI1AGATGATTAAAACTTCATIM TAAT17AAAAGGATCTAGGTGAAGATCC1TrMrGATAATCTCATGACCAAAATCCCT TAACGTGAGI I TG1TCCACTGAGCGTCAGACCCCGTAGAAAAGATCAAAGGATC TrCTGAGATCCTT1TCTGCGCGTAATCTGCTGC1TGCAAACAAAAAAACCACC GCTACCAGCGGTGGMFGTIGCCGGATCAAGAGCTACCAACTC1TrMCCGAAGGT AACTGGCTT'CAGCAGAGCGCAGATACCAAATACTGTrCTCTAGTGTAGCCGTAGTr AGGCCACCACTTCAAGAACTCTGTAGCACCGCCTACATACCTCGCTCTGCTAATCCT G1TACCAGTGGCTGCTGCCAGTGGCGATAAGTCGTGTCUACCGGGTTGGACTCAA GACGATAGTlACCGGATAAGGCGCAGCGGTCGGGCTGAACGGGGGGflCGTGCAC ACAGCCCAGCTTrGGAGCGAACGACCTACACCGAACTGAGATACCTACAGCGTGAGC TATGAGAAAGCGCCACGCITCCCGAAGGGAGAAAGGCGGACAGGTATCCGGTAAG CGGCAGGGTCGGAACAGGAGAGCGCACGAGGGAGC'I1CCAGGGGGAAACGCCTGG TATCTTrATAGTCCTGTCGGGi I IGCCACCTCTGACTrGAGCGTCGA1TTMGTGAT GCTCGTCAGGGGGGCGGAGCCTATGGAAAAACGCCAGCAACGCGGCCI=ACGG TrCCTGGCC=FGCTGGCCTI=GCTCACATGTTC1TCCTGCGTrATCCCCTGA~rC TGTGGATAACCGTATIACCGCCITITGAGTGAGCTGATACCGCTCGCCGCAGCCGAA CGACCGAGCGCAGCGAGTCAGTGAGCGAGGAAGCGGAAGAGCGCCCAATACGCAA ACCGCCTCTCCCCGCGCGTTGGCCGArrCA11'AATGCAGCTGGCACGACAGG1TrCC CGACTGGAAAGCGGGCAGTGAGCGCAACGCAATTAATGTGAG1TAGCTCACTCA1T AGGCACCCCAGGCTIACACF1ATGCTlCCGGCTCGTATGTTGTGTGGAA1TGTGA GCGGATAACAA1CACACAGGAAACAGCTATGACCATGATACGCCaagcIcgcggccgc agtactCTGCAGATIMATGCAAAAT1TAAAGTC117GTGACAACAGCT1TCTCCTTAAGTG CAAATATCGCCCATTCTTTCCTCTITCGTATATAAATGCTGTAATAGTAGGATGTC GTACCCGTAAAGGTACGACATTGAATATT7AATATACTCCTAAG1TAC1TCCCAAT AmATATAGGACGTCCCCTCGGGTAAATAAA1TrAGTGGCAGTGGTACCGCCA CTCCCTA1TIAATACTGCGAAGGAGGCAG1IGGCAGGCAACTCGTCGTTCGCAGTA TATAAATATCCACTAATATTIATAYI'CCCGTAAGGGGACGTCCCGAAGGGGAAGGG GAAAGAAGCAGTCGCCTCCTGCGAAAAGGTrACTTGCCCGACCAGTGAA AAGCA TGCTGTAAGATATAAATCTACCCTGAAAGGGATGCA1TICACCATAATACTATACA AATGGTGTTACCCT11GAGGATCATAACGGTGCTACTGGAATATATGGTCTC1TCAT GGATAGACGATAGCCATTTA'11ACCCA1TAAGGGGACATrAGTGGCCTGTCACTGC TCC7rACGAGACGCCAGTGGACGTTCGTCCTAGAAAATATGCGCTGCCTAGAAG CCCCAAAAGGGAAGTTACTGACTCGTTAGAGCGTGCGCTAACAGG111'AAATACT TCAATATGTATAflAGGACGCCGGTGGCAGTGGTACCGCCACTGCCACCGTCGGAG GACGTCCCTTACGGTATATTATATACTAGGA1TPAATACTCCGAAGGAGGCAGTGG CGGTACCACTGCCACTAATA1TATA1TCCCGTAAGGGACGTCCTCCTTCGGAGTAT GTAAACA-TCTAAGTTACTIGCCCAATAI1-rATA1TAGGCAGTrGGCAGGCAACTG CTAGCTCTCCTCCTICGGAGTATGTAAACATCGCAGTATATAAATATCCACTAATAT 7rATAUCCCGTAAGGGGACGTCCCGAAGGGGAAGGGGAAGGACGTCAGTGGCAG TTGCCTGCCAACTGCCTAGGCAAGTAAACTTAGGAGTATATAAATATAGGCAGTCG CGGTACCACTGCCACTGACGTCCTGCCAACTGCCTAGGCAAGTAAACUrAAGTGGC

