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AU2005201855B2 - Chroman derived compounds and formulations thereof for use in therapy - Google Patents
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AU2005201855B2 - Chroman derived compounds and formulations thereof for use in therapy - Google Patents

Chroman derived compounds and formulations thereof for use in therapy Download PDF

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Publication number
AU2005201855B2
AU2005201855B2 AU2005201855A AU2005201855A AU2005201855B2 AU 2005201855 B2 AU2005201855 B2 AU 2005201855B2 AU 2005201855 A AU2005201855 A AU 2005201855A AU 2005201855 A AU2005201855 A AU 2005201855A AU 2005201855 B2 AU2005201855 B2 AU 2005201855B2
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AU
Australia
Prior art keywords
formula
hmc
compounds
compound
hydroxyphenyl
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AU2005201855A
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AU2005201855A1 (en
Inventor
Andrew Heaton
Alan Husband
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Marshall Edwards Inc
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Marshall Edwards Inc
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Filing date
Publication date
Priority claimed from JP2004315009A external-priority patent/JP4976649B2/en
Priority claimed from AU2004906363A external-priority patent/AU2004906363A0/en
Application filed by Marshall Edwards Inc filed Critical Marshall Edwards Inc
Priority to AU2005201855A priority Critical patent/AU2005201855B2/en
Priority to MX2007003216A priority patent/MX2007003216A/en
Priority to ES05787045T priority patent/ES2431045T3/en
Priority to ES11175917.1T priority patent/ES2516067T3/en
Priority to ES05779877T priority patent/ES2377073T3/en
Priority to PCT/AU2005/001436 priority patent/WO2006032086A1/en
Priority to PCT/AU2005/001435 priority patent/WO2006032085A1/en
Priority to CN2005800380156A priority patent/CN101094844B/en
Priority to HK07113859.6A priority patent/HK1108685B/en
Priority to ES11180383.9T priority patent/ES2586847T3/en
Priority to AT05779877T priority patent/ATE532777T1/en
Priority to NZ553834A priority patent/NZ553834A/en
Priority to HK08101549.6A priority patent/HK1112617B/en
Priority to EP05787045.3A priority patent/EP1809618B1/en
Priority to EP11180383.9A priority patent/EP2436680B1/en
Priority to EP05779877A priority patent/EP1794141B1/en
Priority to EP20110175917 priority patent/EP2407462B1/en
Priority to CA2581316A priority patent/CA2581316C/en
Priority to NZ553835A priority patent/NZ553835A/en
Priority to AU2005287865A priority patent/AU2005287865B2/en
Priority to CN2005800381178A priority patent/CN101056868B/en
Priority to JP2007531541A priority patent/JP4913056B2/en
Priority to MX2007003215A priority patent/MX2007003215A/en
Publication of AU2005201855A1 publication Critical patent/AU2005201855A1/en
Priority to IL182034A priority patent/IL182034A/en
Priority to IL182042A priority patent/IL182042A/en
Priority to NO20071578A priority patent/NO20071578L/en
Priority to NO20072004A priority patent/NO20072004L/en
Assigned to MARSHALL EDWARDS, INC. reassignment MARSHALL EDWARDS, INC. Request for Assignment Assignors: NOVOGEN RESEARCH PTY LTD
Publication of AU2005201855B2 publication Critical patent/AU2005201855B2/en
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Description

AUSTRALIA PATENTS ACT 1990 COMPLETE SPECIFICATION NAME OF APPLICANT(S):: Novogen Research Pty Ltd ADDRESS FOR SERVICE: DAVIES COLLISON CAVE Patent Attorneys Level 10, 10 Barrack Street,Sydney, New South Wales, Australia, 2000 INVENTION TITLE: Chroman derived compounds and formulations thereof for use in therapy The following statement is a full description of this invention, including the best method of performing it known to me/us:- C:WRPonb\DCC\1MDT\4150213_1 DOC-22PJ2/2012 -1 CHROMAN DERIVED COMPOUNDS & FORMULATIONS THEREOF FOR USE IN THERAPY Field of the Invention The present invention relates to certain novel isoflavan derivatives, compositions containing same, methods for their preparation and uses thereof as therapeutic agents particularly as anti-cancer and chemotherapeutic selective agents. Background of the Invention Over 700 different naturally occurring isoflavones are known some of which have biological properties with potential therapeutic benefit. US 5,726,202 generically discloses certain isoflavan compounds, particularly 3,4 diarylchroman and centchroman for the treatment of benign prostatic hypertrophy. WO 01/17986 also discloses certain isoflavan compounds. Summary of the Invention Surprisingly, the present inventors have found a novel group of compounds of the general formula (I) which exhibit important therapeutic activities including strong anti-cancer activity, chemotherapeutic selectivity and radiosensitisation of cancers. In a first aspect the present invention provides a compound of the general formula (I): Rx R10 0 (I) --- R3 0 R2 R5 R6 R4 wherein C:\NRPortblDCC\MDT4 150213_1.DOC-22A12/2012 -2
R
1 is hydrogen,
R
2 and R 3 are independently hydrogen, hydroxy, alkoxy, alkyl, cycloalkyl, halo or
OC(O)R
7 , with the exception that R 2 and R 3 are not both hydrogen, R4, R 5 and R.
6 are independently hydrogen, hydroxy, alkoxy, alkyl, cycloalkyl, acyl,
NH
2 , NHC 1
-C
4 alkyl or N(Ci-C 4 alkyl) 2 , OC(O)R 7 or OR 8 ,
R
7 is hydrogen, alkyl, cycloalkyl, aryl, arylalkyl or amino,
R
8 is phenyl or benzyl, and Rx is hydrogen, hydroxy, alkoxy, alkyl, cycloalkyl or halo, or a pharmaceutically acceptable salt thereof. In a second aspect the present invention provides a compound of formula (I) according to the first aspect of the general formula (I-X): (I-X) -R3 R5 R6 R R4 wherein R, is hydrogen,
R
2 and R 3 are independently hydrogen, hydroxy, alkoxy, alkyl, cycloalkyl, halo or
OC(O)R
7 , with the exception that R 2 and R 3 are not both hydrogen,
R
4 , R 5 and R 6 are independently hydrogen, hydroxy, alkoxy, alkyl, cycloalkyl, acyl or
OC(O)R
7 , and
R
7 is hydrogen, alkyl, cycloalkyl, aryl, arylalkyl or amino, or a pharmaceutically acceptable salt thereof. In a third aspect the present invention provides a process for the preparation of a compound of formula (I-X) as defined in the second aspect comprising the step of reacting C:\NRPortbI\DCC\MD\4150213. .DOC-22M2/202 -3 the 4-keto group of a compound of the formula (II): R10 0 (II) - R3 R2 wherein
R
1 , is alkyl or Si(RA) 3 ,
R
2 and R 3 are independently hydrogen, alkoxy or OSi(RA)3, with the exception that R 2 and R 3 are not both hydrogen, and RA is independently alkyl or aryl, with an arylating agent W~M*, wherein W~ is a benzene ring optionally substituted with the groups R 4 , R 5 and R 6 , wherein R 4 ,
R
5 , R 6 and R 7 are as defined in the second aspect, and M+ is one or more counter ions, to form the intermediate tertiary alcohol of formula (III): R10 O (III) HO - -R3 R2 or a salt thereof and which is dehydrated to form a compound of formula (IV): R10 0 (IV) --- R3 R2 which is subsequently hydrogenated and deprotected to form a compound of formula (I-X).
CINRPonbl\DCCMDT4150213_l.DOC-222/2112 -4 Disclosed herein is a compound of the general formula (III), compositions containing same and uses thereof. Also disclosed herein is a compound of the general formula (IV), compositions containing same and uses thereof. Further disclosed herein is the use of a compound of formula (I) in therapy, particularly chemotherapy and/or as radiosensitising or chemosensiti sing agents. In a fourth aspect the present invention provides a method for the treatment or amelioration of a cancer or a tumour mass, which comprises administering to a subject one or more compounds of the formula (I) or (I-X) as defined in the first or second aspects or a pharmaceutically acceptable salt or derivative thereof, optionally in association with a carrier and/or excipient. In a fifth aspect the present invention provides use of one or more compounds of formula (I) or (I-X) as defined in the first or second aspects in the treatment of cancer or a tumour mass. In a sixth aspect the present invention provides use of one or more compounds of formula (I) or (I-X) as defined in the first or second aspects or a pharmaceutically acceptable salt or derivative thereof, in the manufacture of a medicament for the treatment of cancer or a tumour mass. In a seventh aspect the present invention provides an agent for the treatment, prophylaxis or amelioration of cancer or a tumour mass, which agent comprises one or more compounds of formula (I) or (I-X) as defined in the first or second aspects or a pharmaceutically acceptable salt or derivative thereof.
C:\NRPonbl\DCCMDT\415023_ LDOC-22/22012 - 4a In an eighth aspect the present invention provides a pharmaceutical composition which comprises one or more compounds of formula (I) or (I-X) as defined in the first or second aspects or a pharmaceutically acceptable salt thereof, in association with one or more pharmaceutical carriers, excipients, auxiliaries and/or diluents. In a ninth aspect the present invention provides a drink or food-stuff, which contains one or more compounds of formula (I) or (I-X) as defined in the first or second aspects or a pharmaceutically acceptable salt thereof. These and other aspects of the invention will become evident from the description and claims which follow, together with the accompanying drawings. Brief Description of the Figures Fig. I represents a comparison of dehydroequol (DHE graph A), 3-(4-hydroxyphenyl)-4 (4-methoxyphenyl)chroman-7-ol (HMC compound 1 according to the invention graph B) and cisplatin (graph C) toxicity in neonatal foreskin fibroblasts. Fig. 2 represents HMC efficacy in melanoma cells in comparison with cisplatin. Fig. 3 represents a pharmacokinetic profile of free and total forms of HMC (A) and DHE (B) after p.o (peri oral) administration to BALB/c mice (50 mg/kg).
P:\WPDOCS\Bah\NOVOG EN\SPEC\1 254345 .AUcomplete.doc-03/05/05 -5 Fig. 4 represents a comparison of the pharmacokinetic profile the HMC concentration in serum after i.v (intravenously) and i.p (intraperitoneally) administration of HMC formulated in 20% hydroxypropyl-beta-cyclodextrin at a dose of 50 mg/kg. Fig. 5 represents comparative mean tumour volume data taken from nude mice bearing HPAC pancreatic cancer tumours treated with either i.p dosed 20% HPBCD (vehicle control, qdx15) or HMC (100 mg/kg, qdx15). Data represented as mean ± SEM *, student's T-test, p < 0.01. Fig. 6 represents comparative mean terminal tumour mass data taken from nude mice bearing HPAC pancreatic cancer tumours treated with either i.p dosed 20% HPBCD (vehicle control, qdx15) or HMC (100 mg/kg, qdx15). Data represented as mean ± SEM *, student's T-test, p <0.01. Fig. 7 represents comparative mean terminal tumour mass data taken from nude mice bearing HPAC pancreatic cancer tumours treated with either i.p dosed 20% HPBCD (vehicle control, qdx15) or HMC (100 mg/kg, qdx15). Data represented as mean ± SEM. *, student's T-test, p < 0.01. Fig. 8 represents a summary of apoptosis incidence in DHE and HMC treated melanoma cells over a 24 and 48 hour period. Fig. 9 represents selective initiation of programmed cell death in HMC and DHE treated malignant melanoma cells (Mel-RM and Me4405). The same concentration of DHE and HMC and exposure times do not induce apoptosis in normal fibroblasts (MRC-5). Fig. 10 represents a 3D analysis of HMC-cisplatin synergy cytotoxicity data in the MM200 melanoma cell line. HMC-cisplatin combinations were assessed using a 5-day combination protocol (Fig 10 A), or a 24 hr HMC-+ anti-cancer sequence (Fig 10 B). For each combination experiment HMC was assessed at 10, 5, 2 and 1 pM. See Table 8 for raw data. Fig. 11 represents the percentage inhibition of TNFx in murine macrophages by compounds 6 and 7 of the invention. Fig. 12 represents the chromatograph of 3-(4-hydroxyphenyl)-4-(4 hydroxyphenyl)chroman-7-ol when subjected to preparative HPLC.
P:\WPDOCS\Bah\NOVOGEN\SPECI254345 LAUcomplete.doc-03/0 5 /0 5 -6 Detailed Description of the Invention The present inventors have found that a class of isoflavan derivatives of the general formula (I) show surprising and unexpected biological and pharmaceutical properties. The compounds of formula (I) of the invention are believed to have favourable toxicity profiles with normal cells and good bioavailability. Surprisingly the compounds of the invention exhibit anti-cancer activity, significantly better than or at least comparable to known cancer treatments. The compounds of formula (I) are cytostatic and cytotoxic against a broad range of cancer cells of human and animal origin. By cancer cells, it is meant cells that display malignant characteristics and which are distinguished from non-cancer cells by unregulated growth and behaviour which usually ultimately is life-threatening unless successfully treated. The cancer cells that have been found to be responsive to compounds of formula (I) are of epithelial origin (for example, prostate, ovarian, cervical, breast, gall-bladder, pancreatic, colorectal, renal, and non-small lung cancer cells), of mesenchymal origin (for example, melanoma, mesothelioma and sarcoma cancer cells), and of neural origin (for example glioma cancer cells). It is highly unusual and surprising to find a related group of compounds that display such potent cytotoxicity against cancer cells, but with low toxicity against non-cancer cells such as keratinocytes derived from human foreskin. Such cancer cell selectivity is highly unusual and unexpected. Advantageously the compounds of formula (I) show cytotoxicity against cancer cells that are well recognized for being poorly sensitive to standard anti-cancer drugs. It is highly unusual and unexpected to find such potent activity against cancers, for example, cholangiocarcinoma, pancreatic adenocarcinoma and melanoma. Advantageously the compounds of formula (I) also unexpectedly display an ability to radio-sensitise cancer cells, by which it is meant that these compounds either lower the amount of gamma-irradiation that is required to kill the cells, or they convert cancer cells from a state of radio-resistance to a radio-sensitive state.