ACTAAAATGCAMGCCCGAAGGGGAAGGAGGACGCCAGTGGCAGTGGTACCGCC

SEQ ID Sequence Use NO. ACTGCCTCCTTCGGAGTATITAAAATCCTAGTATGTAAATCTGCTAGCGCAGGAAATA AATnATCTATI'ATATACTCCGTAGGAGGTAAGTAAACCCC117CCCC17CGGG ACGTCAGTGCAGTITGCCTGCCAACTGCCTAATATAAATATAGACCACTAAAGTFIG GCAACTGCCAACTGTITGTCCTCGGAGGAAAAAAAATGG7AACTCGCAAGCAGfl AACATAACTAAAG1rGTrACTITACCGAAGACG1TACCCIT[CGGTrAAGGAG ACGGAGACAGTGCACTGTGACTGCCTAGTATAGCAATIGTITrGTTrATATGC TCGACAAAATGACTCATAAAAATATAAAGTAGTAGCTAGrA=~ATATCACT ATAACTAGGGTCTCAGAGGCACCGAAGTCACnGTAAAAATAGTACTFIAACTT GTTrAATC1TCGTGTTC1TCAAAAGGATCACGTAA1TFI1TGAAGGTGGACCAAAA CTAACATAAACTGAATAGCCAGTTACACTTAACAGAAGAAACCATAAAAAAAAGG TAAAGAAAAAAGCTGGAC71TCCATAGCTCA1TAATAATAAAATTATTCTCTTrrC AACATATCTC1TAGATAGTrCAAAAGACTrGACGACTGTGTCCCACATITFAAACA AAATTAATCTACTCAAAATMGCCCTGAGAAAGAATAACTrACTTCGTITFGCAG TAGCCA1TCATGTCACT-GAAACTGTCCTrACAAAGTIAAACATrAATUAAAAA17 ATFAA11TrATATAACAAATATrATATAAATAAAAAATGAACAAAGAACTFCTA AGATCGTCT1TAGTGAGTAATTAAAGAGThAC17ACCAGACAAGGCAGTTIC ATTCTITAAAGCAGGCAGflCTGAAGGGGAAAAGGGACTGCCTACTGCGGTCCTA GGTAAATACATITIATGCAATrAm1CTGTGCTAGTAGGT1CTATACTCACAAG AAGCAACCCCTTGACGAGAGAACGU7ATCCTCAGAGTA1ATAATCCTGAGAGGG AATGCACTGAAGAATA=1ICC17A'TITIACAGAAAGTAAATAAAATAGCGCTAA TAACGCTTAATrCATrAATCAATnATGGCAACAGGAACTI'CTAAAGCTAAACCATC AAAAGTAAATTCAGACTrTCCAAGAACCTGGTMAGTJTACACCAT7AGGTACTT-rA11 ACGTCCAC1-rAACTCAGAAGCAGGTAAAGTA'ACCAGGCTGGGGTACAACTG=~ TAATGGCTGTATATCCTTATTGCAGCATCTATAATCA1TfAGAANITA CAACAGTTC1TTAA1T-rAGATGACGTTrCTATGAGTrGGGAAAC1TrrAGCTAAAGT T7CrAATT1ATTAACACAAACATAAAATATAAAACTGTTAAGGCTAGCTG CTAAGTCTCT1TICGCTAAGGTAAACTAAGCAACTCAACCATKTTATATTCGGCA GTGGACCGCCAACTGCCACTGGCCTTCCGTrAAGATAAACGCGTggatctcacgtgactagtc acctagtgtcgagtggtaccgccactgcctagtatataaatatcggcagtuggcaggatatttatatactccgaaggaacttgttagccgatag gcgaggcaactgccactaaaattatttgcctcctaacggagcattaa~ltccctaagtttacttgcccgtaaggggaaggggactccact aatatttatattaggcagttggcaggcaacaataaatacattgtcccgtaflggggacgtcctgccaactgcctatggtagctattaagtatata tatatgaaaagtggtataaacaaactaaaataaaccaggtatggttaaccagattatttagttaaaaaaaaattaggttgagctagagI tagttgaagctaagtcagaTTAACCGG11TCCTfATCATCATCATC1TGTAATCAC11'CCACCG CCACCTGAGCCTTGAAAGTATAAG I I IACCGGTACCTGCAGCAGCTATTAATTCA TCAAATAAAGGTTAAAC=AGCACTCTFI=AGGGAAACG11T=GGCCGnrM CGTAATCAACGTAGGTTACACCAAAACGTGTAACGTAACCATCAGCCCATlCAAAG TTATCCATrAAAGACCATc3CGAAATAACCTI=ACA1TACACCATCTAATTCAACG GCTGTAACCATAGCTCTAATGTATCGTTATAATACTTAACACGAAAATCATC'ITCA AGA ATCTFTCCTTGGTAAGTCACTTCACCTITATIGATG1T-CCGTTICTGTAA CATAAATTGGTGGATAACCATAACG1TIGCTnATCCATACAAGGAAGTCACGGAAA CCAGCTGCACAAGGACGAAGCCAGGGGCTCTGTG1TCAGGACCGATACAAT-TACC TTG1TATTAGTAAATAAAACATCTACArTACCTACTGTGTCATCAGCACTTGCGGG TGAGCTACGGTGACGAATATAG1TTGAAGTATAGTGGFI7CATACCATAAAAGTCAT SEQ ID Sequence Use NO. TACTACCATGAACTAAAGCACGT-rC11'CTGGTGTAAAAGTAGGTAAACGATCACCT AATTG1TTACGCA1TGAAGCAGGATAATCACCAAGATAGATGGGGTCAGCAAACCA AGCAGTGAAAAATTCTAAGCGACGT-CAGCGGCTrCTIrATCTGCAGGATCAGCGG CATCCCAGGGATATGTGAAGTCACCATIAACACAATACCTA1TGACCATCACCTG AAGCAGGTrrGAAATCATCTCTATATGCTM~ACAGCTCTACCGTGAGCTACTAAAA TGTTATGGCCCACTGTCCAGGGCTCACflGTACITGTCTGCCTGGGGCAAAGGTGC CTGAACCATAACCAGGAATAGCAGAACATAAAGG11'CAT1AAAAGTAATCCAGTIrT CT'rAC~rTGGGAAGTGCACGAAACATAACTC11GCATAG1TTCGAAATCTAAAGGA AATTCTGTACGGTTnAAAAGACCACCATAACGT-rGGTGTAAACCTrCAGGTAAATCC CAGTGAAATAAAGTGATAAAAGGTGTAATACCTGCGTCTAATAAGTCATCTACAAA T-1TAACATAGTGATCAATACCAGCTrGATrACTGCGTCACCACGGCCACCrrTCAGG AATAArTCTCACCATGAGATAGAGAAACGATATGA'I1TAGCACCTAAAGATIA AAAGTGCAATGTCTTCAGCTGTACGA1TATATGAGTCACATGCTGTTACACCTGATG AACCATCAGCAATIMACCTGGTrGTGCACAGAATGTGTCCCAAATAGAAGGTCCA CGTCCATCTrTGATCAACTGCACCTrCAATTGATAAGCTGCGGTAGCGAAACCCCAT TGGAAATCC1TGGTAATGGTACCATatgcacttgcatacctccgtacaaattattttgatttctataaagttmgcta aataaaaatttttaatttttaacgtccacccatataaataataaatatggtgaaacctttaacaacaaatcctcttgtaccatattaatccaaaag aattaaggacaaaagcttatctccaacatttaaaacacagagtaaaaataatgttgtitttaagaatagaattttataacttgtattttaaatatga tctaatttatttgtgctaaaaattgcagttggaaagtaattutaaaaataatttagatcatattattaaataaagttgatttaaaacaactaatcgttt ggaccttttctatgggatatttatatttcctaacaagcaatcggcgtcaaaactttaggctacgacgcctgggacgtcccccccttccc cttacgggcaagtaaacttagggattttaatgcaataaataaattigtcctcttcgggcaaatgaattttagtatttaaatatgacaagggtgaac ttttatttattttttcttttttCGTATGGAATGCCCAATATrATrCAACAA11TATCGGAAACAGCGT TTrAGAGCCAAATAAAATrrGGTCAGTCGCCATCGGATG1TrCYTrAATCGAAA TAATGAAACTITFTCTTAAGCGATCTAGCACTI1ATATACAGAGACCACATACAG TGTCTCTCGTGAAGCGAAAATGTrGAG1TGGCTCTCTGAGAAAT7AAAGGTGCCTG AACTCATCATGACTTTCAGGATGAGCAGTTrGAA1TATGATCACTAAAGCGATCA ATGCAAAACCAATrrCAGCGCTTTTAACAGACCAAGAA'TGCTrGCTATCTATA AGGAGGCACTCAATCTGTI'AAATTCAATTGCTATTATflGATTGTCCATITATITCAA ACATTGATCATCGGTrAAAAGAGTCAAAATTrATrGATAACCAACTCCTTGACG ATATAGA1'CAAGATGA1TrGACACTGAATTATGGGGAGACCATAAAAC1TACCTA AGTCTATGGAATGAGTfTAACCGAGACTCGTGTGAAGAAAGArrGG1TITTCTCAT GGCGATATCACGGATAGTAATATI=ATAGATAAA7CAATGAAA11ATI11A GACC~rrGGTCGTGCTGGGTTAGCAGATGAATGTAGATATATCCTTrGrGAACGT TGCCTAAGAGAGGATGCATCGGAGGAAACTGCGAAAATA1TITAAAGCATTAAA AAATGATAGACCTGACAAAAGGAATATI1TAAAACflGATGAATlGAA1TGAttc caagcattatctaaaalactctgcaggcacgctagctgtactcaagctcgtaacgaaggtcgtgaccttgcLcgtgaaggtggcgacgtaa ttcgttcagcttgtaaatggtctccagaacttgctgctgcatgtgaagtltggaaagaaattaaaUtcgaacttgatactatlgacaaaclltaattt ttatttcatgatgtttatgtgaltagcataaacatcgttttattagggtaggtaaataccaaacacatttacatttaaa3Uaagttc SEQ ID Sequence Use NO. uttataagttataataalagaaatagtaacatactaaagcggatgtagcgcgtttatCttaacggaaggaattcggcgcctacgtacccgggt cgcgaggatccACGCGTTAATAGCTCACTPTT1AAATI'AATIAA1TTAAAGGTG TAAGCAAA1TGCCTGACGAGAGATCCACTTAAAGGATGACAGTGGCGGGCTACTGC CTACfCCCTCCGGGATAAAATIATrGAAAAACGTAGTTACTTCCTAACGGAGC ATTGACATCCCCATATIATATAGGACGTCCCCflCGGGTAAATAAAITIAGTGG ACGTCCCCTCGGGCAAATAAATITAGTGGACAATAAATAAA1TIGTITGCCTGCCA ACTGCCTAGGCAAGTAAAC'TGGGAGTATAAAATAGGACGTCAGTGGCAG1ITGCC TGCCAACTGCCTATATTTATATACTGCGAAGCAGGCAGTGGCGGTACCACTGCCACT GGCGTCCTAATATAAATATrGGGCAACTAAAGTITrATAGCAGTATrAACATCCTATA TTrATATACTCCGAAGGAAC1TGTAGCCGATAGGCGAGGCAACAAAMTTTA1T GTCCGGTAAAAGGATGCCTCCAGCATCGAAGGGGAAGGGGACGTCCTAGGCCATA AAACTAAAGGGAAATCCATAGTAACTGATGTI'ATAAAT1TATAGACTCCAAAAAAC AGCTGCGflATAAATAAc1TCTGTTAAATATGGCCAAGGGGACAGGGGCAC1TTTCA ACTAAGTGTACATTAAAAAT-rGACAATrCAATITTTAATnATAATATATATITA GTAAAATATAACAAAAAGCCCCCATCGTCTAGgtagaattccagctggcggccgccctatg 24 agatctcgatcccgcgaaattaatacgactcactataggggaattgtgagcggataacaattcccctctagaaataattttgtttaactttaaga Exo-p3 aggagatataCATATGGTACCATATCGTAAAC1TOGCTGrTATrAGTGC1TTCT-rAGCTACT glucanase GCTCGTGCACAGTCAGCATGTACCTACAATCTGAAACTCATCCTCCAT-AACATGG insertion CAAAAATGTI'CTCAGGAGGTACUGTACACAACAAACTGGCTCTGTAGTAATTGAT cset GCTAACTGGCGTlGGACACATGCCACTAATAGflCAACTAA11'GTIATGACGGTAAT(pT2I ACTTGGTCATCAACACT'GTCCCGATAACGAAACTTGTGCTAAAAATrGTGr1TA GATGGTGCAGCflACGC1TCAACT-ACGGCGTI'ACTACATCAGGTAACTCAflATCA BOI ATTGG1TCGTGACTCAATCAGCACAAAAAAATGTAGGCGCACG'IIATACTTAATG GCAAGTGACACAACCTATCAAGAA-I-ITACA1TrArrAGGTAATGAGTTCAG1TCGAC GTAGATGTGAGTCAATACCATGTGGTrAAATGGTGCTC'TrAT1TCG I I IAATG GACGCTGATGGCGGTGTAAGCAAATATCCTACTAATACAGCAGGTGCTAAATACGG AACAGGCTATGTGATFCTCAGTGTCCTCGTGATTAAAG1TATTAACGGTCAAGC TAACGTGGAAGGTI'GGGAACCAAGTAGTAATAATGCAAATACTGGAATTGGTGGTC ACGGATCTTGTTTCTGAAATGGATA1TGGGAAGCTAATUCAATTAGTGAAGCAT TAACTCCACATCCTTGTACTACCGTrGGCCAAGAAAM~GTGAAGGCGACGGT1GCG GTGGAACATACAGTGATAACCG'TATGGTGGTACATGTGATCCTGATGGCTGCGAT TGGGACCCATATCGTTrAGGAAATACATCTTATGGACCAGGAAG1TCATrCACA TrAGATACAACTAAAAAGrrAACAGTI'GTFACACAGTTCGAAACTAGCGGTGCTAT TAATCGTATACGTGCAAAATGGTGTAACT71rCAACAACCAAATGCAGAATrAG GTFC1TA~rCTGGTAACGGCCTfAATGACGATTArGTACAGCAGAAGAAGCAGAA T'ITGGTGGTAGCAGCT-rCTCAGATAAAGGTGG1TAACTCAAflCAAGAAAGCAAC ATCAGGTGGTATGGTITAG1TATGTCMTrATGGGATGACTAflATGCTAATATG1T ATGG1TAGATAGTACATATCCTACAAACGAAAC1TCAAGCACTCCTGGTGCTGflCG TGGTTCATGTCAAC1CAAGTGGTGTACCTGCTCAAGTI'GAAAGCCAAAGTCCTAA TGCAAAAGTAACrMAGTAATATCAAA1TGGTCCAATrGGCTCTACAGGCGATCC TTCAGGTGGTAATCCACCAGGTGGAAATCCACCTGGCACCACTACAACACGTCGTC CTGCTACTACCACAGGTrC11'CTCCTGGACCAACACAATCTCAT-rACGGTCAATGTG GTGGTA11-GGTrATTCAGGTCCAACTGTGTGTGCATCAGGAACTACATGTCAAGTrT SEQ ID Sequence Use NO. TAAATCCATATTATAGCCAATGTIAGGTACCGGTGAAAACTrATACIICAAGGCT CAGGTGGCGGTGGAAGTGATTrACAAAGATGATGATGATAAAGGAACCGG1TAATCT AGACTCGAGcaccaccaccaccaccactgagatccggctgctaacaaagcccgaaaggaagctgagttggctgctgccaccgc tgagcaataactagcataaccccttggggcctctaaacgggtcttgaggggtttttgctgaaaggaggaactatatecggattggcgltg ggacgcgccctgtagcggcgcattaagcgcggcgggtgtggtggttacgcgcagcgtgaccgctacactgcagcgccctagcgccc gcwcctttcgctttcttcccttcctttctcgccacgttcgccggcttcccgtcaagctctaaatcgggggctccctttagggttccgatttagtg ctttacggcacctcgaccccaanaacttgattagggtgatggttcacgtagtgggccatcgccctgatagacggtttttcgccctttgacgtt ggagtccacgttcttaatagtggactctigttccaaactggaacacactcaccctatctcggtctattctfgatttataagggatttgccg atttcggccattggttaaaaatgagctgatttaacaaaaatttaacgcgaattaacaaaatattaacgtttacaattcaggtggcacttttcg gggaaatgtgcgcggaaccccatttgtttatttttctaaatacaflcaaflatgtatccgctcatgagacaataacccigataaatgcttcaata atattgaaaaaggaagagtatgagtattcaacatttccgtgtcgcccttattcccttttgcggcatttgccttcctgttttgctcacccagaaa cgctggtgaaagtaalagatgctgaaatcagttgggtgcacgagtgggttacatcgaactggatctcaacagcggtaagatccttgagag ttttcgccccgaagaacgttttccaatgatgagcacttttaaagtctgctatgtggcgcggtattatcccgtattgacgccgggcaagagcaa crcggtcgccgcataCactattctcagaatgacttggttgagtactcaccagtcacagaaaagcatcttacggatggcatgacagtaagaga attatgcagtgctgccataaccatgagtgataacactgcggccaacttacttctgacaacgatcggaggaccgaaggagctaaccgctttttt gcacaacatgggggatcatgtaacLcgccttgatcgttgggaaccggagctgatgaagccataccaaacgacgagcgtgacaccacga tgcctgcagcaatggcaacaacgttgcgcaaactattaactggcgaactactactctagcttcccggcaacaattaatagactggatggag gcggataaagttgcaggaccacttctgcgcteggcccttccggctggctggttattgctgataaatctggagccggtgagcgtgggctcg cggtatcattgcagcactggggccagatggtaagccctcccgtatcgtagttatctacacgacggggagtcaggcaactatggatgaacg aaatagacagatcgctgagataggtgcctcactgattaagcattggtaactgtcagaccaagtttactcatatatactttagattgatttaaaact rcatttutaatttaaaaggatctaggtgaagatcctttttgataatctcatgaccaaaatcccttaacgtgagttttcgttccactgagcgtcagac cccgtagaaaagatcaaaggatctctgagatcctltttctgcgcgtaatctgctgctgcaaacaaaaaaaccaccgctaccagcggtg gtttgtttgccggatcaagagctaccaactctmttccgaaggtaactggcttcagcagagcgcagataccaatactgtccttctagtgtagc cgtagttaggccaccacttcaagaactctgtagcaccgcctacatacctcgctctgctaatcctgttaccagtggctgctgccagtggcgata agtcgtgtcttaccgggttggactcaagacgatagttaccggataaggcgcagcggtcgggctgaacggggggttcgtgcacacagccc agcttggagcgaacgacctacaccgaactgagatacctacagcgtgagctatgagaaagcgccacgcttcccgaagggagaaaggcg gacaggtatccggtaagcggcagggtcggaacaggagagcgcacgagggagcttccagggggaaacgcctggtatctttatagtcctgt cgggtttcgccacctctgacttgagcgtcgatttttgtgatgctcgtcaggggggcggagcctatggaaaaacgccagcaacgcggcctttt tacggttcctggccttttgctggccttttgctcaCatgttctttcctgcgttatcccctgattctgtggataaccgtattaccgcctttgagtgagct gataccgctcgccgcagccgaacgaccgagcgcagcgagtcagtgagcgaggaagcggaagagcgcctgatgcggtattttctcctta cgcatctgtgcggtatttcaeaccgcatatatggtgcactctcagtacaatctgctctgatgccgcatagttaagccagtatacactccgctatc gctacgtgactgggtcatggctgcgccccgacacccgccaacaccgctgacgcgccctgacgggcttgtctgctcccggcatccgctta cagacaagctgtgaccgtctccgggagctgcatgtgtcagaggttttCaccgtcatcaccgaaacgcgcgaggcagctgcggtaaagctc atcagcgtggtcgtgaagcgattcacagatgtctgcctgttcatccgcgtccagctcgttgagttttccagaagcgttaatgtctggcttctg ataaagcgggccatgttaagggcggttttticctgtttggtcactgatgcctccgtgtaagggggatttctgttcatgggggtaatgtaccgat gaaacgagagaggatgctcacgatacgggttacgatgatgaacagcccggttactggaacgttgtgagggtaaacaactggcggtatg gatgcggcgggaccagagaaaatcactcagggtcaatgcCagCgCttCgttaatacagatgtaggtgttccacagggtagccagcagc atcctgcgatgcagatccggaacataatggtgcagggcgctgactccgcgtttccagactttacgaaacacggaaccglagaccattca tgttgttgctcaggtcgcagacgttttgcagcagcagtcgcttcacgttcgctcgcgtatcggtgattcattctgctaaccagtaaggcaaccc cgccagcctagccgggtcctcaacgacaggagcacgatcatgcgcacccgtggggccgccatgccggcgataatggcctgcttctcgc cgaaacgtttggtggcgggaccagtgacgaaggcttgagcgagggcgtgcaagattccgaataccgcaagcgacaggccgatcacgt cgcgctccagcgaaagcggtcctcgccgaaaatgacccagagcgctgccggcacctgtcctacgagttgcatgataaagaagacagtca taagtgcggcgacgatagtcatgccccgcgcccaccggaaggagctgactgggttgaaggctctcaagggcatcggtcgagatcccgg SEQ ID Sequence Use NO. tgcctaatgagtgagct~Cactattaatgcgttgcgctcactgcccgcttccagtcgggacctgtcgtgccagctgcattgatc ggccaacgcgCggggagaggcggtttgcgtattgggcgccagggtggtttctticaccagtgagacgggcaacagctgattgCCCttc accgcctggcccigagagagttgcagcaagcggtccacgctggtttccccagcaggcgaaatcctgtgatggtggtaggcggg atataacatgagctgtcttggatcgtcgtatcccactaccgagatatccgcaccaacgcgcagcccggactcggtafltggcgcgcattg cgcccagcgccatctgatcgttggcaaccagcatcgcagtgggaacgatgccclcattcagcatttgcatggtttgllgaaccggacag gcactccagtcgccttCCCgttccgCtatcggctgaattugfftgcgagtgagatattagccagccagccagacgcagacgcgccgaga cagaacttaatgggcccgctaacagcgcgaltgctgggacccaatgcgaccagatgctccaCgcccagtcgcgtaccgtcttcatggg agaaaa.,iaatactgttgatgggtgtctggtcagagacatcagaaataacgccggaacattagtgcaggcagcttccacagcatggcatc czggtcatccagcggatagtaatgatcagcccacgacgcgtgcgcgagaagattgtgcaccgCCgctacaggcutcgacgccgctt cgttcaccatcgacaccaccacgctggcacccagttgatcggcgcgagalhtaatcgccgcgacaatttgcgacggcgcgtgcagggcc agactggaggtggcaacgccaatcagcaacgactgtttgcccgCCagttgttgtgccacgcggttgggaatgtaattcagctccgccatcg ccgcttccactttttcccgcgttttcgcagaaacgtggczggcctggttcaccacgcgggaaacggtctgataagagacaccggcatactct gcgacatcgtataacgttctggtttcacattcaccaccctgaattgactctcttccgggcgctatcatgccataccgcgaaggtttgcgcc attcgatggtgtccgggaccgacgctctcctflatgcgactcctgcattaggaagcagcccagtagtaggtgaggccgtgagcaccgc cgccgcaaggaatggtgcatgcaaggagatggcgcccaacagtcccccggccacggggcctgccaccatacccacgccgaaacaag cgctcatgagcccgaagtggcgagcccgatcttccccatcgggatgtcggcgaaaggcgccagcaaccgcactgtggcgccggtg atgccggccacgatgcgtccggcgtagaggatcg 25 agatctcgatcccgcgaaattaatacgactcactataggggaattgtgagcggataacaattcccctctagaaataattttgttactttaaga Endo-pJ aggagatataCATATGGTACCAAACAAAAGCGTAGCACCATAlrAC17GCTGCATCTAT glucanase C1-rATATGGTGGTGCTGT'TGCTCAACAGACTGTTGGGGTCAGTGTGGTGGTATTGG insertion TTGGTCTGGTCCTACCAATTGTGCTCCTGGCTCAGCATGTAGTACCTrAAATCC1'A cset CTATGCTCAATGTATI'CCAGGTGCAACAACTATAACAACATCAACTCGCCCTCC1TC AGGTCCAACTACAACAACTCGTGCTACTAGCACU'CTAGCAGCACACCTCCTACATC (pET-2 1 a 1-rCTGGAGTACGT CGCTGGTGTAATATTGCAGGITTCGA1TrGGTGTACTACC BDO5) GATGGTACATGTGTTACCAGTAAAGTTATCCCCCTITAAAAAATIACTGGCTCA AACAATrATCCAGATGGCATTGGTCAAATGCAACACMrGTAAATGAAGATGGTAT GACTATrCCGTTrACCAGTGGGCTGGCAATACTTAGTrAACAACAA1TrrAGGTGG TAAC'FrAGATAGTACATCAA'ITAGTAAATATGATCAATTAGTACAAGGTI'GCTTATC