P:\WPDOCS\Bah\NOVOGEN\SPEC\ 254345 1. AUcomplete.doc-03/05/05 -7 Additionally the compounds of formula (I) are thought to possess chemo-sensitising activity, that is they increase the cytotoxicity of chemotherapeutic agents, especially to cancer cells, and/or convert cancerous cells from a state of chemo-resistance to a chemo sensitive state. Compounds of the invention may also provide chemo and/or radio-protective properties for non-cancerous cells. This has significant therapeutic implications because the traumatic side-effects of chemotherapy and radiotherapy are caused by the toxicity of the traditional treatments to non-cancerous cells. The properties described above offer significant clinical advantages. The radio and/or chemo-protective properties of the compounds of the invention may be employed to protect healthly individuals from the effects of radiation and/or chemical toxins, or lessen the effects of the same. Thus, the invention also provides the use of compounds of formula (I) to treat patients with cancer by either reducing the rate of growth of such tumors or by reducing the size of such tumors through therapy with said compounds alone, and/or in combination with each other, and/or in combination with other anti-cancer agents, and/or in combination with radiotherapy. The use of compounds of the present invention either alone or in combination therapy as described above may reduce the adverse side-effects often experienced by patients when treated with standard anti-cancer treatments. The use of compounds of the invention may mean that lower doses can be employed in such therapy which represents an important advance for cancer sufferers. Preferably R 3 in compounds of formula (I) is in the 3-position. In one aspect of the invention Rx is not hydrogen. However, preferably in compounds of formula (I) Rx is hydrogen or CI-C 4 alkyl such as methyl, especially hydrogen.
P:\WPDOCS\Bah\NOVOGEN\SPEC\l2543451.AUcomplete.do-0 3 /05/05 References to compounds of formula (I) in this specification are intended to include other compounds/formulas of the invention unless otherwise indicated. Compounds of the invention include those of formula (I-a): R10 0 R3 (I-a) R5 R6 R 5Y R4 wherein
R
1 is hydrogen, alkyl, cycloalkyl or C(O)R 7 ,
R
2 and R 3 are independently hydrogen, hydroxy, alkoxy, halo or OC(O)R 7 , with the exception that R 2 and R 3 are not both hydrogen,
R
4 , R 5 and R 6 are independently hydrogen, hydroxy, alkoxy, alkyl, cycloalkyl, acyl, OC(O)R7, and
R
7 is hydrogen, alkyl, cycloalkyl, aryl or arylalkyl. Preferably in compounds of formula (I-a):
R
1 is hydrogen, CI-C 4 alkyl or C(O)R 7 ,
R
2 and R 3 are independently hydrogen, hydroxy, C I-C 4 alkoxy, halo or OC(O)R 7 , provided that R 2 and R 3 are not both hydrogen, R4, R 5 and R 6 are independently hydrogen, hydroxy, alkoxy, alkyl, cycloalkyl, acyl,
OC(O)R
7 , and
R
7 is C 1
-C
4 alkyl, phenyl or benzyl, or a pharmaceutically acceptable salt or derivative thereof. More preferably in compounds of formula (I-a):
R
1 is hydrogen, methyl, ethyl, propyl, isopropyl or acetyl,
R
2 and R 3 are independently hydrogen, hydroxy, methoxy, ethoxy, propoxy, isopropoxy, bromo, chloro, fluoro or acetyloxy, with the exception that R 2 and R 3 P:\WPDOCS\Bah\NOVOGEN\SPECI254345 1. AUcoplIet.doc-03/05/05 -9 are not both hydrogen,
R
4 is hydrogen, hydroxy, methoxy, ethoxy, propoxy, isopropoxy or acetyloxy, and
R
5 and R 6 are independently hydrogen, hydroxy, methoxy, ethoxy, propoxy, isopropoxy, acetyl, or acetyloxy, or a pharmaceutically acceptable salt or derivative thereof. Particular preferred compounds of formula (I-a) have the following substituents where:
R
1 is hydrogen, methyl or acetyl,
R
2 and R 3 are independently hydrogen, hydroxy, methoxy, bromo or acetyloxy, with the exception that R 2 and R 3 are not both hydrogen,
R
4 and R 6 are independently hydrogen, hydroxy, methoxy or acetyloxy, and
R
5 is hydrogen, or a pharmaceutically acceptable salt or derivative thereof. The invention also extends to compounds of formula (I-b) R O O (I-b) R5 R4 wherein:
R
1 represents hydrogen or CI-C 6 alkyl, more preferably hydrogen or methyl, especially hydrogen.
R
2 represents hydrogen, hydroxy or C 1
-C
6 alkoxy such as methoxy, ethoxy, propoxy, more preferably hydroxy or methoxy, especially hydroxy.
R
3 represents hydrogen, hydroxy C 1
-C
6 alkoxy such as methoxy, ethoxy, propoxy, more preferably hydrogen or methoxy, especially hydrogen, with the proviso that R 2 and R 3 do not both represent hydrogen,
R
4 represents hydrogen, hydroxy C 1
-C
6 alkoxy such as methoxy, ethoxy, propoxy, C 1
-
P:\WPDOCS\Bah\NOVOGEN\SPEC\l2543451.AUomplete.do-0 3 /0 5 /05 -10
C
6 alkyl such as methyl, ethyl, propyl, isopropyl, especially hydrogen, hydroxy, methoxy or methyl particularly methoxy or hydroxy,
R
5 represents hydrogen, C 1
-C
6 alkoxy, Ci-C 6 alkyl, especially hydrogen, methoxy, hydroxy, particularly hydrogen, or a pharmaceutically acceptable salt or derivative thereof. Preferred compounds of the invention include those of the general formula (I-c): R10 0 (I-c) OR2a wherein:
R
1 is hydrogen or C 1
-C
6 alkyl such as methyl, ethyl, propyl, isopropyl, butyl, isobutyl, secbutyl, tertiary butyl,
R
2 a is hydrogen or C 1
-C
6 alkyl such as methyl, ethyl, propyl, isopropyl, butyl, isobutyl, secbutyl, tertiary butyl, and
R
3 a is hydrogen or CI-C 6 alkyl such as methyl, ethyl, propyl, isopropyl, butyl, isobutyl, secbutyl, tertiary butyl, or a pharmaceutically acceptable salt or a derivative thereof. More preferably in compounds of formula (I-c) R 1 is hydrogen or methyl, especially hydrogen. More preferably in compounds of formula (I-c) R 2 a is hydrogen or methyl, especially hydrogen. More preferably in compounds of formula (I-c) R 3 a is hydrogen or methyl, especially methyl.