M~AGGTGCCTA1TGTATrGTTGATAFrCATAATTATGCCCGT'TGGAACGGTGGTA1T ATTGGTCAAGGTGGTCCAACTAATGCTCAA1TACATCAn7ATGGAGCCAATrAGCT TCAAAATATGCTAGTCAATCACGTGTTGGTICGGTATrATGAATGAACCTCACGAT GTGAACATAAATACTrGGGCTGCAACTGTGCAAGAAGTAGTAACTGCTAn7CGTAA TGCTGGTGCAACATCACAA1TCATTAG'ITACCAGGCAACGATrGGCAATCTGCCGG CGC7-FrA1CTGACGGTAGCGCAGCTGCTCTTAGTCAAGTGACTAACCCAGACGG TAGTACCACTAAC~rAATA17CGATGTACATAAATATC1TGA~rCTGATAATAGCGG AACACACGCCGAATGTACCACAAATAATATI'GATGGTGC1TIAGTCC1TI'AGCAAC TTGGTTACGTCAAAATAATCGCCAAGCCATrAACTGAAACAGGTGGTGGAAACG TGCAGAGTTGTATCCAAGACATGTGTCAACAAAT-rCAGTAC1TAAATCAAAACTCT GACGTGTACTAGGTTATGTAGG'rrGGGGTGCTGG1TrCTGATCAACrT7ATGTA TTAACCGAAACCCCTAC'rC1TrCTGGAAACTCATGGACAGACACTrCA1TAGTAAGT AGTIG1TT7AGCTCGCAAGGGTACCGGTGAAAACTflATACTICAAGGCTCAGGTGG CGGTGGAAGTGATITACAAAGATGATGATGATAAAGGAACCGGtT'AATCTAGACTCG AGcaccaccaccaccaccactgagatccggctgctaacaaagcccgaaaggaagctgagtggctgctgccaccgctgagcaataacl SEQ ID Sequence Use NO. agcataaccccttggggcctc2lCkgggtcttgaggggttttttgctgaaaggaggaactatatccggattggcgaatgggacgcgccct gtagcggcgcataagcgcggcgggtgtggtggtcgcgcagcgtgaccgcacaflgccagcgccctagcgcccgctccitcgctt tcttccLcttctctcgccacgtcgccggttccccgtcaagctctaaatcgggggctccctttagggtccgattagtgctttacggcacc tcgaccccaaaaacttgattagggtgatgttcacgtagtgggccatcgccctgatagacggtnttcgccc1itgacgttggagtccacgtt ct~atgccttcaatgaacccactttcgcatttgtttagattcgttgctt ggtannggtatacaattaggattan~atnagtaattaggccitggaagg grgaccttttttittatctcattttcgtaggcaaC~gtatctataataaa gaagagtatgagtattcaacatttccgtgtcgcccttattcccttttttgcggcattttgccttccgtttitgctcacccagcgctggtgaa gtaaaagatgctgaagatcagttgggtgcacgagtgggtcatgaactggatctcacagcggtagatccttgagagttttcgccccga agaacgttttccaatgatgagcactttaaagttctgctatgtggcgcggtattatcccgtattgacgccgggcagagcaactcggtcgccg catacactattctcagaatgacttggttgagtactcaccagtcacagaagcatcttacggatggcatgacagtaagagaatatgcagtgc tgccataaccatgagtgataacactgcggccaactacttctgacaacgaLcggaggaccgaaggagctaaccgctttttgcacaacatgg gggatcatgtaactcgccttgatcgttgggaaccggagctgaatgaagccataccaaacgacgagcgtgacaccacgatgcctgcagca atggcaacaacgttgcgcaaactattaacggcgactacttactctagcttcccggcaacaataatagactggatggaggcggataaagt tgcaggaccacttctgcgctcggcccttccggctggctggtttattgctgataaatctggagccggtgagcgtgggtctcgcggtatcattgc agcactggggccagatggtaagccctcccgtatcgtagttatctacacgacggggagcaggcactatggatgaacgaatagacagat cgtaaaggcccgtagatgacgcgcagttccttlc~tgtgttaatctttata aaggatctaggtgaagacctttttgataatctcatgaccaaaatcccttaacgtgagttttcgtccactgagcgtcagaccccgtagaaaag atcaaaggatcUttgagatcctttttttctgcgcgtaatctgctgcttgcacaaaaaccCgctaccagcggtggtttgttgccgga tcaagagctaccaactctttcegaaggtaactggcttcagcagagcgcagataccaatactgtccttctagtgtagccgtagttaggcca ccacttcaagaactctgtagcaccgcctacatacctcgctctgctaatcctgttaccagtggctgctgccagtggcgataagtcgtgtcttacc gggttggactcaagacgatagtuaccggataaggcgcagcggtcgggctgaacggggggttcgtgcacacagcccagcttggagcgaa cgacctacaccgaactgagaacctacagcgtgagctatgagaagcgccacgcttcccgaagggagaaaggcggacaggtatccggt aagcggcagggtcggaacaggagagcgcacgagggagcttccagggggaaacgccggtatctttatagtcctgtcgggtttcgccacc tctgacttgagcgtcgattttggatgctcgtcaggggggCggagcctatggaaaaacgccagcaacgcggccttttacggttcctggcc ttttgctggccttutgctcacatgltutcctgcgttatcccctgattctgtggataaccgtattaccgcctttgagtgagctgataccgctcgccg cagccgaacgaccgagcgcagcgagtcagtgagcgaggaagcggaagagCgccgatgcggtatttictctacgcatctgtgcggta tttcacaccgcatatatggtgcactctagtacaatctgctctgatgccgcatagttaagccagtatacactccgctacgctacgtgactggg tcatggctgcgccccgacccgccaacacccgcgacgcgccctgacgggcttgtctgctcccggcatccgcttacagacaagctgtg accgtctccgggagctgcatgtgtcagaggttttcaccgtcatcaccgaaacgcgcgaggcagctgcggtaaagctcacagcgtggtcg tgaagcgattcacagagtcgcctgtcatccgcgtccagctcgttgagLttccagaagcgttaatgtctggcttctgataaagcgggcca Cttaagggcggtuttttcctgtttggtcactgatgcctccgtgtaagggggaltctgttcatgggggtaatgataccgatgaaacgagagag gatgctcacgatacgggttactgatgatgaacatgcccggttactggaacgttgtgagggtaacaactggcggtatggatgcggcggga ccagagaaaaacactcagggtcaatgccagcgcttcgtuaatacagatgtaggtgttccacagggagccagcagcatcctgcgatgca gatccggaacataatggtgcagggcgctgacttCcgcgtttccagactacgaaacacggaaaccgaagaccattcatgttgttgctcagg tcgcagacgttttgcagcagcagtcgcttcacgtcgctcgcgtatcggtgatcactgctaaccagtaaggcaaccccgccagcctagc cgggtcctcaacgacaggagcacgatcatgcgcacccgtggggccgccatgccggcgataatggcctgcttctcgccga.3cgitiggt ggcgggaccagtgacgaaggcttgagcgagggcgtgcaagattccgaataccgcaagcgacaggccgatcatcgtcgcgctccagcg aaagcggtcctcgccgaaaatgacccagagcgctgccggcacctgtccLacgagttgcatgataaagaagacagtcataagtgcggcga cgatagtcatgccccgcgcccaccggaaggagctgactgggttgaaggctctcaagggcatcggtcgagatcccggtgcctaatgagtg agctaacttacattaattgcgttgcgctcactgcccgctttCCagtcgggaaacctgtcgtgccagctgcattaatgaatcggccaacgcgcg gggagaggcggttgcgtattgggcgccagggtggtt~tttcttaccagtgagacgggcaacagctgattgcccttcaccgcctggccct gagagagttgcagcaagcggtccacgctggttgccccagcaggcgaaaatCcgtttgatggtggttaacggcgggatataacatgagc S§E QI D Sequence Use NO. tgtcttcggtatcgtcgtatcccactaccgagatatccgcacacC~gcgcagcccgatggatggctgcgcgattgcgccagcgccat gcccgctaacagcgcgatttgctggtgacccaagcgaccagatgctccacgcccagtcgcgtaccgtcttcatgggagastatactg ttgatgggtgtctggtcagagacatcaagaataacgccggaactagtgcaggcagcttccacagcatggcatcctggtcatccagcg gatagttaatgatcagcccactgacgcgttgcgcgagagattgtgaccgccgctttacaggctcgggcttcgttctaccatcgac accaccacgctggcacccagttgatcggcgcgagatttaatcgccgcgacaatttgcgacggcgcgtgcaggccagactggaggtgg caacgccaatcagcaacgactgttgcccgccagttgttgtgccacgcggtgggaatgtaattcagctccgccatcgccgcttccactitc cccgcgttttcgcagaaacgtggctggcctggttcaccacgcgggacggtctgataagagacaccggcatactctgcgacatcgtata acgttactggtcacattcaccaccctgaattgactctcttccgggctatcatgccaaccgcgaaggttttgcgccattcgatggtgtcc gggatctcgacgcItccccttatgcgactcctgcattagggagcccagtagaggtgaggccgttgagcaccgccgccgcaaga tggtgcatgcaaggagatggcgcccaacagtcccccggccacggggcctgccaccatccacgccgaacagcgctcatgagccc gaagtggcgagcccgatcttccccatcggtgatgtcggcgatataggcgccagcaaccgcaccgtggcgccggtgatgccggccacg atgcgtccggcgtagaggatcg 26ttgtcggatatcatacaaggattacgtaatccccaaaattgtactag P -giuo aggagatataCATATGGTACCA1TACCAAAGGA1TICCAATGGGGmTCGCTACCGCAGC sidase nATCAAAnGAAGGTGCAGTrGATCAAGATGGACGTGGACCnrCTAMGGGACA setn CATTCTGTGCACAACCAGGTAAAA'ITGCTGATGGn7CATCAGGTGTAACAGCATGT cset GACTCATATAATCGTACAGCTGAAGACA7GCACfl=AAAATCTTAGGTGCTAAA (pT21 TCATATCG1TCTCTATCTCATGGTCAAGAATrATTCCTGAAGGTGGCCGTGGTGAC pT2Ia GCAGTAAATCAAGCTGGTATGATCACTATGTrAAATIGTAGATGAC'I1AUAGAC BDO9) GCAGGTATrACACC-rTATCAC1TA-Tr7CACTGGGA'TrACCTGAAGGT'I7ACACC AACGTTATGGTGGTCTn-AAACCGTACAGAA1TrCCTIAGA1CGAAAACTATG CAAGAGTTATGTTCGTGCAC1TCCCAAAGTAAGAAACTGGATAC=AATGAAC C.I1TATGTnCTGCTATTCCTGGnrATGGTUCAGGCACCmGCCCCAGGCAGACAAA GTACAAGTGAGCCCTGGACAGTGGGCCATAACA1TIAGTAGCTCACGGTAGAGCT GTAAAAGCATATAGAGATGA I I IAAACCTGCTTCAGGTGATGGTCAAATAGGTAT TGTGTfAAATGGTGACTTCACATATCCCTGGGATGCCGCTGATCCTGCAGATAAAGA AGCCGCTGAACGTCGCTAGAATCACTGC~rGGTI7GCTGACCCCATTATCTT GGTGA~rATCCTGCTTCAATGCGTAAACAATVFAGGTGATCGTrACCTACTm'ACA CCAGAAGAACGTGCmAGTrCATGGTAGTAATGAC=ATGGTATGAACCACT'AT ACYTrCAAACTATATCGTCACCGTAGCTCACCCGCAAGTGCTGATGACACAGTAGGT AATGTAGATG I II 'A1TIACTAATAAACAAGGTAATlGTATCGGTCCTGAAACACAG AGCCCCTGGCrCGTCC17GTGCAGCTGG1TrrCCGTGACTICCTrGTATGGATAAGC AAACGTATGGTITATCCACCAATTATGUrACAGAAAACGGAACATCAATAAAAGG TGAAAGTGACTTACCAAAGGAAAAGATCTTGAAGATGA1TrCGTG1TAAGTA1T ATAACGAATACATTAGAGCTATGGUrACAGCCGTUGAATUAGATGGTGTAAATGTA AAAGGTATCGCATGGTCTrAATGGATAAC1TGAATGGGTGATGGnTACGTT ACACGT1TGGTGTAACCTACGT-GA1TACGAAAACGGCCAAAAACGT1TCCCTAA AAAGAGTGCTAAAAGTFAAAACCT1TAMGATGAArAATAGCTGCTGCAGGTA CCGGTGAAAACTTATACTCAAGGCTCAGGTGGCGGTGGAAGTGAnrACAAAGAT GAGTAAAGACGTACAATG~accaccaccggtcgt ctaaagcg____________tcacgtagatacacaaccctggct~aaggttg SEQ ID Sequence Use NO. ggggttttllgctgaaggaggaacatatccggattggcgaatgggacgcgccctgtgcggcgcattaagCgcggcgggtgtggiggt tacgcgcagcgtgaccgctacacttgccagcgcccagcgcccgctcctttcgctttcttcccttcctttctcgccacgttcgccggctttccc cgtcaagctctaaatcgggggctccctttagggttccgatttatgctacggcacctcgaccccnaaaaacttgaltagggtgatggttcac gtagtgggccatCgccctgatagacggtttttcgccctttgacgttggagtccacgttcttatagtggactcttgttccaaactggaacac ctcaaccctatctcggtctaldlttigatataagggattttgccgattcggcctattggttaaaaatgagctgatttaacnaaaaaltaacgc gaattttaacannatataacgtttacaatttcaggtggactttcggggaatgtgcgcggaacccctatttgtttatttctaatacattc3.a atatgtatccgctcatgagacaataaccctgataalgctcaataatattgaaaaggaagagaigagtatcaacatttccgtgtcgcccit attcccttttttgcggcattttgccttcctgtttttgctcacccagaaCgctggtgaaagtaaaagatgctgaagatcagttgggtgcacgagt gggttacatcgaactggatctcaacagcggtagtccttgagagttttcgccccgaagaacgtttccaatgatgagcacitttaaagttctg ctatgtggcgcggtattatcccgtattgacgccgggcaagagcaactcggtcgccgcatacactattcagatgacttggttgagtactca ccagtcacagaaaagcatcttacggatggcatgacagtaagagaatatgcagtgctgcacaaaccatgagtgataacacgcggccaact taclttctgacaacgatcggaggaccgaaggagctaaccgcttttttgcacaacatgggggatcatgtaaccgcctgatcgttgggaaccg gagctgaatgaagccataccaaacgacgagcgtgacaccacgatgcctgcagcaatggcaaacgttgcgcaaactattaflctggcga actacttactctagcttcccggcaacaattaatagactggatggaggcggataaagttgcaggaccacttctgcgctcggcccttccggctg gctggtttattgctgataatctggagccgggagcggggtctgcggtatcattgcagcactggggccagaggtaagcccLcccgtatc gtagttatcacacgacggggagtcaggcaactatggatgaacgaaatagacagatcgctgagataggtgcctcactgalt82gcattggt aactgtcagaccaagitactcatataacitagatgattaaaacticaLtttaatttaaaaggatctaggtgagaccttttgataatctat gaccaaaatcccttaacgtgagttttcgttccactgagcgtcagaccccgtagaaagatcaagatcttctgagatccttttttctgcgcg taatctgctgcttgcaaacaaaaaaaccaccgctaccagcggtggtttgttgccggatcaagagctaccaactctttttccgaaggtaactg gcttcagcagagcgcagataccaaatactgtcctctagtgtagccgtagttaggccaccacttcagaactcgtagcaccgcctacatac ctcgctctgctaatcctgttaccagtggctgctgccagtggcgataagtcggcttaccgggttggactcaagacgatagttac cggataag gcgcagcggtcgggctgaacgggggggLgtgcacacagcccagcttggagcgaacgacctacaccgaactgagatacctacagcgt gagctatgagaaagcgccacgcttcccgaagggagaaaggcggacaggtatccggtaagcggCagggtcggaacaggagagcgcac gagggagcttccagggggaaacgcctggtatctttatagtcctgtcgggtttcgccacctctgactigagcgtcgatttttgtgatgctcgtca ggggggcggagcctatggaaaacgccagcaacgcggcctttttacggttcctggcctttgcggcdtttgctcacatgttctttcctgcgt tatcccctgattctgtggaaaccgataccgccttgagtgagcgataccgctcgccgcagccgaacgaccgagcgcagcgagtcagt gagcgaggaagcggaagagcgcctgatgcggtattctcctacgcatctgtgcggtatttcaCaccgcatatatggtgcactctcagtaca atctgctctgatgccgcatagtaagCcagtatacactccgctatcgctagcgtgctgggtcatggctgcgccccgacacccgccaacacc cgctgacgcgccctgacgggcttgtctgctcccggcatccgcttacagacaagctgtgaccgtctccgggagctgcatgtgtcagaggttt tcaccgtcatcaccgaaacgcgcgaggcagctgcggaaagctcatcagcgtggtcgtgaagcgattcacagatgtctgcctgttcatccg cgtccagctcgttgagtttctccagaagcgttaatgtctggcttctgataaagcgggccatgttaagggcggttttcctgtttggtcactgatg cctccgtgtaagggggattctgttcagggggtaatgataccgatgaalcgagagaggatgctcacgatacgggtactgatgatgaacat gcccggttactggaacgttggagggtaaacaactggcggtatggagcggcgggaccagagaaaaatcactcagggtcaatgccagc gcttcgttaatacagatgtaggtgttccacagggtagccagcagcatcctgcgatgcagatccggaacataatggtgcagggcgctgact ccgcgttccagacttacgaaacacggaaaccgaagaccatcaggtgctcaggtCgcagacgtttgcagcagcagtcgcttcacgt tcgctcgcgtatcggtgattcattctgctaaccagtaaggcaaccccgccagcctagccgggtcctcaacgacaggagcacgatcatgcg cacccgtggggccgccatgccggcgaaatggcctgCtttcLgccgaaacgtttggtggcgggaccagtgacgaaggcttgagcgagg gcgtgcaagatccgaataccgcaagcgacaggccgaicatcgtcgcgctccagcgaaagcggtcctcgccgaaaalgacccagagcg ctgccggcacctgtcctacgagtgcatgataaagaagacagtcataagtgcggcgacgaagtcatgccccgcgcccaccggaaggag ctgactgggttgaaggctctcaagggcatcggtcgagatcccggtgcctaalgagtgagctaacttacttaatgcgttgcgctcactgcc cgctttccagtcgggaaacctgtcgtgccagctgcattaatgaatcggccaacgcgcggggagaggcggtttgcgtattgggcgccagg gtggtttcttttcaccagtgagacgggcaacagctgattgccctcaccgcctggccctgagagagttgcagcaagcggtccacgctggt ttgccccagcaggcgaaaatcctgtttgatggtggttaacggcgggatataacagagctgcttcggtatcgtcgatcccactaccgagat SEQ ID Sequence Use NO. atccgcaccaacgcgcagcccggactcggtaatggcgcgcattgcgcccagcgccatctgatgttggcaaccagcategcagtggga acgatgccctcattcagcatttgcaggtttgttgaaaaccggacatggcactccagtcgccttcccgttccgtatggctgaatttgattgc gagtgagatatttatgccagccagccagacgcagacgcgccgagacagaacttaatgggcccgctaacaggcgatttgtggtgaccc aatggaccagatgtccacgcccagtcgcgtaccgtcttcatgggagaaaatactgttgatgggtgtctggtcagagacatcaagaa ataacgccggaacattagtgcaggcagttccacagcaatggcatcctggtcatccagcggatagttaatgatcagcccactgacgcgttg cgcgagaagattgtgcaccgccgctttacaggttgagcgccttcgtttaccatcgacaccaccacgctggcacccagttgatcggcg cgagatttaatcgccgcgacaatttgcgacggcgcgtgcagggccagactggaggtggcaacgccaatcagcaacgactgtttgcccgc cagttgttgtgccacgcggttgggaatgtaattcagctccgccatgccgcttccactttttcccgcgttttcgcagaaacgtggctggcctgg ttcaccacgcgggaaacggttgataagagacaccggcatactctggacatgtataagttactggtttcacattcaccaccctgaattga ctctcttccgggcgtatcatgccataccgcgaaaggttttgcgccattgatggtgtcgggattcgacgtctcccttatgcgactcctgc attaggaagcagcccagtagtaggttgaggccgttgagcaccgccgccgcaaggaatggtgcatgcaaggagatggcgcccaacagtc ccccggccacggggcctgccaccatacccacgccgaaacaagcgctcatgagcccgaagtggcgagcccgatcttccccatcggtgat gtcggcgatataggcgccagcaaccgcacctgtggcgccggtgatgccggccacgatgcgtccggcgtagaggatcg 27 agatctcgatcccgcgaaattaatacgactcactataggggaattgtgagcggataacaattcccctctagaaataattttgtttaactttaaga Endo aggagatataCATATGGTACCAGTATCTITCACAAGTCTTTAGCAGCATCTCCACC17CA xylanase CGTGCAAGTTGCCGTCCAGCTGCTGAAGTGGAATCAGTTGCAGTAGAAAAACGTCA insertion AACAATTCAACCAGGTACAGGTrACAATAACGGTTACTITTATCTrACTGGAATGA cassette TGGACACGGTGGTGTTACATATACTAATGGACCTGGTGGTCAATITAGTGTAAATrG GAGTAACTCAGGCAATITIIGTTGGAGGAAAAGGTrGGCAACCTGGTACAAAGAATA (pET-2 Ia AGGTAATCAATITrCTCTGGTAGTrACAACCCTAATGGTAATTCTrATITAAGTGTAT BDIl) ACGGTTGGAGCCGTAACCCATrAATGAATATrATATIGTAGAGAACITGGTACAT ACAACCCTfCAACAGGTGCTACTAAATrAGGTGAAGTTACTrCAGATGGATCAGTT ATGATATTATCGTACTCAACGCGTAAATCAACCATCTATAATTGGAACTGCCACTr TCTACCAATACTGGAGTGTAAGACGTAATCATCGTTCAAGTGGTAGTGTTAATACA GCAAACCACTTrAATGCATGGGCTCAACAAGGTTAACATAGGTACAATGGACTA TCAAATrGTAGCTGTTGAAGGTrATTI ICATCAGGTAGTGCTTCTATCACTGTTAGC GGTACCGGTGAAAACTATACTITCAAGGCTCAGGTGGCGGTGGAAGTGATTACAA AGATGATGATGATAAAGGAACCGGTTAATCTAGACTCGAGcaccaccaccaccaccactgagatc cggctgctaacaaagcccgaaaggaagtgagttggtgtgccaccgctgagcaataactagataaccccttggggcctctaaacgg gtcttgaggggttttttgctgaaaggaggaactatatccggattggcgaatgggacgcgccctgtagcggcgcattaagcgcggcgggtgt ggtggttacgcgcagcgtgaccgctacacttgccaggccctaggcccgtccttcgctttcttcccttcctttctegccacgttcgccgg ctttccccgtcaagctctaaatcgggggtccctttagggttccgatttagtgtttacggcacctcgaccccaaaaaattgattagggtgat ggttcacgtagtgggccatgccctgatagacggtttttgccctttgacgttggagtccacgttctttaatagtggactcttgttccaaactgg aacaacactcaaccctattcggtctattcttttgatttataagggattttgccgatttcggcctattggttaaaaaatgagctgattaacaaaaat