P:\PDCS&hNOOGN\SEC 2435 A~o~pet~-11-010 Especially preferred compounds of formula (I) include: 3-(-yrxpey)4(-etoyhnlcrmn7o (HMC) (Cpd. 1); 3-(4-hydroxyphenyl)-4-phenylchroman7-o (Cpd. 2); 3-4hdoyhnl--3mtoyhnlcrmn7o (Cpd. 3); 3-(3 ,4-dimethoxyphenyl)-4-(4-methoxyphenyl)chroman 7 oI (Cpd. 4); 3-(-yrxpeyl -4mtypenlcrmn7o (Cpd. 5); 3-(-ehxpey) -4mtoyhnl)7mtoyhoa (Cpd. 6); 3-(-yrxpey)4(,-iehoy4hdoyhnlcrmn7o (Cpd. 7); 3-(4-hydroxyphenyl)-4-(2-hydroxyphenyl)chroman- 7 -oI (Cpd. 8); 3-4hdoyhnl--3ay--ydoy4mtoyhnlcrmn7o (Cpd. 9); 3 -(3 -hydroxyphenyl)-4-(3-methoxyphenyl)chroman 7 -o (Cpd. 10); 3-4hdoyhnl--4hdoyhnlcrmn7o (Cpd. 11); 3-(4-bromophenyl)-4-(4-methoxyphenyl)chroman- 7 -o (Cpd. 12); 3-(4-hydroxyphenyl)-4-(3-mfethoXyphenyl)chroman 7 -o (Cpd. 13); 3 -(4-hydroxyphenyl)-4-(3-aminophenyl)chroman 7 -o (Cpd. 14); 3-(4-hydroxyphenyl)-4-(4-phenoxypheflyl)chroman 7 -o (Cpd 15); 3-(3,4dmtoyhnl -4mtoxpey)8mtycrmn7o (Cpd 16). 1 1 ( ) 1 1(2) PAWPDOCS\BWhNOVOGEN\SPEC\1 2543451. AUCmpktcd.-3/ 5
/
5 HO~ 12 -e (6) ((8) OH(12) Me(14) P:\WPDOCS\Bah\NOVOGEN\SPECI 2543451.AUcomplete.doc-03/05/05 - 13 HO 0 OH(15) HO O W 0 (16) OWe or a pharmaceutically acceptable salt thereof. The compounds of formula (I) according to the invention include two chiral centres. The present invention includes all the enantiomers and diastereoisomers as well as mixtures thereof in any proportions. The invention also extends to isolated enantiomers or pairs of enantiomers. Methods of separating enantiomers and diastereoisomers are well known to person skilled in the art. It will be clear to persons skilled in the art that the in compounds of formula (I) the aryl substituents on the heterocyclic ring can be cis or trans relative to each other. Preferably in the compounds of formula (I) these substituents will be cis. A particularly preferred compound of the present invention is the cis-isomer of HMC: HO 0 OH OWe or a pharmaceutically acceptable salt thereof. Likewise, particularly preferred compounds are compound Nos. (2) to (16) in the cis conformation.
p:\WPDOCS\Bah\NOVOGEN\SPEC\254345.AUcomplete.doc03/0 5 /05 -14 In an alternative aspect the invention provides compounds of formula (I-d): R10 0 R2b (1-d) OR3a wherein:
R
1 is as defined above for compounds of formula (I), R2b represents hydroxy, C 1
-C
6 alkyl or C 1
-C
6 alkoxy, especially hydroxy or methoxy, and R3a is as defined above for compounds of formula (I-c) In a further alternative aspect the invention provides compounds of formula (I-e): R10 0 R3 R2 (I-e) wherein
R
1 , R2 and R3 are as defined above for compouds of formula (I).
p:\WPDOCS\Bah\NOVOGEN\SPEC\12543451.AI~complete.doc-03/05/05 - 15 Preferably in compounds of formula (I-e) R 1 represents hydrogen or methyl, especially hydrogen. Preferably in compounds of formula (I-e) R 2 represents hydroxy or C 1
-C
6 alkoxy such as methoxy. In compounds of formula (I-e) preferably R 3 represents hydrogen, hydroxy or methoxy, especially hydrogen. In a further alternative aspect the invention provides compounds of formula (I-f): R10 0 R2 (I-f) R4a wherein
R
1 , R 2 and R 3 are as defined above for compouds of formula (I), and
R
4 a represents hydroxy, alkoxy, alkyl, cycloalkyl, acyl, NH 2 , NHCI-C 4 alkyl or N(C 1
-C
4 alkyl)2, OC(O)R 7 or OR 8 , and
R
8 is defined above for compounds of formula (I). Preferably in compounds of formula (I-f) R 1 represents hydrogen or methyl, especially hydrogen. Preferably in compounds of formula (I-f) R 2 represents hydroxy or C 1
-C
6 alkoxy such as methoxy, especially hydroxy. Preferably in compounds of formula (I-f) R 3 represents hydrogen or C 1
-C
6 alkoxy such as methoxy, especially hydrogen.
P:\WPDOCS\Bah\NOVOGEN\SPEC\l 254345 1. AUcOmplete.doc-03/05/05 - 16 Preferably in compounds of formula (I-f) R 3 is in the 3-position. Preferably in compounds of formula (14) R 4 a represents NH2, NHC 1
-C
4 alkyl or N(C 1
-C
4 alkyl)2, especially NH 2 . The compounds of formulae (III) and (IV) are intermediates as set out herein. Each corresponding isoflavan-4-ol and isoflavan-3-ene intermediate of compound Nos. (1) to (12) are also preferred compounds of the present invention. W in compounds of formula (III) and (IV) may, for example, represent the following radicals: R (V-1) (V-2) R5 0R5 R6 R4 R4 R5 R6 (V-3)
R
6 (V-4)
R
5 R4 R4 or a protected derivative thereof wherein R 4 , R 5 and R 6 are as defined above for compounds of formula (I). The term "isoflavone" as used herein is to be taken broadly to include as isoflavones, isoflavenes, isoflavans, isoflavanones, isoflavanols and the like. The term "alkyl" is taken to include straight chain and branched chain saturated alkyl groups of 1 to 6 carbon atoms, such as methyl, ethyl, propyl, isopropyl, butyl, isobutyl, secbutyl, tertiary butyl, pentyl and the like. The alkyl group more preferably contains P:\WPDOCS\3ah\NOVOGEN\SPECI254345t AUcomplee.doc-03/05/05 - 17 preferably from 1 to 4 carbon atoms, especially methyl, ethyl, propyl or isopropyl. Cycloalkyl includes C 3
.