tnaacgcgaattttaacaaaatattaacgtttacaatttcaggtggcacttLtCggggaaatgtgcgcggaacccctatttgtttatttttctaaata cattcaaatatgtatccgtcatgagacaataaccctgataaatgettcaataatattgaaaaaggaagagtatgagtattcaacatttccgtgt cgcccttattcccttttttgcggcattttgccttcctgtttttgctcacccagaaacgctggtgaaagtaaaagatgctgaagatcagttgggtgc acgagtgggttacatcgaactggattcaacagggtaagatccttgagagtttcgccccgaagaacgttttccaatgatgagcacttttaa agttctgctatgtggcgcggtattatcccgtattgacgccgggcaagagcaactcggtcgccgcatacactattctcagaatgacttggttga gtactcaccagtcacagaaaagcatcttacggatggcatgacagtaagagaattatgcagtgctgccataaccatgagtgataacactgcg gccaacttacttctgacaacgatcggaggaccgaaggagctaaccgcttttttgcacaacatgggggatcatgtaactcgccttgatcgttg ggaaccggagtgaatgaagccataccaaacgacgaggtgacaccacgatgcctgcagcaatggcaacaacgttgcgcaaactatta actggcgaactactactctagettcccggcaacaattaatagactggatggaggggataaagttgcaggaccacttctggctcggccct SEQ ID Sequence Use NO. tccggctggctggtttattgctgataaatctggagccggtgagcgtgggtctcgcgglatcattgcagcactggggccagatggtaagccct cccgtatCgtgttatctacacgacggggagtcaggcaactatggatgaacgaaatagacagatcgctgagataggtgcctcactgattaa gcattggtaactgtcagaccaagtttactcatatatttagattgatttaaaacttcatttttaatttaaaaggatctaggtgaagatcctttttgat aatctcatgaccaaaatcccttaacggagtttcgttccactgagcgtcagacccgtagaflaagatcaaaggatctttgagatccttttttt ctgcgcgtaatctgctgCttgCaaacaaaacCaCCgcaccagcggtggittgttgccggatcagagctaccactctttttccgaag gtaactggcttcagcagagcgcagataccaatactgtrcttctagtgtagccgtagtaggccaccacttcagaactctgtagcaccgcc tacatacctcgctctgctaatcctgttaccagtggctgctgccagtggcgataagtCgtgtcttaccgggttggactcaagacgatagttacc ggataaggcgcagcggtcgggctgaacggggggttcgtgcacacagcccagcttggagcga~cgacctacaccga.3ctgagatacct acagcgtgagctatgagaaagcgccacgcttcccgaagggagaaaggcggacaggtatccggtaagcggcagggtcggaacaggag agcgcacgaggggcttccaggggaaacgccggtatcttatagtcctgcggttcgccacctctgacttgagcgtcgatttgtgat gctcgtcaggggggcggagcctaggaaaacgccagcaacgcggccttttacggttcctggcctttgctggccttttg~tcacatgttct ttcctgcgttatccctgattctgtggataaccgtataccgccitgagtgagcgataccgctcgccgcagccgaacgaccgagcgcagc gagtcagt gagcgaggaagcggaagagcgcctg atgcggtattttctccttacgcatctgtgcggtatttcacaccgcatatatggtgc act ctcagtacaatctgctctgatgccgcatagttaagccagtatacactccgcatcgctacgtgactgggtcatggctgcgCCCCgacacccg ccaacacccgctgacgcgccctgacgggcgtctgctcccggcatccgcttaCagacaagctggaccgtctccgggagctgcatgtgt cagaggCtttcaccgtcatcaccgaaacgcgcgaggcagctgcggtaaagctcatcagcgtggtcgtgaagcgatcacagatgtctgcct gttcaccgcgtccagctcgtgagttccagagcgttaatgtctggcttctgataagcgggccatgttaagggcggttttttcctgtttgg tcactgatgcctccgtgtaagggggaittctgtcatgggggtaatgataccgatgaaacgagagaggatgctcacgatacgggttactgat gatgaacatgcccggttactggaacgttgtgagggtaaaCaactggcggatggatgcggcgggaccagagaaaatcactcagggtca atgccagcgcttcgtatacgatgtaggtgttccacagggtagccagcagcatcctgcgatgcagatccggacatatggtgcaggg cgctgacticcgcgtttccagactttacgaaacacggaaaccgaagaccattcatgttgttgCtcaggtcgcagacgttttgcagcagcagtc gcttcacgttcgctcgcgtatcggtgatcattctgctfaaccagtaaggcaaccccgccagcctagccgggtcctcaacgacaggagcacg atcatgcgcacccgtggggccgccatgccggcgataatggcctgctctcgccgacgttggtggcgggaccagtgacgaaggcttg agcgagggcgtgcagattccgaaaccgcaagcgacaggccgatcatcgtcgcgctccagcgaaagcggtcctcgccgaaaatgacc cagagcgctgccggcacctgtcctacgagttgcatgataaagaagacagtcataagtgcggcgacgatagtcatgccccgcgcccaccg gaaggagctgactgggttgaaggctctcaagggcatcggtcgagatcccggtgcctaatgagtgagctactacattaatgcgttgcgct cactgcccgctttccagtcgggaaacctgtcggccagctgcattaatgaatcggccaacgcgcggggagaggcggtttgcgtattgggc gccagggtggtttttctttcaccagtgagacgggcaacagctgattgcccttcaccgCCtggccctgagagagttgcagcaagcggtcca cgctggtttgccccagcaggcgaatncctgttgatgtggtaacggcgggatataacatgagctgtcttcggtatcgtcgtatcccacta ccgagatatccgcaccaacgcgcagcccggactcggtaatggcgcgcatgcgcccagcgccatctgatcgttggcaaccagcatcgca gtgggaacgatgccctcattcagcattgcatggttgttgaaaaccggacatggcactccagtcgccttcccgttccgctatcggctgaatt gattgcgagtgagatattatgccagccagccagacgagacgcgccgagacagaactaatgggcccgctaacagcgcgatttgctggt gacccaatgcgaccagatgctccacgcccagtcgcgtaccgtcttcCagggagaaaataatactgttgatgggtgtctggtcagagacatc aagaaataacgccggaacattagtgcaggcagcttccacagcaatggcatcctggtcatccagcggatagtaatgatcagcccactgac gcgttgcgcgagaagattgtgcaccgccgcttacaggcttcgacgccgcttcgttctaccatcgacaccaccacgctggcacccagttga tcggcgcgagatttaatcgccgcgacaatttgcgacggcgcgtgcagggccagactggaggtggcaagccatcagcaacgactgttt gcccgccagtttgtgccacgcggtgggaatgtaattcagctccgccatcgccgcttccactttcCgCgtttcgcagaaacgtggct ggcctggttcaccacgcgggaaacggtctgataagagacaccggcatactctgcgacatcgtataacgttactggtttcacattcaccaccc tgaattgactctcttccgggcgctatcatgccaaccgcgaaggtttgcgccattcgatgggtccgggatctcgacgctctccctagcg actcctgcattaggaagcagcccagtagtaggttgaggccgttgagcaccgccgccgcaaggaatggtgcatgcaaggagatggcgcc caacagtcccccggccacggggccgccaccatacccacgccgaaacaagcgctcagagcccgaagtggcgagcccgatcttcccc atcggtgatgtcggcgatataggcgccagcaaccgcacctgtggcgccggtgatgccggccacgatgcgtccggcgtagaggatcg 28 GTGCACTCTCAGTACAATCTGCTCTGATGCCGCATAGU-AAGCCAGCCCCGACACCC Endo-p- SEQ ID Sequence Use NO. GCCAACACCCGCTGACGCGCCCTGACGGGCTGTCTGCTCCCGGCATCCGCTIACA glucanase GACAAGCTGTGACCGTCTCCGGGAGCTGCATGTGTCAGAGG=IICACCGTCATCAC insertion CGAAACGCGCGAGACGAAAGGGCCTCGTGATACGCCTATITIATAGG1TAATGTC cassette ATGATAATAATGGTrCT-rAGACGTCAGGTGGCACT1TCGGGGAAATGTGCGCGG (pSE AACCCCTA1TTG1TI'A1TI1CTAAATACA1TrCAAATATGTATCCGCTCATGAGACA 3BK ATAACCCTGATAAATGC1?TCAATAATATGAAAAAGGAAGAGTATGAGTA'TrCAAC AJI iTICGTGTCGCCCTATCCC'FIr1GCGGCA1TIGCCTrCCTGTI=GCTCAC rbcL:BDO CCAGAAACGCTGGTGAAAGTAAAAGATGCTGAAGATCAGU7GGGTGCACGAGTGG 5) GrrACATCGAACTGGATCTCAACAGCGGTAAGATCCTrGAGAGrFICGCCCCGAA GAACGTTMCCAATGATGAGCACTMAAAG~rCTGCTATGTGGCGCGGTA1TATCC CGTA1TGACGCCGGGCAAGAGCAACTCGGTCGCCGCATACACTATTCTCAGAATGA CT-rGGTFGAGTACTCACCAGTCACAGAAAAGCATCITACGGATGGCATGACAGTAA GAGAATTATGCAGTGCTGCCATAACCATGAGTGATAACACTGCGGCCAAC11ACnT CTGACAACGATCGGAGGACCGAAGGAGCTAACCGC'FIITGCACAACATGGGGGA TCATGTAACTCGCCTTGATCGTTGGGAACCGGAGCTGAATGAAGCCATACCAAACG ACGAGCGTGACACCACGATGCCTGTAGCAATGGCAACAACGTTGCGCAAACTATTA ACTGGCGAACTACTTACTCTAGC1TCCCGGCA.ACAA1TAATAGACTGGATGGAGGC GGATAAAGTTGCAGGACCACTrCTGCGCTCGGCCCTCCGGCTGGCTGG11TA1TGC TGATAAATCTGGAGCCGGTGAGCGTGGGTCTCGCGGTATCAT-rGCAGCACTGGGGC CAGATGGTAAGCCCTCCCGTATCGTAG11'ATCTACACGACGGGGAGTCAGGCAACT ATGGATGAACGAAATAGACAGATCGCTGAGATAGGTGCCTCACTGATlAAGCATTG GTAACTGTCAGACCAAG1TACTCATATATACTrrAGATGATAAAACTTCATTT TAATAAAAGGATCTAGGTGAAGATCC'FI1TGATAATCTCATGACCAAAATCCCT TAACGTGAGTIMCGTCCACTGAGCGTCAGACCCCGTAGAAAAGATCAAAGGATC T7C TGAGATCC 1I I ICTGCGCGTAATCTGCTGCTrGCAAACAAAAAAACCACC GCTACCAGCGGTGG1TGTTGCCGGATCAAGAGCTACCAACTC1TITCCGAAGGT AACTGGC11CAGCAGAGCGCAGATACCAAATACTGUrCTrCTAGTGTAGCCGTAGTfl AGGCCACCACTnCAAGAACTCTGTAGCACCGCCTACATACCTCGCTCTGCTAATCCT GTITACCAGTGGCTGCTGCCAGTGGCGATAAGTCGTGTC'FIACCGGGTrGGACTCAA GACGATAGnrACCGGATAAGGCGCAGCGGTCGGGCTGAACGGGGGGTUCGTGCAC ACAGCCCAGCTTGGAGCGAACGACCTACACCGAACTGAGATACCTACAGCGTGAGC TATGAGAAAGCGCCACGCTITCCCGAAGGGAGAAAGGCGGACAGGTATCCGGTAAG CGGCAc3GGTCGGAACAGGAGAGCCCACGAGGGAGCTCCAGGGGGAAACGCCTGG TATC1-ITATAGTCCTGTCGGG1TCGCCACCTCTGACTrGAGCGTCGATITITGTGAT GCTCGTCAGGGGGGCGGAGCCTATGGAAAAACGCCAGCAACGCGGCC'T-rACGG TrCCTGGCC=rIGCTGGCCT1rGCTCACATG77CI=CCTGCG1TATCCCCTGATrC TGTGGATAACCGTA'FrACCGCC7TTGAGTGAGCTGATACCGCTCGCCGCAGCCGAA CGACCGAGCGCAGCGAGTCAGTGAGCGAGGAAGCGGAAGAGCGCCCAATACGCAA ACCGCCTCTCCCCGCGCGTrGGCCGATrCATTAATGCAGCTGGCACGACAGG1TICC CGACTGGAAAGCGGGCAGTGAGCGCAACGCAATfAATGTGAGTTAGCTCACTCAT AGGCACCCCAGGCTTACACTI'ATGCI'CCGGCTCGTATG1TGTGTGGAA1-rGTGA GCGATAACAATTCACACAGGAAACAGCTATGACCATGATACGCCaagctcgcggccgc agtactCTGCAGATATGCAAAAT'AAAGTC1TrGTGACAACAGCTITCTCC11AAGTG SEQ ID Sequence Use NO. CAAATATCGCCCAITCTITCCTC1TMCGTATATAAATGCTGTAATAGTAGGATGTC GTACCCGTAAAGGTACGACATGAATATrAATATACTCCAAGnTACTMCCCAAT AMIATA1TAGGACGTCCCCITCGGGTAAATAAAFF'AGTGGCAGTGGTACCGCCA CTCCCTATIMAATACTGCGAAGGAGGCAGrGGCAGGCAACTCGTCGTrCGCAGTA TATAAATATCCACTAATA1ATA1TCCCGTAAGGGGACGTCCCGAAGGGGAAGGG GAAAGAAGCAGTCGCCTCC~rGCGAAAAGG11TACT-rGCCCGACCAGTGAAAAGCA TGCTGTAAGATATAAATCTACCCTGAAAGGGATGCATICACCATAATACTATACA AATGGTGTI'ACCC1TGAGGATCATAACGGTGCTACTGGAATATATGGTCTC1TCAT GGATAGACGATAGCCATTrATrACCCATTAAGGGGACArAGTGGCCTGTCACTGC TCCT-rACGAGACGCCAGTGGACGrrCGTCCTAGAAAA1TTATGCGCTGCCTAGAAG CCCCAAAAGGGAAGMIACTGACTCGTTAGAGCGTGCGCTAACAGG1TrAAATACT TCAATATGTATATrAGGACGCCGGTGGCAGTGGTACCGCCACTGCCACCGTCGGAG GACGTCCCTrrACGGTATATTATATACTAGGATI=AATACTCCGAAGGAGGCAGTGG CGGTACCACTGCCACTAATATI1ATATTCCCGTAAGGGACGTCCTCCTlCGGAGTAT GTAAACATrCTAAG1TrACTrGCCCAATA1ATATTAGGCAGTGGCAGGCAACTG CTAGCTCTCCTCCITCGGAGTATGTAAACATCGCAGTATATAAATATCCACTAATAT TTATA'ITCCCGTAAGGGGACGTCCCGAAGGGGAAGGGGAAGGACGTCAGTGGCAG TrGCCTGCCAACTGCCTAGGCAAGTAAAC1TAGGAGTATATAAATATAGGCAGTCG CGGTACCACTGCCACTGACGTCCTGCCAACTGCCTAGGCAAGTAAACTTAAGTGGC ACTAAAATGCAMTGCCCGAAGGGGAAGGAGGACGCCAGTGGCAGTGGTACCGCC ACTGCCTCCTTCGGAGTA1T-AAAATCCTAGTATGTAAATCTGCTAGCGCAGGAAATA AA1TMATrCTATrATATCTCCGTAGGAGGTAAGTAAACCCC1TCCCCTCGGG ACGTCAGTGCAGTITGCCTGCCAACTGCCTAATATAAATATTAGACCACTAAAGTThVG GCAACTGCCAACTGTITGTCCTflCGGAGGAAAAAAAATGGTTAACTCGCAAGCAGTI AACATAACTAAAGTTIGTTACTTACCGAAGACGTTACCCTTCTCGGTrAAGGAG ACGGAGACAGTIGCACTGTGACTGCCTAGTATAGCAATI=GTITTrIATATGC TCGACAAAATGACTTTCATAAAAATATAAAGTAG1TAGCTAGflA1TITATATCACT ATAACTAGGGTTCTCAGAGGCACCGAAGTCACTTGTAAAAATAGTACTITAACTr GTAATC1TCGTGTrCTrCAAAAGGATCACGTAATT11rMGAAGGTGGACCAAAA CTAACATAAACTGAATAGCCAGTI'ACACTTAACAGAAGAAACCATAAAAAAAAGG TAAAGAAAAAAGCTGGACTrCCATAGCTCAT1TAATAATAAAATrATCTCTIMC AACATATCTCT-rAGATAGTTCAAAAGACTrGACGACTGTGTCCCACATTrAAACA AAATTAATCTACTCAAAA1TIGCCCTGAGAAAGAATAACTTAC11TCGTITIGCAG TAGCCATTCATGTCAC1TrGAAACTGTCC1TACAAAGTTAAACATrAArrAAAAAT7 ATAA1TI=ATATAACAAATA11'ATATrAAATAAAAAATGAACAAAGAACTrCTA AGATCGTCTAGTGAGTAATTAAAGAG1TIACTTACCAGACAAGGCAGFITFIC A1TCTIMAAAGCAGGCAG1T-CTGAAGGGGAAAAGGGACTGCCTACTGCGGTCCTA GGTAAATACA1TrATGCAATIMATrCTTGTGCTAGTAGGT7rCTATACTCACAAG AAGCAACCCCTUGACGAGAGAACGTTATCCTCAGAGTA1TATAATCCTGAGAGGG AATGCACTGAAGAATAT1TCCTTATITI1ACAGAAAGTAAATAAAATAGCGCTAA TAACGC'FrAATCAITrAATCAATATGGCAACAGGAAC17CTAAAGCTAAACCATC AAAAGTAAATCAGACTrCCAAGAACCTGGT-n7AGTrACACCA77AGGTACTr ACGTCCACTIAACTCAGAAGCAGGTAAAGTA11'ACCAGGCTGGGGTACAACTGTIT S-EQID Sequence Use NO. TAATGGCTGTATATCC11TA1TTGCAGCA1TCTrATTrAATCATTAGAAArrTA CAACAGT-rCTIAA1TrAGATGACGTrCTATGAG1GGGAAACTTrAGCTAAAGT TTCrAATTAT7AACACAAACATAAAATATAAAACTG1T7AAGGCTAGCTG CTAAGTCTIrC1I I1 ICGCTAAGGTAAACTA AGCAACTCAACCATATI'ATA1TCGGCA GTGGCACCGCCAACTGCCACTGGCC1TCCGUAAGATAAACGCGTggIctcacgtgACTA GTcacctagtgtcgagtggtaccgccactgcctagtatataakatatcggcagttggcaggatattatatactccgaaggaactgtagcc gataggcgaggcactgccacL~aatttatttgcctcctaacggagcatta33aLccctaagttacttgcccgtaggggaaggggacgt agagttagttgaagcaagtctagaTTAACCGGTTCCTTrATCATCATCATC1TGTAATCACT1TCCA CCGCCACCTGAGCCTTGAAAGTATAAGTITTCACCGGTACCCUTGCGAGCTAAACA ACTACTTACTAATGAAGTGTCTGTCCATGAG1TTCCAGAAGAAGTAGGGGTITCGGT TAATACATAAGT-rGAATCAAAAGAACCAGCACCCCAACCTACATAACCTAAGTACA CGTCAGAG I I IGA1TTAAGTACTGAA11GTrGACACATGTCTnGGATACAACTCT GCACGTTCCACCACCTGtI1CAGTI'AAAATGGCflGGCGATTT'GACGTAACC AAGTIGCTAAAGGACTAAAAGCACCATCAATATTATITGTGGTACATTCGGCGTGT GTrCCGCTA1TATCAGAATCAAGATATrATGTACATCGAATATAAG~rAGTGGTA CTACCGTCTGGG17AGTCAC1TGACTAAGAGCAGCTGCGCTACCGTCAGAAATAAA AGCGCCGGCAGATTGCCAATCGTITGCCTGGTAAACTAATGAAnrGTGATGT-GCAC CAGCATrACGAATAGCAG1TACTACTrCTrGCACAGTTGCAGCCCAAGTA1TATGT TCACATCGTGAGGTT'CATrCATAATACCGAACCAAACACGTGATGACTAGCATAn7 nGAAGCTAAnGGCTCCATAATGATGTAAAnGAGCATUAGUTGGACCACCT7GAC CAATAATACCACCG'TCCAACGGGCATAATTATGAATATCAACAATACAATAGGCA CCTAAAGATAAGCAACCTTGTACTAATTGATCATATrACTAATnGATGTACTATCT AAGTACCACCTAAA'FTGTTG11'AACTAAGTATIGCCAGCCCACTGGTAAACGGAA AATAGTCATACCATCTCA1T1ACAAAGTGTTGCATIGACCAATGCCATCTCGATA ATGTTGAGCCAGTAAAATITITAAAGGGGGATAAAC'TI7ACTGGTAACACATGT ACCATCGGTAGTACAACCAAAATCGAAACCTGCAATAUrAACACCAGCGAAACGTA CTCCAGAAGATGTAGGAGGTGTGCTGCTAGAAGTGCTAGTAGCACGAGUTGUGTA GITGGACCTGAAGGAGGGCGAGTGATGTrG17ATAGTTTnGCACCTGGAATACA 11'GAGCATAGTAAGGAITIAAGGTACTACATGCTGAGCCAGGAGCACAATflGGTAG GACCAGACCAACCAATACCACCACACTGACCCCAAACAGTCTG1TGAGCAACAGCA CCACCATATAAGATAGATGCAGCAAGTAATAATGGTGCTACGCTr7G1GGTACC ATatgcactttgcattacctccgtacaaattttttgatttctataagtttgcttaaataaaattttaatttttaacgtccacccatataataat aaatatggtgaaaccttaacaacaaaatccCtctgtaccatattaatccaaaagaataggacaaaagctatcccaacattLLLtaaa cagagtaaaaataatgttgttttaagaatagaattttataacttgtatttaaatagatctaatttatttgtgctaaa3attgcagttggaaagtaatt ttaaaaata atttag atc atatuatt aaataaagt g attaaaacaac ttaatcgttUL tatgttaattaaaaac at aatt t aaatcttt t tatattta aattaccttatatactactaggtgACTATGgatatctacgtaatcgatgaattcgatcccattttataactggatctcaaraCatacaaac ~ccaacaaagcaatcggcgtcaaaactttagtgciCacgacgcctgtggacgtcccccccttcccctacgggcaagtaaacttagggatt utaatgcaataaataaat tgtcctcttcgggcaaagaattLagtatttaaatagacaagggtgaaccattacttttgttaacaagtgatcttac SEQ ID Sequence Use NO. GGAATrGCCCAATATTA~rCAACAATITATCGGAAACAGCG1TIAGAGCCAAATA AAAT"TGGTCAGTCGCCATCGGATGTIT7ATTCTTAATCGAAATAATGAAACTT rrCT'AAGCGATCTAGCAC1TATATACAGAGACCACATACAGTGTCTCTCGTGAAG CGAAAATGnrGAGTGGCTCTCTGAGAAAnAAAGGTGCCTGAACTCATCATGAC17 T7CAGGATGAGCAGTIGAA1TI'ATGATCACTAAAGCGATCAATGCAAAACCAATT TCAGCGCTTI1AACAGACCAAGAATTGCTrGCTATCTATAAGGAGGCACTCAAT CTGT7AAATrCAATrGCTAUrATrGArGTCCA1TrCAAACATGATCATCGGT TAAAAGAGTCAAAATITIT1ATAACCAACTCCTTGACGATATAGATCAAGATG ATIGACACTGAAT'TATGGGGAGACCATAAAACTTACCTAAGTCTATGGAATGAG 1TAACCGAGACTCGTGnrGAAGAAAGATrGGT1TI1CTCATGGCGATATCACGGAT AGTAATATI IIIIATAGATAAAT1CAATGAAATTATTIAGACCflGGTCGTGCTG GGTTAGCAGATGAA1TGTAGATATATCCTrGAACGTTGCCTAAGAGAGGATG CATCGGAGGAAACTGCGAAAATATITAAAGCA1TTTAAAAAATGATAGACCTGAC ~AAAGAATATITrAAAACTAGATGAA~rGAUtccaagcattatctaaatactctgcagg cacgctagcttgtactcaagctcgtaacgaaggtcgigaccttgctcgigaaggiggcgacgtaatLcgttcagcttgtaaatggtctccaga acttgctgctgcatgtgaagtttggaaagaattaaattcgaattgatactattgacaaactttaattttatttttcatgatgtttatgtgatagca taaacatcgtttmatttttatggtgtttaggttaaatacctaaacatcattutacattwtnaaataagtctaaagttatctttgtttaaattgcctgt ctttataaattacgatgtgccagaaaaataa3Ztcttagctttttattatagaatttactttatgtattatatataagtatataaagaatagta acatactaaagcggatgtagcgcgtttatctaacggaaggaattcggcgcctacgtacccgggtcgcgaggaLccACGCGTAA TAGCTCAC1TTMCTTTAAA1TrAATITIAATIAAAGGTGTAAGCAAATTGCCTGAC GAGAGATCCACTTAAAGGATGACAGTGGCGGGCTACTGCCTACTTCCCTCCGGGAT AAAATTrAGAAAACGTAGTACTCCTAACGGAGCATrGACATCCCCATA1T TATATTAGGACGTCCCCTI'CGGGTAAATAAA1T1AGTGGACGTCCCC1TCGGGCAA ATAAA1TTAGTGGACAATAAATAAATIGTITGCCTGCCAACTGCCTAGGCAAGTA AACTTGGGAGTATAAAATAGGACGTCAGTGGCAGTlGCCTGCCAACTGCCTATAT TrATATACTGCGAAGCAGGCAGTGGCGGTACCACTGCCACTGGCGTCCTAATATAA ATATTGGGCAACTAAAG1ATAGCAGTATTAACATCCTATATTEATATACTCCGAA GGAACT-rGTrAGCCGATAGGCGAGGCAACAAAMArATGTCCCGTAAAAGGA TGCCTCCAGCATCGAAGGGGAAGGGGACGTCCTAGGCCATAAAACTAAAGGGAAA TCCATAGTAACTGATGTTATAAATTTATAGACTCCAAAAAACAGCTGCG'rATAAAT AACTrCTG17AAATATGGCCAAGGGGACAGGGGCACTrCAACTAAGTGTACATUA AAAATTGACAATCAATTrTAATTATAATATATA1TTrAGTAAAATATAACAAA AAGCCCCCATCGTCTAGgtagaattccagctggcggccgccctatg 29 GTGCACTCTCAGTACAATCTGCTCTGATGCCGCATAGTTAAGCCAGCCCCGACACCC Exo-p GCCAACACCCGCTGACGCGCCCTGACGGGC1TGTCTGCTCCCGGCATCCGC1TACA glucanase GACAAGCTGTGACCGTCTCCGGGAGCTGCATGTGTCAGAGGT1ICACCGTCATCAC insertion CGAAACGCGCGAGACGAAAGGGCCTCGTGATACGCCTAT1TYATAGG1TAATGTC cset ATGATAATAATGGTTCTIAGACGTCAGGTGGCACTTfCGGGGAAATGTGCGCGG AACCCCTAITT'GTr7A1T!CTAAATACATrCAAATATGTATCCGCTCATGAGACA (pSE ATAACCCTGATAAATGCTrCAATAATATTGAAAAAGGAAGAGTATGAGTATTCAAC 3~B-K ATTrCCGTGTCGCCCTrATrCCCFTTGCGGCATTTGCC'TCCTGT=rGCTCAC tD2: CCAGAAACGCTGGTGAAAGTAAAAGATGCTGAAGATCAGTTGGGTGCACGAGTGG BDO 1) G1TACATCGAACTGGATCTCAACAGCGGTAAGATCCTrGAGAG I I ICGCCCCGAA SEQ ID Sequence Use NO. GAACG I I I ICAATGATGAGCAC1TFI'AAAGTrCTGCTATGTGGCGCGGTATTATCC CGTAnGACGCCGGGCAAGAGCAACTCGGTCGCCGCATACACTA'ITCTCAGAATGA C'GGTGAGTACTCACCAGTCACAGAAAAGCATCTTACGGATGGCATGACAGTAA GAGAA11'ATGCAGTGCTGCCATAACCATGAGTGATAACACTGCGGCCAACTrAc1T CTGACAACGATCGGAGGACCGAAGGAGCTAACCGCTTI=GCACAACATGGGGGA TCATGTAACTCGCCTGATCGTTGGGAACCGGAGCTGAATGAAGCCATACCAAACG ACGAGCGTGACACCACGATGCCTGTAGCAATGGCAACAACGflGCGCAAACTA~rA ACTGGCGAACTAC11'ACTCTAGCTUCCCGGCAACAATIAATAGACTGGATGGAGGC GGATAAAGTrGCAGGACCACTTCTGCGCTCGGCCCTrCCGGCTGGCTGG1TTGC TGATAAATCTGGAGCCGGTGAGCGTGGGTCTCGCGGTATCATTGCAGCACTGGGGC CAGATGGTAAGCCCTCCCGTATCGTAGTTATCTACACGACGGGGAGTCAGGCAACT ATGGATGAACGAAATAGACAGATCGCTGAGATAGGTGCCTCACTGATTAAGCATlG GTAACTGTCAGACCAAGTTACTCATATATAC11AGATrGATI1'AAAACT-rCATIT TAATTTAAAAGGATCTAGGTGAAGATCCTTIGATAATCTCATGACCAAAATCCCT TAACGTGAGTT17CGTTCCACTGAGCGTCAGACCCCGTAGAAAAGATCAAAGGATC TTCTTGAGATCCTITr=CTGCGCGTAATCTGCTGCTrGCAAACAAAAAAACCACC GCTACCAGCGGTGGTTrG1TGCCGGATCAAGAGCTACCAACTCT1TCCGAAGGT AACTGGCTITCAGCAGAGCGCAGATACCAAATACTGTCTCTAGTGTAGCCGTAGTl AGGCCACCACTrCAAGAACTCTGTAGCACCGCCTACATACCTCGCTCTGCTAATCCT GTrACCAGTGGCTGCTGCCAGTGGCGATAAGTCGTGTCTrACCGGG17GGACTCAA GACGATAGTrACCGGATAAGGCGCAGCGGTCGGGCTGAACGGGGGGTUCGTGCAC ACAGCCCAGCTTGGAGCGAACGACCTACACCGAACTGAGATACCTACAGCGTGAGC TATGAGAAAGCGCCACGCTTCCCGAAGGGAGAAAGGCGGACAGGTATCCGGTAAG CGGCAGGGTCGGAACAGGAGAGCGCACGAGGGAGCTTCCAGGGGGAAACGCCTGG TATC1TATAGTCCTGTCGGGTITCGCCACCTCTGACTrGAGCGTCGATFI=GTGAT GCTCGTCAGGGGGGCGGAGCCTATGGAAAAACGCCAGCAACGCGGCCTr=ACGG 1-rCCTGGCCT'TGCTGGCC1rMGCTCACATGTTrCT1CCTGCGT-ATCCCCTGAT'C TGTGGATAACCGTATIACCGCCTTTGAGTGAGCTGATACCGCTCGCCGCAGCCGAA CGACCGAGCGCAGCGAGTCAGTGAGCGAGGAAGCGGAAGAGCGCCCAATACGCAA ACCGCCTCTCCCCGCGCGTGGCCGATrCATrAATGCAGCTGGCACGACAGG1CC CGACTGGAAAGCGGGCAGTGAGCGCAACGCAATTAATGTGAGTTAGCTCACTCATl AGGCACCCCAGGCTTACAC1TATGCTrCCGGCTCGTATGTrGTGTGGAATTGTGA GCGGATAACAATTrCACACAGGAAACAGCTATGACCATGATACGCCaagctcgcggccgc agtacLCTGCAGA'1TATGCAAAA'FIAAAGTCTTGTGACAACAGCmCTCCTTAAGTG CAAATATCGCCCATrCTTCCTCT1TCGTATATAAATGCTGTAATAGTAGGATGTC GTACCCGTAAAGGTACGACATrGAATATrAATATACTCCTAAGTACT11'CCCAAT A1TrATA1TAGGACGTCCCCTFCGGGTAAATAAA1T=AGTGGCAGTGGTACCGCCA CTCCCTA-rTrAATACTGCGAAGGAGGCAGTTGGCAGGCAACTCGTCGTTCGCAGTA TATAAATATCCACTAATATfATAT-rCCCGTAAGGGGACGTCCCGAAGGGGAAGGG GAAAGAAGCAGTCGCCTCCTITGCGAAAAGGTI'ACUrGCCCGACCAGTGAAAAGCA TGCTGTAAGATATAAATCTACCCTGAAAGGGATGCA M CACCATAATACTATACA AATGGTGTTACCC1TGAGGATCATAACGGTGCTACTGGAATATATGGTCTCTUCAT GGATAGACGATAGCCAT1AT1TACCCAT-TAAGGGGACATTAGTGGCCTGTCACTGC SEQ ID Sequence Use NO. TCCTrACGAGACGCCAGTGGACG7CGTCTAGAAAAflATGCGTGCCTAGAAG CCCCAAAAGGGAAGMACTGACTCGAGAGCGTGCCAACAGGm'AAATACT TCAATATGTATATnAGGACGCCGGTGGCAGTGGTACCGCCACGCCACCGTCGGAG GACGTCCCTTACGGTATATrATATACTAGGAMAATACCCGAAGGAGGCAGTGG CGGTACCACTGCCACTAATATATA77CCCGTAAGGGACGTCTCCTCGGAGTAT GTAAACATCTAAGTACTGCCCAATArATAnrAGGCAG7GGCAGGAACTG CTAGCTCTCCTCCflCGGAGTATGTAAACATCGCAGTATATAAATATCCACTAATAT T-rATA1TCCCGTAAGGGGACGTCCCGAAGGGGAAGGGGAAGGACGTCAGTGGCAG TTrGCCTGCCAACTGCCTAGGCAAGTAAACITAGGAGTATATAAATATAGGCAGTCG CGGTACCACTGCCACTGACGTCCTGCCAACTGCCTAGGCAAGTAAACTTAAGTGGC ACTAAAATGCATTGCCCGAAGGGGAAGGAGGACGCCAGTGGCAGTGGTACCGCC ACTGCCTCCflCGGAGTATAAAATCCTAGTATGTAAATCTGCTAGCGAGGAAATA AA1TIATrCTATIT7ATATACTCCG~rAGGAGGTAAGTAAACCCCTUCCCCTUCGGG ACGTCAGTGCAGTnGCCTGCCAACTGCCTAATATAAATAUrAGACCACTAAAG'IMTG GCAACTGCCAACTGn7GTCCT'CGGAGGAAAAAAAATGGTUAACTCGCAAGCAGfl AACATAACTAAAGMG1TAC1TACCGAAGACGMTACCCM1CTCGGUrAAGGAG ACGGAGACAGTTGCACTGTGACTGCCTAGTATAGCAATMGTTrG'FITATATGC TCGACAAAATGACT'CATAAAAATATAAAGTAGITAGCTAGFAITTATATCACT ATAACTAGGGTrCTCAGAGGCACCGAAGTCACTGTAAAAATAGTACm'AACIT GTrAATCTrCGTcYTrCTrCAAAAGGATCACGTAArrr111GAAGGTGGACCAAAA CTAACATAAACTGAATAGCCAGT1ACACTTAACAGAAGAAACCATAAAAAAAAGG TAAAGAA AAAAGCtGACrnCCATAGCTCAT17AATAATAAAATTA1TCTC'I1TrC AACATATCTCTAGATAGTCAAAAGACGACGACTGTGTCCCACA=AAACA AAA1rAATCTACTCAAAATTITGCCCTGAGAAAGAATAACTTACTTCG I I I IGCAG TAGCCA11'CATGTCACTTTGAAACTGTCCTACAAAG1AAACAfAAlAAAAATl A1AA1111ATATAACAAATATATATTAAATAAAAAATGAACAAAGAACTTCTA AGATCGTCTTAGTGAGTAATAAAGAG1=FACTrACCAGACAAGGCAG~m=C ATrC1TrT.AAAGCAGGCAGTTCTGAAGGGGAAAAGGGACTGCCTACTGCGGTCCTA GGTAAATACAT1TfATGCAATTCTGTGCTAGTAGGTTrCTATACTCACAAG AAGCAACCCCT-rGACGAGAGAACGTTATCCTCAGAGTATIATAATCCTGAGAGGG AATGCACTGAAGAATATI=CC'I1A iII IIACAGAAAGTAAATAAAATAGCGCTAA TAACGCT-rAATTCA1TIAATCAA17ATGGCAACAGGAAC1rCTAAAGCTAAACCATC AAAAGTAAAT1'CAGACTrCCAAGAACCTGGTIAGTIACACCAnAGGTAC1TT ACGTCCACTITAACTCAGAAGCAGGTAAAGTA11ACCAGGCTGGGGTACAACTG1M TAATGGCTGTATTATCCTMAT-rGCAGCA1rCTTATTAATCA=T'AGAAA1A CAACAGTTCTAATI=AGATGACGTrCTATGAGTTGGGAAACm7AGCTAAAGT TrC1TAATIn7ATrAACACAAACATAAAATATAAAACTG1TGTTAAGGCTAGCTG CTAAGTCflC1TICGCTAAGGTAAACTAAGCAACTCAACCATATTATAUTCGGCA GTGGCACCGCCAACTGCCACTGGCCrCCGrAAGATAAACGCGTggatctcacggACTA GTgtcgagtggtaccgccactgcctagtatataaatatcggcagttggcaggatatttatatactccgaaggaacttgttagccgataggcg aggcaactgccactaaatttatttgcctcctaacggagcataaaatccctaagtttacttgcccgtaaggggaaggggacgiccactaata tttatattaggcagutggcaggcaacaataaatacatttgtcccgtaaggggacgtcctgccaactgcctaggtagctattaagtatatatata rgaaaagtgtgtataaacaaactaaaataaaccaggtatggtaaccagatttattttagtttaaaaaaaaatagtgttgagctagagttagt SEQ ID Sequence Use NO. tgaagctaagtcagaTrAACCGG1rCCTfATCATCATCATCTTTGTAATCACT-rCCACCGCC ACCTGAGCCTTGAAAGTATAAGTITCACCGGTACCTAAACATTGGCTATAATATGG ATrAAAACTGACATGTAGTflCCTGATGCACACACAGTGGACCTGAATAACCAAT ACCACCACAITGACCGTAATGAGAUrGTGT'GGTCCAGGAGAAGAACCTGTGGTAG TAGCAGGACGACGTGTTGTAGTGGTGCCAGGTGGAYICCACCTGGTGGA1TACCA CCTGAAGGATCGCCTGTAGAGCCAATrGGACCAAA1TGATATTACTAAAAGTTAC *nTTGCA-fAGGACTT-GGCTrCAACrrGAGCAGGTACACCACTrrGAAG~rGAACA TGAACCACGAACAGCACCAGGAGTGCTrGAAGm1CGTTGTAGGATATGTACTAT CTAACCATAACATA1TAGCATAATAGTCATCCCATAATGACATAACTAAAACCATA CCACCTGATGTlGCTflCTlGAATGAGTAAACCACC1ATCTGAGAAGCTGCTA CCACCAAAT'CTGCUrCTfCTGCTGTACAATAATCGTCATfAAGGCCGT-rACCAGAA TAAGAACCTAA1TCTGCATITGG1rGTrGAAAAGTnACACCATITGCACGTAATAA CGArrAATAGCACCGCTAGTrCGAACTGTGTAACAACTG1rAACTI1AGTGTA TCTAATGTGAATGAACTCCTGGTCCATAAAAAGATGTATCCTAAACGATATGGG TCCCAATCGCAGCCATCAGGATCACATGTACCACCATAACGGTATCACTGTATGflr CCACCGCAACCGTCGCCITCACAAATC1TGGCCAACGGTAGTACAAGGATGTGG AG77AATGC1TCACTAA11'GAA17AGC1TCCCAAATATCCA1CAGAACAACAAGA TCCGTGACCACCAAT'CCAGTATfGCA11'ATTACTACTIGGTTCCCAACCTTCCACG TTAGCTTGACCGTrAATAAACTIAAATCACGAGGACACTGAGAATCACAATAGCC TGTTCCGTA111AGCACCTGCTGTATTAGTAGGATATrGCT7ACACCGCCATCAGC GTCCATTGAAACGAAATAAAGAGCACCATITAAACCACATGGTAATTGACTCACAT CTACGTCGAAACTGAACTCATI'ACCTAATAATGTAAATC11'GATAGGflGTGTCAC 1rGCCATrAAGTATAAACGTGCGCCTACA1TTTGTGCTGATrGAGTCACGAAAC CAATTGATAATGAGTTACCTGATGTAGTAACGCCGTAAG-GAAGCGTAAGCTGCA CCATCTAAACAACAATTIAGCACAAGTTTCG1T-ATCGGGACAAAGTGTTGATGAC CAAGTATrACCGTCATAACAATrAGTrGAACTATnAGTGGCATGTGTCCAACGCCAG TTAGCATCAATTACTACAGAGCCAG1TfGTGTACAAGTACCTCCTGAAGAACAT IrMGCCATG1TAATGGAGGATGAGTTCAGATTGTAAGGTACATGCTGACTGTGCA CGAGCAGTAGCTAAGAAAGCACTAATAACAGCAAG1TACGATATGGTACCATatgcg cgtatctccaaaataaaaaacaactcatcgttacgttaaatttattattatttaattttaatcattgtgtattaatatataactt~hataataatt aaaaataagcattttttacacacatattttuaaataaalcttaaacgggttatatatagttatatatatgggactagaactgcttgtgcatagtcat cacaattaitatattataaccatgataaaggtttatattatgatataaaaatgcataaaattttataaattttgcaagfaaaattattagg aaaaaatttannatttaaaatgttagtcaagtttacaactaatacttttaatttgtattttaagtattggacatttttgtggaattaaatgtaccaa tccattaattcatACTAGTgatatctacgtaatcgagaattcgatcccattttaaacggatcaaaatacctataaacccatgtCt gcaatcggcgtcataaacittagttgcttacgacgcctgtggacgtcccccccttccecCtacgggcaagtaaacttagggatttatgcaat aaataaatttgtcctcttcgggcaaatgaatttagtatttaaaatgacagggtgaaccattacttttgttaacaaggatctaCCaCtcactat utttgttgaattttaaacttatttaaaattctcgagaaagattttaaaaataaacttttttaactttuatttattttcttttttCGTATGGAAlT7 GCCCAATAT-rA1TCAACAAT1TATCGGAAACAGCG1T=AGAGCCAAATAAAAnTG GTCAGTCGCCATCGGATGTrATIC11TIAATCGAAATAATGAAACTTTrCAA GCGATCTAGCAC1ATATACAGAGACCACATACAGTGTCTCTCGTGAAGCGAAAA TGTGAGTGGCTCTCTGAGAAA1T-AAAGGTGCCTGAACTCATCATGAC1TMCAGG SEQ ID Sequence Use NO. ATGAGCAGTrrGAATrrATGATCACTAAAGCGATCAATGCAAAACCAATITCAGCG C-rTTFIAACAGACCAAGAAIrGCTGCTATCTATAAGGAGGCACTCAATCTGTTA AATrCAATTGCTATrATTGATGTCCATrATCAAACATTGATCATCGGTrAAAA GAGTCAAAA1TITITA1TGATAACCAACTCC1TGACGATATAGATCAAGATGA1TI GACACTGAATTATGGGGAGACCATAAAACTTACCTAAGTCTATGGAATGAGTTAAC CGAGACTCGTGTrGAAGAAAGA1TGG1ITrCTCATGGCGATATCACGGATAGTAA TAI I IATAGATAAATTCAATGAAA'TA TI ITTIIAGACC1GGTCGTGCTGGG'I1A GCAGATGAATIGTAGATATATCC1TGTTGAACGTTGCCTAAGAGAGGATGCATCG GAGGAAACTGCGAAAATATITAAAGCATIAAAAAATGATAGACCTGACAAAAG GAAfl'ATr=AAAACTGATGAATTGAAGAttccaagcattatctaaaatactctgcaggcacgctag cttgtactcaagctcgtaacgaaggtcgtgaccttgctcgtgaaggtggcgacgtattcgttcagcttgtaatggtctccagaactgcgc tgcatgtgaagtttggaaagaattaaattcgaatttgatactatgacaaactttaattttattttcatgatgtttatgtgaatagcatacatcg tttatttatggtgtttaggttaatacctaaacatcatttacattttaaattaagttctaaagttatctttgtttaaatttgcctgtctttataatt acgatgtgccagaaaataaaatcttagctitttattatagaatttatctttatgtattatatttatagttataataaaagaatagtaacatactaa agcggatgtagcgcgtttatcttuacggaaggaattcggcgcctacgtacccgggtcgcgaggatccACGCGITAATAGCT CAC=TT-rAAAMTAA1TI1AATrAAAGGTGTAAGCAAATTGCCTGACGAGA GATCCAC17AAAGGATGACAGTGGCGGGCTACTGCCTAC'rCCCTCCGGGATAAAA TATTGAAAAACG~rAGTACTrCCTAACGGAGCAT1GACATCCCCATAVIATA 1TAGGACGTCCCCTTCGGGTAAATAAA1TIAGTGGACGTCCCC1TCGGGCAAATAA ATTTTAGTGGACAATAAATAAA1T1GCCTGCCAACTGCCTAGGCAAGTAAACTT GGGAGTATrAAAATAGGACGTCAGTGGCAGTrGCCTGCCAACTGCCTATATrrATAT ACTGCGAAGCAGGCAGTGGCGGTACCACTGCCACTGGCGTCCTAATATAAATATIG GGCAACTAAAGmATAGCAGTATrTAACATCCTATA1TTATATACTCCGAAGGA ACT TGTTAGCCGATAGGCGAGGCAACAAATnrA'IIAT'GTCCCGTAAAAGGATGCCTCC AGCATCGAAGGGGAAGGGGACGTCCTAGGCCATAAAACTAAAGGGAAATCCATAG TAACTGATGUrATAAA1TfATAGACTCCAAAAAACAGCTGCG1TATAAATAACTI'CT G1-rAAATATGGCCAAGGGGACAGGGGCAC717CAACTAAGTGTACATrAAAAATTG ACAATrCAA111TF-rlAATrATAATATATATTrAGTAAAATATAACAAAAAGCCCC CATCGTCTAGgtagaatcccagctggcggccgccctatg 30 GTGCACTCTCAGTACAATCTGCTCTGATGCCGCATAGTTrAAGCCAGCCCCGACACCC Endo-p GCCAACACCCGCTGACGCGCCCTGACGGGCTTGTCTGCTCCCGGCATCCGCTTACA glucanase GACAAGCTGTGACCGTCTCCGGGAGCTGCATGTGTCAGAGG11TICACCGTCATCAC insertion CGAAACGCGCGAGACGAAAGGGCCTCGTGATACGCCTA1TTATAGG1TAATGTC cassette ATGATAATAATGGTICTTAGACGTCAGGTGGCAC1TTCGGGGAAATGTGCGCGG (p AACCCCTATTrGTT-rA1TICTAAATACATrCAAATATGTATCCGCTCATGAGACA pE ATAACCCTGATAAATGCTTCAATAATArGAAAAAGGAAGAGTATGAGTATTCAAC 3H-K A'f7rCCGTGTCGCCC1'TArCCCTFTI'GCGGCA1TIGCCTCCTGFITIGCTCAC tD2: CCAGAAACGCTGGTGAAAGTAAAAGATGCTGAAGATCAG1TGGGTGCACGAGTGG BD05) GT-rACATCGAACTGGATCTCAACAGCGGTAAGATCCTrGAGAGTICGCCCCGAA GAACG1TrCCAATGATGAGCACT71TAAAGTTCTGCTATGTGGCGCGGTA1TrATCC CGTATTGACGCCGGGCAAGAGCAACTCGGTCGCCGCATACACTATTCTCAGAATGA CTTGG1TGAGTACTCACCAGTCACAGAAAAGCATCT-rACGGATGGCATGACAGTAA GAGAATITATGCAGTGCTGCCATAACCATGAGTGATAACACTGCGGCCAACT-ACT-r '7 SEQ ID Sequence Use NO. CTGACAACGATCGGAGGACCGAAGGAGCTAACCGCTITTGCACAACATGGGGGA TCATGTAACTCGCCTUGATCGflGGGAACCGGAGCTGAATGAAGCCATACCAAACG ACGAGCGTGACACCACGATGCCTGTAGCAATGGCAACAACGTTGCGCAAACTAITA ACTGGCGAACTAC1TACTCTAGC11TCCCGGCAACAAflAATAGACTGGATGGAGGC GGATAAAG11'GCAGGACCACTrCTGCGCTCGGCCCTrCCGGCTGGCTGGC1TrATTGC TGATAAATCTGGAGCCGGTGAGCGTGGGTCTCGCGGTATCATTGCAGCACTGGGGC CAGATGGTAAGCCCTCCCGTATCGTAGTTATCTACACGACGGGGAGTCAGGCAACT ATGGATGAACGAAATAGACAGATCGCTGAGATAGGTGCCTCACTGATTAAGCA1TG GTAACTGTCAGACCAAGT1TACT'CATATATACT17IAGATGATTrAAAACT-TCATIT TAA1TAAAAGGATCTAGGTGAAGATCCT11TGATAATCTCATGACCAAAATCCCT TAACGTGAGTTICGTTCCACTGAGCGTCAGACCCCGTAGAAAAGATCAAAGGATC TTC'FrGAGATCCTITTFICTGCGCGTAATCTGCTGCTrGCAAACAAAAAAACCACC GCTACCAGCGGTGG1TGMrGCCGGATCAAGAGCTACCAACTCTITFCCGAAGGT AACTGGCTUCAGCAGAGCGCAGATACCAAATACTGTrCTI'CTAGTGTAGCCGTAG1T AGGCCACCACTTCAAGAACTCTGTAGCACCGCCTACATACCTCGCTCTGCTAATCCT GTITACCAGTGGCTGCTGCCAGTGGCGATAAGTCGTGTCTTACCGGG11'GGACTCAA GACGATAGT1'ACCGGATAAGGCGCAGCGGTCGGGCTGAACGGGGGG11'CGTGCAC ACAGCCCAGCT1GGAGCGAACGACCTACACCGAACTGAGATACCTACAGCGTGAGC TATGAGAAAGCGCCACGCTlCCCGAAGGGAGAAAGGCGGACAGGTATCCGGTAAG CGGCAGGGTCGGAACAGGAGAGCGCACGAGGGAGCTTCCAGGGGGAAACGCCTGG TATC1TATAGTCCTGTCGGG1TTCCJCCACCTCTGAC11'GAGCGTCGATT1TGTGAT GCTCGTCAGGGGGGCGGAGCCTATGGAAAAACGCCAGCAACGCGGCC1TTIACGG TrCCTGGCCTInfGCTGGCCTITTGCTCACATGTTC1TrCCTGCGTrATCCCCTGA17C TGTGGATAACCGTA'TrACCGCC1TTGAGTGAGCTGATACCGCTCGCCGCAGCCGAA CGACCGAGCGCAGCGAGTCAGTGAGCGAGGAAGCGGAAGAGCGCCCAATACGCAA ACCGCCTCTCCCCGCGCG1TGGCCGATTCATTAATGCAGCTGGCACGACAGG1TCC CGACTGGAAAGCGGGCAGTGAGCGCAACGCAATAATGTGAGUAGCTCACTCAT7 AGGCACCCCAGGC1TrACAC1TATGCTrCCGGCTCGTATG1TGTGTGGAATrGTGA GCGATAACAATTCACACAGGAAACAGCTATGACCATGATTACGCCagctcgcggccgc agtactCTGCAGAT1TATGCAAAA1TAAAGTC1TGTGACAACAGCTTICTCC1TAAGTG CAAATATCGCCCA'FICrC T TCGTATATAAATGCTGTAATAGTAGGATGTC GTACCCGTAAAGGTACGACATTGAATATrAATATACTCCTAAG1TACFITCCCAAT A1TI'ATAT1AGGACGTCCCCTTrCGGGTAAATAAA'I1TTAGTGGCAGTGGTACCGCCA CTCCCTA1I IIAATACTGCGAAGGAGGCAGTTGGCAGGCAACTCGTCGYI'CGCAGTA TATAAATATCCACTAATA11ATATTFCCCGTAAGGGGACGTCCCGAAGGGGAAGGG GAAAGAAGCAGTCGCCTCCTrGCGAAAAGGTTACTTGCCCGACCAGTGAAAAGCA TGCTGTAAGATATAAATCTACCCTGAAAGGGATGCA11CACCATAATACTATACA AATGGTGTIACCCTGAGGATCATAACGGTGCTACTGGAATATATGGTCTCTUCAT GGATAGACGATAGCCATATITACCCAT-AAGGGGACATTAGTGGCCTGTCACTGC TCCTTACGAGACGCCAGTGGACGTrCGTCCTAGAAAA1TATGCGCTGCCTAGAAG CCCCAAAAGGGAAGTTACTGACTCGTTAGAGCGTGCGCTAACAGGITTAAATACT TCAATATGTATA1TAGGACGCCGGTGGCAGTGGTACCGCCACTGCCACCGTCGGAG