6 cycloalkyl such as cylopropyl, cyclobutyl, cyclopentyl and cyclohexyl. The alkyl group or cycloalkyl group may optionally be substituted by one or more of fluorine, chlorine, bromine, iodine, carboxyl, CI-C 4 -alkoxycarbonyl,
C
1
-C
4 -alkylamino carbonyl, di-(CI-C 4 -alkyl)-amino-carbonyl, hydroxyl, CI-C 4 -alkoxy, formyloxy, C 1
-C
4 alkyl-carbonyloxy, C1-C 4 -alkylthio, C 3
-C
6 -cycloalkyl or phenyl. Preferably the alkyl group does not bear any substituents. The term "aryl" is taken to include phenyl, benzyl, biphenyl and naphthyl and may be optionally substituted by one or more C 1
-C
4 -alkyl, hydroxy, C 1
-C
4 -alkoxy, carbonyl, CI
C
4 -alkoxycarbonyl,
C
1
-C
4 -alkylcarbonyloxy, nitro or halo. The term "halo" is taken to include fluoro, chloro, bromo and iodo, preferably fluoro and chloro, more preferably fluoro. Reference to for example "haloalkyl" will include monohalogenated, dihalogenated and up to perhalogenated alkyl groups. Preferred haloalkyl groups are trifluoromethyl and pentafluoroethyl. The compounds of the invention include all salts, such as acid addition salts, anionic salts and zwitterionic salts, and in particular include pharmaceutically acceptable salts as would be known to those skilled in the art. The term "pharmaceutically acceptable salt" refers to an organic or inorganic moiety that carries a charge and that can be administered in association with a pharmaceutical agent, for example, as a counter-cation or counter-anion in a salt. Pharmaceutically acceptable cations are known to those of skilled in the art, and include but are not limited to sodium, potassium, calcium, zinc and quaternary amine. Pharmaceutically acceptable anions are known to those of skill in the art, and include but are not limited to chloride, acetate, tosylate, citrate, bicarbonate and carbonate. Pharmaceutically acceptable salts include those formed from: acetic, ascorbic, aspartic, PAWPDOCSBah\NOVOGEN\SPEC\12543451.AUcompletedoc-03/05/05 - 18 benzoic, benzenesulphonic, citric, cinnamic, ethanesulphonic, fumaric, glutamic, glutaric, gluconic, hydrochloric, hydrobromic, lactic, maleic, malic, methanesulphonic, naphthoic, hydroxynaphthoic, naphthalenesulphonic, naphthalenedisulphonic, naphthaleneacrylic, oleic, oxalic, oxaloacetic, phosphoric, pyruvic, p-toluenesulphonic, tartaric, trifluoroacetic, triphenylacetic, tricarballylic, salicylic, sulphuric, sulphamic, sulphanilic and succinic acid. The term "pharmaceutically acceptable derivative" or "prodrug" refers to a derivative of the active compound that upon administration to the recipient is capable of providing directly or indirectly, the parent compound or metabolite, or that exhibits activity itself and includes for example phosphate derivatives and sulphonate derivatives. Thus, derivatives include solvates, pharmaceutically active esters, prodrugs or the like. This also includes derivatives with physiologically cleavable leaving groups that can be cleaved in vivo to provide the compounds of the invention or their active moiety. The leaving groups may include acyl, phosphate, sulfate, sulfonate, and preferably are mono-, di- and per-acyl oxy-substituted compounds, where one or more of the pendant hydroxy groups are protected by an acyl group, preferably an acetyl group. Typically acyloxy substituted compounds of the invention are readily cleavable to the corresponding hydroxy substituted compounds. Chemical functional group protection, deprotection, synthons and other techniques known to those skilled in the art may be used where appropriate to aid in the synthesis of the compounds of the present invention, and their starting materials. The protection of functional groups on the compounds and derivatives of the present invention can be carried out by well established methods in the art, for example as described in T. W. Greene, Protective Groups in Organic Synthesis, John Wiley & Sons, New York, 1981. Hydroxyl protecting groups include but are not limited to carboxylic acid esters, eg acetate esters, aryl esters such as benzoate, acetals/ketals such as acetonide and benzylidene, ethers such as o-benzyl and p-methoxy benzyl ether, tetrahydropyranyl ether and silyl ethers such P:\WPDOCS\Bah\NOVOGEN\SPEC\ 254345 1. AUcompletedoc-03/05/05 - 19 as t-butyldimethyl silyl ether. Protecting groups can be removed by, for example, acid or base catalysed hydrolysis or reduction, for example, hydrogenation. Silyl ethers may require hydrogen fluoride or tetrabutylammonium fluoride to be cleaved. It will be clear to persons skilled in the art of medicinal chemistry that compounds of formula (I) may be converted into other compounds of formula (I), for example, where a compound of formula (I) bears one or more hydroxyl substituents then one or more of these substituents can be converted in to a halo substituent such as bromo, chloro or iodo by treating the alcohol with a halogenating agent. Halogenating agents include compounds like NBS, hydrobromic acid, chlorine gas etc. It may be necessary during processes such as halogenation to use protecting groups to protect other functionality in the molecule. Phenolic type hydroxyls may not be readily convertible to the corresponding halogen compound by treatment with a halogenating agent. However, the desired halogen compound may be prepared by, for example, treating an appropriate aryl amine starting material with NaNO 2 in the presence of HCl under reduced temperature conditions such as 0 0 C, to form the corresponding azide salt. Subsequent treatment with CuCl, CuBr, KI or
HBF
4 may be used to convert the azide into the required halo-compound. A general process for preparing compounds of formula (I) comprises the step of treating a compound of formula (IV): R10 0 (IV) -- R3 R2 wherein R 1 , R 2 , R 3 and W are as defined above in relation to compounds of formula (II) with a reducing agent to provide a compounds of formula (I) or a protected derivative P:\WPDOCS\1ah\NOVOGEN\SPEC\l 254345 I.AUcomplete.do-03/05/05 - 20 thereof. Reducing agents are well known to persons skilled in the art and can include hydride sources like borohydrides and alkali metal borohydrides, but would include hydrogen in catalytic hydrogenation where a suitable catalyst such as palladium on carbon may be used. Other suitable hydride sources include sodium triacetoxyborohydride tetrabutyl ammonium triacetoxyborohydride and sodium cyanoborohydride. Preferably the double bond in compounds of formula (IV) is reduced by hydrogenation. Compounds of formula (IV) are prepared by dehydrating a compound of formula (III): R10 0 (III) HO - -R3 R2 wherein R 1 , R 2 , R 3 and W are as defined above, in relation to compounds of formula (II) or a protected derivative thereof. Dehydration can, for example, be catalysed by acid, by base or facilitated by conversion of the tertiary alcohol into a better leaving group as would be known to those skilled in the art. Preferably compounds of formula (III) are dehydrated, for example, by treatment with para-toluene sulphonic acid. Compounds of formula (III) may be prepared by treating compounds of formula (II): P:\WPDOCS\Bah\NOVOGEN\SPEC\ 12543451.AUcomplete.doc-03/05/05 - 21 R10 O (II) -- R3 R2 wherein R 1 , R 2 , R 3 are as defined above for compounds of formula (II) or a protected derivative thereof with an arylating agent, for example, a compound of formula W~M* wherein W- is an optionally substituted aryl radical and M* is one ore more counter ions, preferably [MgBr]+. The arylating agent W-M* may be prepared by Grignard chemistry where the haloaryl compound (V): X
R
5 R6 (V) R4 or a protected derivative thereof wherein
R
4 , R 5 and R 6 are independently hydrogen, alkoxy, alkyl, acyl, OC(O)R 7 or a protected hydroxy such as OSi(RA)3, and RA is independently alkyl or aryl, and X is halo, preferably bromo, is reacted with a metal such as magnesium to form the arylating agent. Preferably the haloaryl compound (V) is selected from: x x x R6 R5 R6 R (VA) / (VB) (VC)
R
5 R4 R4 P:\WPDOCS\Bah\NOVOGEN\SPEC\1254345 .AUcompletedo-03/05105 -22 wherein R 4 , R 5 , Ra and X are as defined above for compounds of formula (V). Reaction of the arylating agent with the ketone of formula (II) provides access to the corresponding isoflavan-4-ols (III), isoflav-3-enes (IV) and isoflavans (I) of the present invention. Alternatively compounds of formula (III) may be prepared by reacting compounds of formula (II) with a compound analogous to compounds of formula (V) wherein X represents any appropriate leaving group L which is lost in the formation of the product by nucleophilic addition of the aryl moiety to a ketone by reactions well known by those skilled in the art. Preferably any free alcohols, esters or other such reactive groups in the keto compounds of formula (II) will be protected, for example, as t-butyldimethylsilyl ethers during the nucleophilic addition reaction. Compounds of formula (II) can be prepared by reducing the eneone double bond in compounds of formula (VI): R10 0 (VI) 0- R3 R2 or a protected derivative thereof, wherein R 1 , R 2 and R 3 are as defined above, for compounds of formula (II). Suitable reducing agents are described above. Preferably reduction of the carbon-carbon double bond can be effected, for example, by hydrogenation. Access to compounds of general formula (VI) is available by general synthetic methods as set out in Scheme 1 below and as described in published International application No.
P:\WPDOCS\Bah\NOVOGEN\SPEC 12543451.AUcomplete~do-03/05/05 - 23 WOO1/17986, the disclosure of which is incorporated herein by reference.
R
1 0 OH + HO
BF
3 /Et 2 O +H
-R
3 70 0 C
R
1 0 OH R10 0 (vi) MeSO 2 CI -- R3 DMF R3 R2 0R2 Scheme I Access to the variatious 3-phenyl substituted chromans is available by varying the substitution pattern on the phenylacetic acid derived group. Access to the 4-phenyl substituted chromans is available by varying the substitution pattern of the arylating agent (V). Analogues of compounds employed in the processes may be used which include a substituent which corresponds to Rx as defined for compounds of formula (I). As used herein, the terms "treatment", "prophylaxis" or "prevention", "amelioration" and the like are to be considered in their broadest context. In particular, the term "treatment" does not necessarily imply that an animal is treated until total recovery. Accordingly, "treatment" includes amelioration of the symptoms or severity of a particular condition or preventing or otherwise reducing the risk of developing a particular condition. The amount of one or more compounds of formula (I) which is required in a therapeutic treatment according to the invention will depend upon a number of factors, which include the specific application, the nature of the particular compound used, the condition being treated, the mode of administration and the condition of the patient.
P:\WPDOCS\Bah\NOVOG EN\SPEC\ 1254345 LAUcomplete.doc-03/05/05 - 24 Compounds of formula (I) may be administered in a manner and amount as is conventionally practised. See, for example, Goodman and Gilman, "The pharmacological basis of therapeutics", 7th Edition, (1985). The specific dosage utilised will depend upon the condition being treated, the state of the subject, the route of administration and other well known factors as indicated above. In general, a daily dose per patient may be in the range of 0.1 mg to 5 g; typically from 0.5 mg to 1 g; preferably from 50 mg to 200 mg. The length of dosing may range from a single dose given once every day or two, to twice or thrice daily doses given over the course of from a week to many months to many years as required, depending on the severity of the condition to be treated or alleviated. It will be further understood that for any particular subject, specific dosage regimens should be adjust over time according to the individual need and the professional judgment of the person administering or supervising the administration of the compositions. Relatively short-term treatments with the active compounds can be used to cause stabilisation or shrinkage or remission of cancers. Longer-term treatments can be employed to prevent the development of cancers in high-risk patients. The production of pharmaceutical compositions for the treatment of the therapeutic indications herein described are typically prepared by admixture of the compounds of the invention (for convenience hereafter referred to as the "active compounds") with one or more pharmaceutically or veterinary acceptable carriers and/or excipients as are well known in the art. The carrier must, of course, be acceptable in the sense of being compatible with any other ingredients in the formulation and must not be deleterious to the subject. The carrier or excipient may be a solid or a liquid, or both, and is preferably formulated with the compound as a unit-dose, for example, a tablet, which may contain up to 100% by weight of the active compound, preferably from 0.5% to 59% by weight of the active compound. One or more active compounds may be incorporated in the formulations of the invention, which may be prepared by any of the well known techniques of pharmacy consisting P:\WPDOCS\Bah\NOVOGEN\SPEC 1254345 LAUcomplete.o-03/05/05 - 25 essentially of admixing the components, optionally including one or more accessory ingredients. The preferred concentration of active compound in the drug composition will depend on absorption, distribution, inactivation, and excretion rates of the drug as well as other factors known to those of skill in the art. The formulations of the invention include those suitable for oral, rectal, ocular, buccal (for example, sublingual), parenteral (for example, subcutaneous, intramuscular, intradermal, or intravenous), transdermal administration including mucosal administration via the nose, mouth, vagina or rectum, and as inhalants, although the most suitable route in any given case will depend on the nature and severity of the condition being treated and on the nature of the particular active compound which is being used. Formulation suitable for oral administration may be presented in discrete units, such as capsules, sachets, lozenges, or tablets, each containing a predetermined amount of the active compound; as a powder or granules; as a solution or a suspension in an aqueous or non-aqueous liquid; or as an oil-in-water or water-in-oil emulsion. Such formulations may be prepared by any suitable method of pharmacy which includes the step of bringing into association the active compound and a suitable carrier (which may contain one or more accessory ingredients as noted above). In general, the formulations of the invention are prepared by uniformly and intimately admixing the active compound with a liquid or finely divided solid carrier, or both, and then, if necessary, shaping the resulting mixture such as to form a unit dosage. For example, a tablet may be prepared by compressing or moulding a powder or granules containing the active compound, optionally with one or more other ingredients. Compressed tablets may be prepared by compressing, in a suitable machine, the compound of the free-flowing, such as a powder or granules optionally mixed with a binder, lubricant, inert diluent, and/or surface active/dispersing agent(s). Moulded tablets may be made by moulding, in a suitable machine, the powdered compound moistened with an inert liquid binder.