GACGTCCCTTACGGTATATTATATACTAGGATITTAATACTCCGAAGGAGGCAGTGG

SEQ ID Sequence Use NO. CGGTACCACTGCCACTAATA1TTrATA1TCCCGTAAGGGACGTCCTCCT?CGGAGTAT GTAAACA1TCTAAGTTTACTrGCCCAATATTTATA1TAGGCAG1TGGCAGGCAACTG CTAGCTCTCCTCCTTCGGAGTATGTAAACATCGCAGTATATAAATATCCACTAATAT TTATATTCCCGTAAGGGGACGTCCCGAAGGGGAAGGGGAAGGACGTCAGTGGCAG TrGCCTGCCAACTGCCTAGGCAAGTAAACTrAGGAGTATATAAATATAGGCAGTCG CGGTACCACTGCCACTGACGTCCTGCCAACTrGCCTAGGCAAGTAAACTTAAGTGGC ACTAAAATGCA1TrrGCCCGAAGGGGAAGGAGGACGCCAGTGGCAGTGGTACCGCC ACTGCCTCCnrCGGAGTATAAAATCCTAGTATGTAAATCTGCTAGCGCAGGAAATA AATTTCTA1TIATATACTCCGTTAGGAGGTAAGTAAACCC11CCCCUTCGGG ACGTCAGTGCAG'I1GCCTGCCAACTGCCTAATATAAATATI'AGACCACTAAAG1TrG GCAACTGCCAACTGTGTCCITCGGAGGAAAAAAAATGGTTAACTCGCAAGCAGTr AACATAACTAAAGTrG1TAC'IMACCGAAGACG1TACCCTTCTCGG11'AAGGAG ACGGAGACAG'I1TGCACTGTGACTGCCTAGTATAGCAA=Tr1FGTFTATATGC TCGACAAAATGAC1TCATAAAAATATAAAGTAGTTAGCTAGTlA I II IATATCACT ATAACTAGGGTrCTCAGAGGCACCGAAGTCACTTGTAAAAATAGTACTT1AACTT GMrAATCTrCGTGTrCTCAAAAGGATCACGTAATTITrGAAGGTGGACCAAAA CTAACATAAACTGAATAGCCAGTTACACTrTAACAGAAGAAACCATAAAAAAAAGG TAAAGAAAAAAGCTGGACTITCCATAGCTCATMAATAATAAAATITATfCTC1TITC AACATATCTC1TAGATAGTTCAAAAGACTrGACGACTGTGTCCCACATITAAACA AAATTAATCTACTCAAAA I i IGCCCTGAGAAAGAATAAC'FFACTICG1T=rGCAG TAGCCATrCATGTCACT1TGAAACTGTCCTrACAAAGT-rAAACATTAATrAAAAATr A1TTAATITIMATATAACAAATATTATArrAAATAAAAAATGAACAAAGAACTTCTA AGATCGTCTTAGTGAGTAATrAAAGAGTI'1ACTTACCAGACAAGGCAGTT=C ATTC1rTAAAGCAGGCAGTTCTGAAGGGGAAAAGGGACTGCCTACTGCGGTCCTA GGTAAATACATIATGCAA1TAMTrGTGCTAGTAGG1TCTATACTCACAAG AAGCAACCCCTrGACGAGAGAACGTrATCCTCAGAGTA1TIATAATCCTGAGAGGG AATGCACTGAAGAATA1TTCCTITATITTIACAGAAAGTAAATAAAATAGCGCTAA TAACGCTTAATrCATTAATCAATTATGGCAACAGGAACT-rCTAAAGCTAAACCATC AAA AGTAAATrCAGACTCCAAGAACCTGGMIAGTFACACCAY[AGGTACTTTATI' ACGTCCACTrAACTCAGAAGCAGGTAAAGTATrACCAGGCTGGGGTACAACTG=1 TAATGGCTGTATATCCT-A1TGCAGCATTCTrATrAATCATTIAGAAATrrA CAACAG1TCTI1'AATr1AGATGACG1TrCTATGAG1TGGGAAACT=AGCTAAAGT TrCTTAA1TrATTrAACACAAACATAAAATATAAAACTG1TGTrAAGGCTAGCTG CTAAGTCTTC1TFCCTAAGGTAAACTAAGCAACTCAACCATA1TTATATI'CGGCA GTGGCACCGCCAACTGCCACTGGCCTTCCGT-rAAGATAAACGCGTggatctcacgtgACTA GTgtcgagtggtaccgccactgccagtatataaatatcggcagttggcaggatatatatactccgaaggaactgttagccgataggcg aggcaactgccactaaaatttatttgcctcctaacggagcataaaatccctaagttactgcccgtaaggggaaggggactccactaata tutatattaggcagttggcaggcaacaataaatacattgtcccgtaaggggacgcctgccaactgcctatggtagctattaagtatatatata tgaaaagtgtgtataaactaaactaaaataaaccaggtatggttaaccagatttatttagtttaaaaaaaattagttgtttgagctagagttagt tgaagctaagtctagaTAACCGG11TCCT1TIATCATCATCATCT1TfGTAATCAC1TCCACCGCC ACCTGAGCCTTGAAAGTATAAG1T=CACCGGTACCCTrGCGAGCTAAACAACTACT TACTAATGAAGTGTCTGTCCATGAG111'CCAGAAGAAGTAGGGGTrrCGGT-rAATAC ATAAGTlGAATCAAAAGAACCAGCACCCCAACCTACATAACCTAAGTACACGTCAG SEQ ID Sequence Use NO. AGTGATrAAGTACTGAA1GTGACACATGTCn"GGATACAACCTGCACGT TTCCACCACCTG1TCAGTTAAAATGGCTTGGCGATUATTIGACGTAACCAAGT1TG CTAAAGGACTAAAAGCACCATCAATATrATIT7GTGGTACATrCGGCGTGTGTTCCGC TAT-rATCAGAATCAAGATATIATGTACATCGAATA1TAAGTAGTGGTACTACCGT CTGGGrrAGTCACTUGACTAAGAGCAGCTGCGCTACCGTCAGAAATAAAAGCGCCG GCAGATTGCCAATCGTnGCCTGGTAAACTAATGAAnTGTGATGTTGCACCAGCATTA CGAATAGCAGTrACTACTFCrGCACAG11rGCAGCCCAAGTA1IATG1TCACATCG TGAGGTTCATI'CATAATACCGAACCAAACACGTGA1TGACTAGCATA1TGAAGCT AA~rGGCTCCATAATGATGTAAA17GAGCA11AG~GGACCACCTGACCAATAATA CCACCGTTCCAACGGGCATAATTATGAATATCAACAATACAATAGGCACCTAAAGA TAAGCAACCTTGTACTAATGATCATAITACTAATGATGTACTATCTAAGT'ACC ACCTAAATTIGTfG1TAACTAAGTA1TGCCAGCCCACTGGTAAACGGAAAATAGTCA TACCATCTTCA1TACAAAGTGTGCA'IrrGACCAATGCCATCTGGATAATTGTI1G AGCCAGTAAAATFITAAAGGGGGATAAAC1TrACTGGTAACACATGTACCATCG GTAGTACAACCAAAATCGAAACCTGCAATATTAACACCAGCGAAACGTACTCCAGA AGATGTAGGAGGTGTGCTGCTAGAAGTGCTAGTAGCACGAGlGT7GTAG1TGGAC CTGAAGGAGGGCGAG11TGATGUrG1TATAG'ITGTITGCACCTGGAATACArrGAGCA TAGTAAGGATI'AAGGTACTACATGCTGAGCCAGGAGCACAAYI'GGTAGGACCAGA CCAACCAATACCACCACACTGACCCCAAACAGTCTGTTGAGCAACAGCACCACCAT ATAAGATAGATGCAGCAAGTAATAATGGTGCTACGC I I IG1TrGGTACCATatgcgtgt atctccaaaataaaaaaacaactcatcgttacgttaaatttattattatttaattutaatcattgtgtatttaatattataacttatataaaataaaallaa aaataagcattttttacacacatatttttaaLtaatctttaaacgggttatatatagttatatatatgggactagaactgctttgtgcatagtcatca caattattatattataaaccatgaataaaggttttattattatgatataaaaatgcataaaatttttataaattttgcaagtaaaatatataattaggaa catttaattcatACTATgaatctacgtaatcgatgattcgatcccatttttataactggatctaaaatacctataaacccatgtcttct aatcggcgtcataaacttagttgcttacgacgccgtggacgtcccccccttcttacgggcaagtaaacttagggattttaatgcaataa ataaatttgtcctcttcgggcaaatgaattttagtattaaatagacaagggtgaaccalacttttgttaacaagtgatcttaccactcactattttt gttgaattttaaacttatttaaaattctcgagaaagattttaaaataaacttttttaatcttmattatttcttllCGTATGGAAT1'GC CCAATAT-rATTrCAACAA1TTrATCGGAAACAGCG1TrAGAGCCAAATAAAATTGGTC AGTCGCCATCGGATGTTATCTrAATCGAAATAATGAAACTTIfCrAAGCG ATCTAGCACTTATATACAGAGACCACATACAGTGTCTCTCGTGAAGCGAAAATG1T GAGTTGGCTCTCTGAGAAA1TAAAGGTGCCTGAACTCATCATGAC1TrCAGGATGA GCAGT1TGAAMTATGATCACTAAAGCGATCAATGCAAAACCAATrCAGCGC'T= 1TrAACAGACCAAGAATTGCTnGCTATCTATAAGGAGGCACTCAATCTGTrAAATrC AATGCTATATTGA~GTCCATA1TCAAACAITGATCATCGG1TAAAAGAGTC AAAA1Tr=ATrGATAACCAACTCCTrGACGATATAGATCAAGATGA1TrGACAC TGAA-IrATGGGGAGACCATAAAACTrACCTAAGTCTATGGAATGAGTrrAACCGAGA CTCGTGTrGAAGAAAGA'FrGGTTrCTCATGGCGATATCACGGATAGTAATAT17 TrATAGATAAATTCAATGAAATrATT=AGACCT-rGGTCGTGCTGGGTrAGCAG ATGAA17IGTAGATATATCC1TGTTGAACGTFGCC-rAAGAGAGGATGCATCGGAG