P:\WPDOCSBah\NOVOGEN\SPEC 12543451.AUcomplete~do-03/05/05 -26 Formulations suitable for buccal (sublingual) administration include lozenges comprising the active compound in a flavoured base, usually sucrose and acacia or tragacanth; and pastilles comprising the compound in an inert base such as gelatine and glycerin or sucrose and acacia. Formulations suitable for ocular administration include liquids, gels and creams comprising the active compound in an ocularly acceptable carrier or diluent. Compositions of the present invention suitable for parenteral administration conveniently comprise sterile aqueous preparations of the active compounds, which preparations are preferably isotonic with the blood of the intended recipient. These preparations are preferably administered intravenously, although administration may also be effected by means of subcutaneous, intramuscular, or intradermal injection. Such preparations may conveniently be prepared by admixing the compound with water or a glycine buffer and rendering the resulting solution sterile and isotonic with the blood. Injectable formulations according to the invention generally contain from 0.1% to 60% w/v of active compound and can be administered at a rate of 0.1 ml/minute/kg. Formulations for infusion, for example, may be prepared employing saline as the carrier and a solubilising agent such as a cyclodextrin or derivative thereof. Suitable cyclodextrins include a-cyclodextrin, 0-cyclodextrin, -- cyclodextrin, dimethyl-0 cyclodextrin, 2-hydroxyethyl-0-cyclodextrin, 2-hydroxypropyl-cyclodextrin, 3 hydroxypropyl--cyclodextrin and tri-methyl--cyclodextrin. More preferably the cyclodextrin is hydroxypropyl-0-cyclodextrin. Suitable derivatives of cyclodextrins include Captisol@ a sulfobutyl ether derivative of cyclodextrin and analogues thereof as described in US 5,134,127. Formulations suitable for rectal administration are preferably presented as unit dose suppositories. Formulations suitable for vaginal administration are preferably presented as unit dose pessaries. These may be prepared by admixing the active compound with one or more conventional solid carriers, for example, cocoa butter, and then shaping the resulting mixture.
P:\WPDOCS\Bah\NOVOGEN\SPEC\1254345.AUometedo-0 3 /05/0 5 - 27 Formulations or compositions suitable for topical administration to the skin preferably take the form of an ointment, cream, lotion, paste, gel, spray, aerosol, or oil. Carriers which may be used include Vasoline, lanoline, polyethylene glycols, alcohols, and combination of two or more thereof The active compound is generally present at a concentration of from 0.1% to 5% w/w, more particularly from 0.5% to 2% w/w. Examples of such compositions include cosmetic skin creams. Formulations suitable for transdermal administration may be presented as discrete patches adapted to remain in intimate contact with the epidermis of the recipient for a prolonged period of time. Such patches suitably contain the active compound as an optionally buffered aqueous solution of, for example, 0.1 M to 0.2 M concentration with respect to the said active compound. See for example Brown, L., et al. (1998). Formulations suitable for transdermal administration may also be delivered by iontophoresis (see, for example, Panchagnula R, et al., 2000) and typically take the form of an optionally buffered aqueous solution of the active compound. Suitable formulations comprise citrate or Bis/Tris buffer (pH 6) or ethanol/water and contain from 0.1 M to 0.2 M active ingredient. Formulations suitable for inhalation may be delivered as a spray composition in the form of a solution, suspension or emulsion. The inhalation spray composition may further comprise a pharmaceutically acceptable propellant such as carbon dioxide or nitrous oxide or a hydrogen containing fluorocarbon such as 1,1,1,2-tetrafluoroethane, 1,1,1,2,3,3,3 heptafluoro-n-propane or mixtures thereof. The active compounds may be provided in the form of food stuffs, such as being added to, admixed into, coated, combined or otherwise added to a food stuff. The term food stuff is used in its widest possible sense and includes liquid formulations such as drinks including dairy products and other foods, such as health bars, desserts, etc. Food formulations containing compounds of the invention can be readily prepared according to standard practices.
P;\WPDOCS\ah\NOVOGEN\SPEC\i254345.AUcmplcte.dc-0 3 /05/0 5 - 28 Therapeutic methods, uses and compositions may be for administration to humans or other animals, including mammals such as companion and domestic animals (such as dogs and cats) and livestock animals (such as cattle, sheep, pigs and goats), birds (such as chickens, turkeys, ducks), marine animals including those in the aquaculture setting (such as fish, crustaceans and shell fish) and the like. The active compound or pharmaceutically acceptable derivatives prodrugs or salts thereof can also be co-administered with other active materials that do not impair the desired action, or with materials that supplement the desired action, such as antibiotics, antifungals, antiinflammatories, or antiviral compounds. The active agent can comprise two or more isoflavones or derivatives thereof in combination or synergistic mixture. The active compounds can also be administered with lipid lowering agents such as probucol and nicotinic acid; platelet aggregation inhibitors such as aspirin; antithrombotic agents such as coumadin; calcium channel blockers such as verapamil, diltiazem, and nifedipine; angiotensin converting enzyme (ACE) inhibitors such as captopril and enalapril, and 3 blockers such as propanolol, terbutalol, and labetalol. The compounds can also be administered in combination with nonsteriodal antiinflammatories such as ibuprofen, indomethacin, aspirin, fenoprofen, mefenamic acid, flufenamic acid and sulindac. The compounds can also be administered with corticosteroids or an anti-emetic such as zofran@. Compounds of formula (I) seem to be particularly suitable for co-administration with one or more anti-cancer drugs such as cisplatin, dehydroequol (DHE), taxol (paclitaxel), gemcitabine, doxorubicin, topotecan and/or camptothecin, especially cisplatin, dehydroequol (DHE), taxol. This may result in improved effects in the treatment, for example in the form of synergistic effects, in comparison to when only one of the medicaments is employed. Particularly the compounds of the presently claimed invention, especially HMC (ie compound 1) seem to be chemosensitisers and increase the cytotoxicity of the one or more anticancer drug co-administered therewith. This seems to be the case even though said anticancer drugs work through a variety of different mechanisms, for example cisplatin is thought to work by interacting with nuclear DNA, taxol is thought to work by blocking cells in the G2/M phase of the cell cycle and prevent P:WPDOCSBah\NOVOGEN\SPEC\12543451.AUoplee.d-03/05/05 - 29 them forming normal mitotic apparatus, gemcitabine is thought to work by incorporating itself into the DNA of the cell, ultimately preventing mitosis, doxorubicin is though to be a topoisomerase II inhibitor thereby preventing DNA replication and transcription and topotecan is thought to be a topoisomerase I inhibitor. Interestingly, in some situations this increased cytotoxicity to cancerous cells is not associated with a corresponding increase in toxicity to non-cancerous cells. Whilst this observation has important implications for the treatment of many cancers, it is especially important to the treatment of cancers such as melanoma, which are extremely difficult to treat. The co-administration may be simultaneous or sequential. Simultaneous administration may be effected by the compounds being in the same unit dose, or in individual and discrete unit doses administered at the same or similar time. Sequential administration may be in any order as required and typically will require an ongoing physiological effect of the first or initial active agent to be current when the second or later active agent is administered, especially where a cumulative or synergistic effect is desired. The invention also extends to a pack comprising the combination therapy. Compounds for use in the preferred synthetic methods of the present invention may be derived from any number of sources readily identifiable to a person skilled in the art. For example, daidzein is readily available or can be synthesised by standard methods known in the art. Suitable methods may be found in, for example, published international patent applications WO 98/08503 and WO 00/49009, and references cited therein, which are incorporated herein in their entirety by reference. Compounds of the general formulae (II), (III) and (IV) described above are intermediates in the production of the active isoflavan compounds of formula (I). These intermediates also represent further aspects of the present invention.