GAAACTGCGAAAATAT-ITAAAGCATTTAAAAAATGATAGACCTGACAAAAGGAA

SEQ ID Sequence Use NO. ctcaagctcgtaacgaaggtcgtgaccttgctcgtgaggtggcgacgttcgttcagcttgtaaggtctccagactgctgctgcat gtgaagtggaaagaaattaaattegaatttgatactattgacaacttt3ttttatttttcatgatgtttatgtgaatagcataacatcgttttta gatgcgcgcgtttatcttaacggalggaattcggcgcctacgtacccgggtcgcgaggatccACGCGTlAATAGCTCAC TTrCTTTAAA1TrAATTrAAITAAAGTGTAAGCAAAI'GCCTGACGAGAGAT CCACTrAAAGGATGACAGTGGCGGGCTACTGCCTACnrCCCTCCGGGATAAAA'lff ArT-rGAAAAACGrAGT-ACTCCTAACGGAGCATrGACATCCCCATATTrATA1TA GGACGTCCCC'I1CGGGTAAATAAATFIAGTGGACGTCCCCTTCGGGCAAATAAA1T TrAGTGGACAATAAATAAATTTr~GCCTGCCAACTGCCTAGGCAAGTAAACI1GG GAGTATrAAAATAGGACGTCAGTGGCAGTTGCCTGCCAACTGCCTATATIATATAC TGCGAAGCAGGCAGTGGCGGTACCACTGCCACTGGCGTCCTAATATAAATATIGGG CAACTAAAG1TTTATAGCAGTATrAACATCCTATATTrATATACTCCGAAGGAACTG TrAGCCGATAGGCGAGGCAACAAA'IMAMTATGTCCCGTAAAAGGATGCCTCCA GCATCGAAGGGGAAGGGGACGTCCTAGGCCATAAAAC'rAAAGGGAAATCCATAGT AACTGATGTTATAAA11TATAGACTCCAAAAAACAGCTGCQTfATAAATAACflCTG TAAATATGGCCAAGGGGACAGGGGCAC1TCAACTAAGTGTACATI'AAAAA1TrGA CAATrCAATI1TFITAA1ATAATATATAMTAGTAAAATATAACAAAAAGCCCCC ATCGTCTAgtagaattccagctggcggccgCCCtatg 31 GTGCACTCTCAGTACAATCTGCTCTGATGCCGCATAG1TAAGCCAGCCCCGACACCC Endo GCCAACACCCGCTGACGCGCCCTGACGGGCTTGTCTGCTCCCGGCATCCGCTTACA xylanase GACAAGCTGTGACCGTCTCCGGGAGCTGCATGTGTCAGAGG1TTCACCGTCATCAC insertion CGAAACGCGCGAGACGAAAGGGCCTCGTGATACGCCTA1TPTATAGG1TAATGTC cassette ATGATAATAATGG111CTTAGACGTCAGGTGGCACTITCGGGGAAATGTGCGCGG

(S

AACCCCTATVIGMTATITCTAAATACATTCAAATATGTATCCGCTCATGAGACA pE ATAACCCTGATAAATGClCAATAATAflGAAAAAGGAAGAGTATGAGTAITCAAC 3BK ATMCCGTGTCGCCCTTA1TCCC1Tr=GCGGCATTrGCCITCCTG1TFTGCTCAC t2 CCAGAAACGCTGGTGAAAGTAAAAGATGCTGAAGATCAGTI'GGGTGCACGAGTGG BD1 1) GTTACATCGAACTGGATCTCAACAGCGGTAAGATCCTrGAGAGTI=CGCCCCGAA GAACG11TCCAATGATGAGCAC1T=AAAGTTCTGCTATGTGGCGCGGTATrATCC CGTATTGACGCCGGGCAAGAGCAACTCGGTCGCCGCATACACTATrCTCAGAATGA C-rrGGTrGAGTACTCACCAGTCACAGAAAAGCATCTTACGGATGGCATGACAGTAA GAGAA17ATGCAGTGCTGCCATAACCATGAGTGATAACACTGCGGCCAACTTACTT CTGACAACGATCGGAGGACCGAAGGAGCTAACCGCTTTTTTGCACAACATGGGGGA TCATGTAACTCGCCTnGATCGTTGGGAACCGGAGCTGAATGAAGCCATACCAAACG ACGAGCGTGACACCACGATGCCTGTAGCAATGGCAACAACG1fGCGCAAACTATTA ACTGGCGAACTAC'ITACTCTAGCUTCCCGGCAACAATTAATAGACTGGATGGAGGC GGATAAAGTTGCAGGACCACTFCTGCGCTCGGCCC'FrCCGGCTGGCTGGTIAT7GC TGATAAATCTGGAGCCGGTGAGCGTGGGTCTCGCGGTATCATTGCAGCACTGGGGC CAGATGGTAAGCCCTCCCGTATCGTAG1TATCTACACGACGGGGAGTCAGGCAACT ATGGATGAACGAAATAGACAGATCGCTGAGATAGGTGCCTCACTGATTAAGCATI'G GTAACTGTCAGACCAAG1TACTCATATATACTIAGATTGATTTAAAACTCA1TI SEQ ID Sequence Use NO. TAATTTAAAAGGATCTAGGTGAAGATCCTTGATAATCTCATGACCAAAATCCCT TAACGTGAG1TfCGTCCACTGAGCGTCAGACCCCGTAGAAAAGATCAAAGGATC T7CT'rGAGATCC1I I I ITGICGCGTAATCTGCTGCTrGCAAACAAAAAAACCACC GCTACCAGCGGTGGT'GMGCCGGATCAAGAGCTACCAACTC1TTTTCCGAAGGT AACTGGC11CAGCAGAGCGCAGATACCAAATACTGUCTI'CTAGTGTAGCCGTAGT7 AGGCCACCACTlCAAGAACTCTGTAGCACCGCCTACATACCTCGCTCTGCTAATCCT GT-rACCAGTGGCTGCTGCCAGTGGCGATAAGTCGTGCrrIACCGGGTfGGACTCAA GACGATAGnrACCGGATAAGGCGCAGCGGTCGGGCTGAACGGGGGGTnCGTGCAC ACAGCCCAGCnGGAGCGAACGACCTACACCGAACTGAGATACCTACAGCGTGAGC TATGAGAAAGCGCCACGCTITCCCGAAGGGAGAAAGGCGGACAGGTATCCGGTAAG CGGCAGGGTCGGAACAGGAGAGCGCACGAGGGAGCTUCCAGGGGGAAACGCCTGG TATC1TrATAcJTCCTGTCGGG1TCGCCACCTCTGACT-rGAGCGTCGATTGTGAT GCTCGTCAGGGGGGCGGAGCCTATGGAAAAACGCCAGCAACGCGGCC11TTACGG TTCCTGGCC1FrGCTGGCC=GCTCACATGTCFCCTGCG1'ATCCCCTGAITC TGTGGATAACCGTAT-rACCGCC1TIGAGTGAGCTGATACCGCTCGCCGCAGCCGAA CGACCGAGCGCAGCGAGTCAGTGAGCGAGGAAGCGGAAGAGCGCCCAATACGCAA ACCGCCTCTCCCCGCGCGTTGGCCGA1TCATrAATGCAGCTGGCACGACAGGTT1TCC CGACTGGAAAGCGGGCAGTGAGCGCAACGCAAflAATGTGAGTrAGCTCACTCAT7 AGGCACCCCAGGCTrACACTrATGCTrCCGGCTCGTATGTrGTGTGGAATrGTGA cJCGGATAACAA1TrCACACAGGAAACAGCTATGACCATGATACGCCaagctcgcggccgc agtactCTGCAGATTITATGCAAAATTAAAGTC17GTGACAACAGC'flTCTCCflAAGTG CAAATATCGCCCATctfICCTCTICGTATATAAATGCTGTAATAGTAGGATGTC GTACCCGTAAAGGTACGACATTGAATATTAATATACTCCTAAGTTTACTrCCCAAT AFFIATATTAGGACGTCCCC'ITCGGGTAAATAAATITAGTGGCAGTGGTACCGCCA CTCCCTATTIAATACTGCGAAGGAGGCAGT1GGCAGGCAACTCGTCG1TCGCAGTA TATAAATATCCACTAATATrATATTCCCGTAAGGGGACGTCCCGAAGGGGAAGGG GAAAGAAGCAGTCGCCTCCTTGCGAAAAGGI-rACTTfGCCCGACCAGTGAAAAGCA TGCTGTAAGATATAAATCTACCCTGAAAGGGATGCATfCACCATAATACTATACA AATGGTGTTACCC1GAGGATCATAACGGTGCTACTGGAATATATGGTCTCT7CAT GGATAGACGATAGCCATTATITACCCATTAAGGGGACATTAGTGGCCTGTCACTGC TCCTTACGAGACGCCAGTGGACGTrCGTCCTAGAAAATrrATGCGCTGCCTAGAAG CCCCAAAAGGGAAGT1TACTGACTCG1TAGAGCGTGCGCTAACAGG1TIAAATACT TCAATATGTATATTAGGACGCCGGTGGCAGTGGTACCGCCACTGCCACCGTCGGAG GACGTCCCTTACGGTATAT-rATATACTAGGA'FTAATACTCCGAAGGAGGCAGTGG CGGTACCACTGCCACTAATATIATAT-rCCCGTAAGGGACGTCCTCCTTCGGAGTAT GTAAACATCTAAGTrACTrGCCCAATATrrATATIAGGCAGTnGGCAGGCAACTG CTAGCTCTCCTCCTUCGGAGTATGTAAACATCGCAGTATATAAATATCCACTAATAT 1TATATTCCCGTAAGGGGACGTCCCGAAGGGGAAGGGGAAGGACGTCAGTGGCAG UrGCCTGCCAACTGCCTAGGCAAGTAAACTAGGAGTATATAAATATAGGCAGTCG CGGTACCACTGCCACTGACGTCCTGCCAACTGCCTAGGCAAGTAAACTTAAGTGGC ACTAAAATGCAKFGCCCGAAGGGGAAGGAGGACGCCAGTGGCAGTGGTACCCC ACTGCCTCCflCGGAGTA1TAAAATCCTAGTATGTAAATCTGCTAGCGCAGGAAATA AATTTCTAT'ATATACTCCGTTAGGAGGTAAGTAAACCCCI1CCCCT-rCGGG SEQ ID Sequence Use NO.I ACGTCAGTGCAGTITGCCTGCCAACTGCCTAATATAAATATITAGACCACTAAAG1T-G GCAACTGCCAACTGTrGTCCTrCGGAGGAAAAAAAATGG1TAACTCGCAAGCAGTr AACATAACTAAAG1TrrAC1ACCGAAGACG1TTACCC1TCTCGGTrAAGGAG ACGGAGACAGWrGCACTGTGACTGCCTAGTATAGCAA1TIG1TITGTATATGC TCGACAAAATGAC1TICATAAAAATATAAAGTAGTAGCTAGTTA I II IATATCACT ATAACTAGGGTTCTCAGAGGCACCGAAGTCACTGTAAAAATAGTACTITAACTIT GTTAATCT1'CGTGTTCITCAAAAGGATCACGTAAI I I IIIGAAGGTGGACCAAAA CTAACATAAACTGAATAGCCAG77ACACrTAACAGAAGAAACCATAAAAAAAAGG TAAAGAAAAAAGCTGGACTCCATAGCTCAT17IAATAATAAAArrATCTCPIC AACATATCTCTI'AGATAGTTCAAAAGACT-rGACGACTGTGTCCCACATITIAAACA AAATI'AATCTACTCAAAA I IGCCCTGAGAAAGAATAAC1TACTrCGFTrGCAG TAGCCATTCATGTCAC1TGAAACTGTCC1TACAAAGTTAAACATTAATrAAAAA1T AT1h7AATITTATATAACAAATATrATA11AAATAAAAAATGAACAAAGAAC1TCTA AGATCGTCTITAGTGAGTAATTAAAGAG1TIACTACCAGACAAGGCAGTITFIC ATTC1TMAAAGCAGGCAGTrCTGAAGGGGAAAAGGGACTGCCTACTGCGGTCCTA GGTAAATACA1TFTATGCAATATTrCTI'GTGCTAGTAGG1rCTATACTCACAAG AAGCAACCCCT-rGACGAGAGAACGTrrATCCTCAGAGTA1TATAATCCTGAGAGGG AATGCACTGAAGAATA1111CCTTATT=ACAGAAAGTAAATAAAATAGCGCTAA TAACGC1TAATTCAT1TAATCAA1rATGGCAACAGGAACTTCTAAAGCTAAACCATC AAAAGTAAATTCAGAC77CCAAGAACCTGGTIAGrrACACCATTAGGTAC1TIAIT ACGTCCAC1TAACTCAGAAGCAGGTAAAGTA1TACCAGGCTGGGGTACAACTGTT TAATGGCTGTATTTATCCT1TATrGCAGCATCTATTAATCA1TrrAGAAATT'A CAACAGTrCTT'AA'AGATGACGTIT7CTATGAGTTGGGAAAC1TAGCTAAAGT TTCTAAnATTAACACAAACATAAAATATAAAACTG=GTAAGGCTAGCTG CTAAGTC11C1TFCGCTAAGGTAAACTAAGCAACTCAACCATATIATA1TCGGCA GTGGCACCGCCAACTGCCACTGGCCTrCCG'FrAAGATAAACGCGTggatctcacgtgACTA GTgtcgagtggtaccgccactgccdagtalataaatatcggcagttggcaggatatttatatactccgaaggaacttgttagccgataggcg aggcaactgccactaaaattattgcctcctaacggagcattaaaatccctaagtttacttgcccgtaaggggaaggggacgtccactaata tttatattaggcagttggcaggcaacaataaatacatttgtcccgtaaggggacgtcctgccaactgcctatggtagctattaagtatatatata tgaaaagtgtgtataaactaaactaaaataaaccaggtatggttaaccagattattttagtttaaaaaainttagtgLttgagctagagtagt tgaagctaagtctagaUTAACCGGU7CC1TATCATCATCATCm~GTAATCACTrCCACCGCC ACCTGAGCCtTGAAAGTATAAG11TCACCGGTACCGCTAACAGTGATAGAAGCAC TACCTGATGAAAAATAACCTTCAACAGCTACAAT1TGATAGTCCATrGTACCTAATG 1TAAACCTTGTTGAGCCCATGCAT1TAAAGTGGTGCTGTATTAACACTACCACTrG AACGATGArrACGTCTACACTCCAGTAT'GGTAGAAAGTGGCAGT-rCCAATrATAG ATGGTITGATTACGCGTFIGAGTACGATAAATATCATAAACTGATCCATCTGAAGTAA CT-rCACCTAA1TIAGTAGCACCTGTTGAAGGG17GTATGTACCAAAGTTCTCTACAA TATAATATrCAATFTAATGGGUTACGGCTCCAACCGTATACACnTAAATAAGAATTAC CATTAGGGnTGTAACTACCAGAGAAATTGATTACCTrA~rTITGTACCAGG1TGCC AACCYI=CCTCCAACAAAATTGCCTGAGTrACTCCAAT=ACACTAAA1TGACCAC CAGGTCCArrAGTATATGTAACACCACCGTGTCCATCA'FrCCAGTAAGAA TA AAA G TAACCGTTArrGTAACCTGTACCTGGT-rGAAITGTTGACG1T=CTACTGCAACTG

ATTCCACTI'CAGCAGCTGGACGGCAACTGCACGTGAAGGTGGAGATGCTGCTAAA

SEQ ID Sequence Use NO. AGAClTcTGAAAGATACTGGTACCATatgcgtgtatctccaaaataanaaaactcatcgttacgttaaatttatt aflatttaattttaatcattgtgtattaatattataactatat~aanattaaattaanaataagcatmtttacacacatatttttaataaatctttaaac gggttatatatagttatatatatgggactagaactgctttgcatagcatcacaattattatattatafaaccatgaataaaggttttattattatgat ataaaaatgcataaaatttttataaattttgcaagtaaata~ataataggaaaaattaZatttaaatgtagtcaagttacaactaatactt taattttgtattttaagtattggacattttgtggaattaaatgtaccaaacatccatttaatttcatACl'AGTgatatctacgtaatcgatgaatt cgatcccattttataacggatctcaaantacctataaacccattgttcttctcttagcctaagaacaatcaflttataaatatatttattattatg ctataatataaatactatataat acatttacc t t tataat acau tttaC ttt~ttatttgc atgatttaatgcttat gctatc t tattagtcc ataacctttaaaggaccltttctuatgggatattatat~ttccaacaaagcaatcggcgcataaacttagtgctacgacgccgtggac gicccccccttccccttacgggcaagtaaacttagggatttaatgcaataaataaatttgtcctcttcgggcaaatgaattttagtatttaaatat gacaagggtgaaccflttacttucgttaacaagtgatcttaccactcactattttrgttgaattttaaacttatttaaaattctcgagaaagattttaaa aataaactwtaatcttttatttatitttttcttttttCGTATGGAAlTGCCCAATAlAtTCAACAATfrATCGG AAACAGCG I ITTIAGAGCCAAATAAAA-rGGTCAGTCGCCATCGGATG1TrC1TI TAATCGAAATAATGAAACTITITCTTAAGCGATCTAGCACTIATATACAGAGAC CACATACAGTGTCTCTCGTGAAGCGAAAATG11'GAGflGGCTCTCTGAGAAAT7AA AGGTGCCTGAACTCATCATGACTI1CAGGATGAGCAGTTrGAATTTATGATCACTA AAGCGATCAATGCAAAACCAA1TI'CAGCGCTI1TIAACAGACCAAGAATrGC1TG CTATCTATAAGGAGGCACTCAATCTGTAAAnCAATrGCTA1A-GAU7GTCCAT TrA1TTCAAACATTGATCATCGGTrAAAAGAGTCAAAATTI1TITTGATAACCAAC TCCYITGACGATATAGATCAAGATGAYI1GACACTGAATTATGGGGAGACCATAAA ACTFACCTAAGTCTATGGAATGAGflAACCGAGACTCGTGUFGAAGAAAGAflGGT 1TI=CTCATGGCGATATCACGGATAGTAATAT11TATAGATAAATTCAATGAAAT 1TA1TTTIAGACCT1TGGTCGTGCTGGGTTAGCAGATGAAT'GTAGATATATCC1TI' GTTGAACGT1GCCTAAGAGAGGATGCATCGGAGGAAACTGCGAAAATATTAAA GCATTrAAAAAATGATAGACCTGACAAAAGGAATrATI11AAAAC1TGATGAAT TGAATGAtccaagcattatctaaaatactcgcaggcacgCtagcttgtactcaagctcgaacgaaggtcgtgaccttgctcgtga aggtggcgacgtattcgttcagcttgtaaatggtctccagaacttgctgctgcatgtgaagtttggaaagaaata.attcgaatttgatacta tttttaaaat taagttctaaagt tatc ttttgtttaaatttgcc tgtctttataaattacgat gt gccag aalaat a n tctt agc tt tattatag aat t tatctttatgtattatatttataagttataataaaagaaatagtaacatactaaagcggagtagcgcgtttacttaacggaaggaattcggcgc ctacgtacccgggtcgcgaggatccACGCGTAATAGCTCAC'flTT1AAATTTAATr11AA1T TAAAGGTGTAAGCAAATI'GCCTGACGAGAGATCCACTTAAAGGATGACAGTGGCGG GCTACTGCCTACTTCCCTCCGGGATAAAATrATFGAAAAACG1'TAGTrACTrCCT AACGGAGCATTGACATCCCCATATITATATTAGGACGTCCCCTlCGGGTAAATAAAT 1'AGTGGACGTCCCCTCGGGCAAATAAATIMAGTGGACAATAAATAAATrGTr GCCTGCCAACTGCCTAGGCAAGTAAACTI'GGGAGTAU7AAAATAGGACGTCAGTGG CAGTITGCCTGCCAACTGCCTATA M ATATACTGCGAAGCAGGCAGTGGCGGTACC ACTGCCACTGGCGTCCTAATATAAATAflGGGCAACTAAAGITTrATAGCAGTA11AA CATCCTATATTTATATACTCCGAAGGAACTGTAGCCGATAGGCGAGGCAACAAA TTTATfAIGTCCCGTAAAAGGATGCCTCCAGCATCGAAGGGGAAGGGGACGTCC TAGGCCATAAAACTAAAGGGAAATCCATAGTAACTGATGnrATAAATATAGACT CCAAAAAACAGCTGCGT-lATAAATAACT-rCTGY[rAAATATGGCCAAGGGGACAGGG GCAC1-TCAACTAAGTGTACATrAAAAATGACAATTCAA1TTIAA1TATAAT ATT M GAATTAAAACCCTGCAgaatcacgcgcc SEQ ID Sequence Use NO. ctatg Examrnle 8. Construction of a C. reinhardifi strain transformed with a construct that does not disrupt photosynthetic capability [001601 In this example a nucleic acid encoding endo-p-glucanase from T. reesei was introduced into C. reinhardii. Transforming DNA (SEQ ID NO. 28, Table 4) is shown graphically in FIG. 2B. In this instance the segment labeled "Transgene" is the endo-$-glucanase encoding gene (SEQ ID NO. 16, Table 3), the segment which drives expression of the transgene (labeled 5' UTR) is the 5' UTR and promoter sequence for the psbC gene from C. reinhardtii,, the segment labeled 3' UTR contains the 3' UTR for the psbA gene from C. reinhardtii, and the segment labeled "Selection Marker" is the kanamycin resistance encoding gene from bacteria, which is regulated by the 5' UTR and promoter sequence for the arpA gene from C. reinhardtii and the 3' UTR sequence for the rbcL gene from from C. reinhardrii. The transgene cassette is targeted to the 3HB locus of C. reinhardiii via the segments labeled "5' Homology" and "3' Homology," which are identical to sequences of DNA flanking the 3HB locus on the 5' and 3' sides, respectively. All DNA manipulations carried out in the construction of this transforming DNA were essentially as described by Sambrook et al., Molecular Cloning: A Laboratory Manual (Cold Spring Harbor Laboratory Press 1989) and Cohen et al., Meth. Enzymol. 297, 192-208, 1998. [00161] For these experiments, all transformations were carried out on C. reinhardii strain 137c (mt+). Cells were grown to late log phase (approximately 7 days) in the presence of 0.5 mM 5-fluorodeoxyuridine in TAP medium (Gorman and Levine, Proc. Natl. Acad. Sci., USA 54:1665-1669, 1965, which is incorporated herein by reference) at 23*C under constant illumination of 450 Lux on a rotary shaker set at 100 rpm. Fifty ml of cells were harvested by centrifugation at 4,000xg at 23*C for 5 min. The supernatant was decanted and cells resuspended in 4 ml TAP medium for subsequent chloroplast transformation by particle bombardment (Cohen et al., supra, 1998). All transformations were carried out under kanamycin selection (100 pg/ml), in which resistance was conferred by the gene encoded by the segment in Figure 2B labeled "Selection Marker." (Chlamydomonas Stock Center, Duke University). [00162] PCR was used to identify transformed strains. For PCR analysis, 106 algae cells (from agar plate or liquid culture) were suspended in 10 mM EDTA and heated to 95'C for 10 minutes, then cooled to near 23'C. A PCR cocktail consisting of reaction buffer, MgCl2, dNTPs, PCR primer pair(s) (Table 2 and shown graphically in FIG. 3B), DNA polymerase, and water was prepared. Algae lysate in EDTA was added to provide template for reaction. Magnesium concentration is varied to compensate for amount and concentration of algae lysate in EDTA added. Annealing temperature gradients were employed to determine optimal annealing temperature for specific primer pairs. [00163] To identify strains that contain the endo-s-glucanase gene, a primer pair was used in which one primer anneals to a site within the psbC 5'UTR (SEQ ID NO. 10) and the other primer anneals within the endo-o-glucanase coding segment (SEQ ID NO. 3). Desired clones are those that yield a PCR product of expected size. To determine the degree to which the endogenous gene locus is displaced (heteroplasmic vs. homoplasmic), a PCR reaction consisting of two sets of primer pairs were employed (in the same reaction). The first pair of primers amplifies the endogenous locus targeted by the expression vector (SEQ ID NOs. 13 and 14). The second pair of primers (SEQ ID NOs. 6 and 7) amplifies a constant, or control region that is not targeted by the expression vector, so should produce a product of expected size in all cases. This reaction confirms that the absence of a PCR product from the endogenous locus did not result from cellular and/or other contaminants that inhibited the PCR reaction. Concentrations of the primer pairs are varied so that both reactions work in the same tube; however, the pair for the endogenous locus is 5X the concentration of the constant pair. The number of cycles used was >30 to increase sensitivity. The most desired clones are those that yield a product for the constant region but not for the endogenous gene locus. Desired clones are also those that give weak-intensity endogenous locus products relative to the control reaction. [00164] Results from this PCR on 96 clones were determined and the results are shown in FIG. 10. Figure 10A shows PCR results using the transgene-specific primer pair. As can be seen, multiple transformed clones are positive for insertion of the endo-p-glucanase gene. Figure 10B shows the PCR results using the primer pairs to differentiate homoplasmic from heteroplasmic clones. As can be seen, multiple transformed clones are either homoplasmic or heteroplasmic to a degree in favor of incorporation of the transgene (e.g. numbers 67, 92). Unnumbered clones demonstrate the presence of wild-type psbA and, thus, were not selected for further analysis. [00165] To ensure that the presence of the endo-p-glucanase-encoding gene led to expression of the endo-p glucanase protein, a Western blot was performed. Approximately 1x.108 algae cells were collected from TAP agar medium and suspended in 0.5 ml of lysis buffer (750 mM Tris, pH=8.0, 15% sucrose, 100 mM beta mercaptoethanol). Cells were lysed by sonication (5x30sec at 15% power). Lysate was mixed 1:1 with loading buffer (5% SDS, 5% beta-mercaptoethanol, 30% sucrose, bromophenol blue) and proteins were separated by SDS-PAGE, followed by transfer to PVDF membrane. The membrane was blocked with TBST + 5% dried, nonfat milk at 23*C for 30 min, incubated with anti-FLAG antibody (diluted 1:1,000 in TBST + 5% dried, nonfat milk) at 4*C for 10 hours, washed three times with TBST, incubated with horseradish-linked anti-mouse antibody (diluted 1:10,000 in TBST + 5% dried, nonfat milk) at 23*C for 1 hour, and washed three times with TBST. Proteins were visualized with chemiluminescent detection. Results from multiple clones (FIG. 10C) show that expression of the endo-p-glucanase gene in C. reinhardtii cells resulted in production of the protein. [00166] Similar results were seen (FIG. 11) with a similar construct containing the p-glucosidase gene from T. reesei (SEQ ID NO. 23, Table 4). The construct containing the endoxylanase gene is depicted in FIG. 2B. In this instance the segment labeled "Transgene" is the P-glucosidase encoding gene (SEQ ID NO. 17, Table 3), the segment which drives expression of the transgene (labeled 5' UTR) is the 5' UTR and promoter sequence for the psbC gene from C. reinhardii, the segment labeled 3' UTR contains the 3' UTR for the psbA gene from C. reinhardtii, and the segment labeled "Selection Marker" is the kanamycin resistance encoding gene from bacteria, which is regulated by the 5' UTR and promoter sequence for the arpA gene from C. reinhardtii and the 3' UTR sequence for the rbcL gene from from C. reinhardtii. The transgene cassette is targeted to the 3HB locus of C. reinhardtii via the segments labeled "5' Homology" and "3' Homology," which are identical to sequences of DNA flanking the 3HB locus on the 5' and 3' sides, respectively. All DNA manipulations carried out in the construction of this transforming DNA were essentially as described by Sambrook et al., Molecular Cloning: A Laboratory Manual (Cold Spring Harbor Laboratory Press 1989) and Cohen et al., Meth. Enzyinol. 297, 192-208, 1998.

[00167] FIG. 1 1A shows PCR using the gene-specific primer pair. As can be seen, multiple transformed clones are positive for insertion of the p-glucosidase gene. Figure IIB shows the PCR results using the primer pairs to differentiate homoplasmic from heteroplasmic clones. As can be seen, multiple transformed clones are either homoplasmic or heteroplasmic to a degree in favor of incorporation of the transgene (e.g. numbers 16, 64). Unnumbered clones demonstrate the presence of wild-type psbA and, thus, were not selected for further analysis. Western blot analysis demonstrating protein expression is demonstrated in FIG. 1 IC. Example 9. Construction of a Cyanobacteria strain expressing a biomass degrading enzyme construct that does not disrupt photosynthetic capability [00168] In this example, a construct is made which is capable of insertion into a selected cyanobacteria species (e.g., Synechocystis sp. strain PCC6803, Synechococcus sp. strain PCC7942, Thermosynechococcus elongates BP-1, and Prochloroccus marina). Examples of such constructs are represented graphically in FIG. 13. In addition to the transgene and regulatory sequences (e.g., promoter and terminator), typically, such constructs will contain a suitable selectable marker (e.g., an antibiotic resistance gene). The transgene may be any gene of interest, but is preferably a biomass degrading enzyme (e.g., a cellulolytic, hemicellulolytic, ligninolytic enzyme). A cassette, or portion of the vector, may be integrated into the host cell genome via homologous recombination when the exogenous DNA to be inserted is flanked by regions which share homology to portions of the cyanobacterial genome. Alternately, the construct may be a self-replicating vector which does not integrate into the host cell genome, but stably or transiently transforms the host cell. In some instances, regulatory elements, transgenes, and/or selectable markers may need to be biased to the preferred codon usage of the host organism. All DNA manipulations are carried out essentially as described by Sambrook et al., Molecular Cloning: A Laboratory Manual (Cold Spring Harbor Laboratory Press 1989) and Cohen et al., Meth. Enzymol. 297, 192-208, 1998. [00169] Transformation of Synechocystis with a construct of the present invention can be carried out by any method known in the art. (See, e.g., Dzelzkalns and Bogorad, J. Bacteriol. 165: 964-71 (1986)). For this example Synechocystis sp. strain 6803 is grown to a density of approximately 2x10 8 cells per ml and harvested by centrifugation. The cell pellet is re-suspended in fresh BG-11 medium (ATCC Medium 616) at a density of 1x10 9 cells per ml and used immediately for transformation. One-hundred microliters of these cells are mixed with 5 ul of a mini-prep solution containing the construct and the cells are incubated with light at 30*C for 4 hours. This mixture is then plated onto nylon filters resting on BG-I I agar supplemented with TES pH 8.0 and grown for 12-18 hours. The filters are then transferred to BG-11 agar + TES + Sug/ml ampicillin and allowed to grow until colonies appear, typically within 7-10 days. [00170] Colonies are then picked into BG-1 1 liquid media containing 5 ug/ml ampicillin and grown for 5 days. The transformed cells are incubated under low light intensity for 1-2 days and thereafter moved to normal growth conditions. These cells are then transferred to BG-11 media containing 10ug/ml ampicilin and allowed to grow for 5 days. Cells were then harvested for PCR analysis to determine the presence of the exogenous insert. Western blots may be performed (essentially as described above) to determine expression levels of the protein(s) encoded by the inserted construct. Example 10. Expression of biomass degrading enzymes in Escherichia coli [00171] In this example a nucleic acid encoding endo-p-glucanase from T. reesei was cloned into pET-21a using the Ndel and Xhol restriction sites present in both the gene and pET-21a. The resulting vector (SEQ ID NO. 25, Table 4) was transformed into E. coli BL-21 cells. Expression was induced when cell density reached OD=0.6. Cells were grown at 30'C for 5 hours and then harvested. Purification was essentially as described previously. Activity of the enzymes expressed in bacteria was determined using assays essentially as described in previous examples. The results of these analyses are shown in FIG. 17 (Lane 2). [001721 Nucleic acids encoding exo- -glucanase, p-glucosidase and endoxylanase were also cloned into pET 21. The resulting vectors (SEQ ID NOs. 24, 26 and 27, respectively, Table 4) were transformed into E. coli BL-21 cells. Expression was induced when cell density reached OD=0.6. Cells were grown at 30'C for 5 hours and then harvested. Purification was essentially as described previously. Activity of the enzymes expressed in bacteria was determined using assays essentially as described in previous examples. The results of these analyses are shown in FIG. 17 (Lane 1: exo->-glucanase; Lane 3: k-glucosidase; and Lane 4: endoxylanase). Enzyme activity was also measured, essentially as previously described. Results, which are presented in background-subtracted values, are provided in Table 5. Table 5. Enzyme activity of bacterially-produced biomass degrading enzymes Enzyme Added Filter paper assay p-glucosidase assay Xylanase assay Control (TBS) 0.000 0-000 0.000 endo-p-glucanase 0.194 0.000 0.020 p-glucosidase 0.006 0.525 0.000 endoxylanase 0.000 0.011 3.131 [00173] This data, along with the data shown in previous examples, demonstrates that the enzymes encoded by the vectors described herein can be functionally expressed by both algae and bacteria, despite the codon bias built into the sequences. [00174] Various modifications, processes, as well as numerous structures that may be applicable herein will be apparent. Various aspects, features or embodiments may have been explained or described in relation to understandings, beliefs, theories, underlying assumptions, and/or working or prophetic examples, although it will be understood that any particular understanding, belief, theory, underlying assumption, and/or working or prophetic example is not limiting. Although the various aspects and features may have been described with respect to various embodiments and specific examples herein, it will be understood that any of same is not limiting with respect to the full scope of the appended claims or other claims that may be associated with this application. [001751 As used herein, except where the context requires otherwise, the term "comprise" and variations of the term, such as "comprising", "comprises" and "comprised", are not intended to exclude other additives, components, integers or steps. [001761 Reference to any prior art in the specification is not, and should not be taken as, an acknowledgment, or any form of suggestion, that this prior art forms part of the common general knowledge in Australia or any other jurisdiction or that this prior art could reasonably be expected to be ascertained, understood and regarded as relevant by a person skilled in the art.

Claims

1. A method for determining endoxylanase activity in a eukaryotic non-vascular photosynthetic organism, comprising obtaining a eukaryotic non-vascular photosynthetic organism having an exogenous nucleotide sequence encoding an endoxylanase; lysing the organism to obtain a lysate; adding an endoxylanase substrate to the lysate; and determining the endoxylanase activity.

2. The method of claim 1, wherein said determining is accomplished by measuring absorbance at 590 nm.

3. The method of claim 1, wherein said organism is selected from the group consisting of cyanophyta, prochlorophyta, rhodophyta, chlorophyta, heterokontophyta, tribophyta, glaucophyta, chlorarachniophytes, euglenophyta, euglenoids, haptophyta, chrysophyta, cryptophyta, cryptomonads, dinophyta, dinoflagellata, pyrmnesiophyta, bacillariophyta, xanthophyta, eustigmatophyta, raphidophyta, and phaeophyta.

4. The method of claim 1, wherein a plastid of said organism is transformed with said nucleotide sequence.

5. The method of claim 4, wherein said plastid is in homoplasmic state.

6. The method of claim 1, wherein said nucleotide sequence is identical to an endoxylanase sequence in a bacterium or an endoxylanase sequence in a fungus.

7. The method of claim 1, wherein said exogenous nucleotide sequence further encodes an epitope tag.

8. The method of claim 7, wherein said epitope tag is a FLAG epitope tag.

9. The method of claim 1, wherein said organism is lysed by sonication.

10. The method of claim 1, further comprising clarifying the lysate to produce a clarified lysate.

11. The method of claim 10, further comprising purifying the endoxylanase using said epitope tag.

12. The method of claim 11, wherein said purifying is accomplished using an antibody to said epitope tag. -83-

13. The method of claim 12, wherein said antibody is to a FLAG epitope tag.

14. The method of claim 1, further comprising filtering said lysate prior to determining the endoxylanase activity.

15. A method for determining endoxylanase activity in a eukaryotic non-vascular photosynthetic organism, comprising obtaining a eukaryotic non-vascular photosynthetic organism having an exogenous nucleotide sequence encoding an endoxylanase and an epitope tag; lysing the organism to obtain a lysate; clarifying the lysate to produce a clarified lysate; isolating the endoxylanase using the epitope tag; adding an endoxylanase substrate to the isolated endoxylanase; and determining the endoxylanase activity.

16. The method of claim 15, wherein said determining is accomplished by measuring absorbance at 590 nm.

17. The method of claim 16, further comprising filtering said isolated endoxylanase prior to determining the endoxylanase activity.

18. A method according to claim 1, substantially as hereinbefore described.

19. A method according to claim 15, substantially as hereinbefore described. _R4_