P:\WPDOCS\Bah\NOVOGEN\SPEC'I254345 LAUcomplte.dc-03/0505 -30 Whilst not wishing to be bound by theory the compounds of the present invention are thought to regulate a wide variety of signal transduction processes within animal cells and that these signal transduction processes are involved in a wide range of functions that are vital to the survival and function of all animal cells. Therefore, these compounds have broad-ranging and important health benefits in animals including humans, and in particular have the potential to prevent and treat important and common human diseases, disorders and functions, which represents a substantial unexpected benefit. Thus it seems that the compounds of the present invention have activity as TNFa inhibitors. It Is hypothesised that TNFa is part of a tightly regulated cytokine network, activating multiple signal transduction pathways and inducing or suppressing a wide variety of genes. TNFa can provide a survival signal for cancer cells and hence it has been referred to as a tumour promoting factor. As a central mediator of inflammation, TNFa provides a molecular link between chronic inflammatory stimuli and the subsequent development of malignant disease. Consequently its inhibition by the compounds of the invention may provide one mechanism by which they exert anti-cancer and/or anti inflammatory activity. Alternatively, these compounds may be used as chemopreventative agents. The particular benefits of this invention lie in (a) the large range of signal transduction processes targeted by the compounds, (b) the fact that regulation of these various processes includes both up-regulation of some processes and down-regulation of others, and (c) that such a broad and varied effect on signal transduction processes also is accompanied by an independent effect on a range of important enzymes that are fundamental to metabolism and steroidogenesis. The isoflavan compounds of the present invention exhibit good in vitro toxicity profiles against normal cells. The isoflavans have broad activity, markedly better than or at least comparable with dehydroequol. The isoflavans are highly active against cancer cells representative of leukaemia, glioma, prostate, ovarian, breast and lung cancer. The isoflavan compounds show potent activity against melanoma and cholangiocarcinoma (gall bladder cancer) cell lines. Good activity was observed against colorectal cancer P:\WPDOCS\Bah\NOVOGEN\SPEC\l2543451.AUcomplcte.dc-03/05/05 -31 cells. Radio-sensitisation in vivo may be tested for example employing human epidermoid vulval carcinoma A431 tumours established on the upper leg and subjected to several doses of local radiation (to the tumour bearing leg only). A radiation treatment regimen of 2.5Gy/day for 4 days will delay tumour growth, and the effect of the radiation dose in combination with the test compound could be assessed by monitoring tumour growth delay. Tumour growth delay of-6 days can be expected using radiation alone. Tumour growth delay using orally dosed test compound can be determined separately. Evidence of test compound mediated radio-sensitisation of A431 tumours is then determined by measuring tumour growth delay using a regimen of orally dosed test compound pre-treated animals followed by the standard radiation therapy regimen described above. A mean growth delay of up to 30 days using the combination treatment compared to up to 10 days using either radiation or test compound monotherapy regimens is evidence of the radio sensitisation properties of the compounds of the invention. Radio-sensitisation in vitro may be tested, for example, employing clonogenic assays using human the human epidermoid vulva carcinoma A431 cell line to measure response to radiation alone or in combination with test compounds. A drug dose causing 10% toxicity to the cells may be used in combination with graded doses of radiation. The appropriate dose of compound would be determined by clonogenic assay. Evidence of test compound mediated radio-sensitisation is shown by, for example, a >20% toxicity to cells using chemoradiation therapy compared to 10% toxicity using the corresponding monotherapy regimens. The invention is further illustrated by the following non-limiting Examples and accompanying drawings. Examples In the Examples and accompanying drawings which follow the abbreviation "DHE" is used for dehydroequol and the abbreviation "HMC" is used herein for the compound, 3-(4 hydroxyphenyl)-4-(4-methoxyphenyl)-chroman-7-ol.
P:\WPDOCS\Bah\NOVOGEN\SPEC\I 254345 1. AUcomplmetedoc-03/05/05 - 32 1.0. Synthesis Example 1: 4',7-Diacetoxydaidzein H O 0 H.0 0 Acetic Anhydride 0 Pyridine O O / OH O / A mixture of daidzein (2.0 g), acetic anhydride (10 ml) and pyridine (2 ml) was heated at 105-110 C for 1h. After cooling the mixture to room temperature, it was stirred for a further 30 min during which time the diacetate crystallised from solution. The product was filtered, washed thoroughly with water and recrystallised from methanol to yield 4',7 diacetoxydaidzein as colourless prisms (2.4 g, 90%). Example 2: 7-Acetoxy-3-(4-acetoxyphenyl)chroman-4-one Y jH 2 , Catalyst YO 0 0 . 0 NN 0 O O Palladium-on-charcoal (5%, 0.02g) was added to a solution of 4',7-diacetoxydaidzein (0.50g, 1.5 mmol) in ethyl acetate (80 ml) and the mixture was stirred at room temperature under a hydrogen atmosphere for 72h. The catalyst was removed by filtration through Celite and the resulting filtrate was evaporated in vacuo. The residue was recrystallised from ethanol to yield 7-acetoxy-3-(4-acetoxyphenyl)chroman-4-one (0.40g, 80%) as colourless plates. Example 3: 7-Hydroxy-3-(4-hydroxyphenyl)chroman-4-one P:\WPDOCS\Bah\NOVOGEN\SPEC\I254345 L.AUcompletedo-03/05/05 -33 O O Imidazole HO 0 0 OH Imidazole (0.63g) was added to a suspension of 4',7-diacetoxydihydrodaidzein (0.26g, 0.08 mmol) in absolute ethanol (5.0 ml) and the mixture was refluxed for 45 min under argon. The solution was concentrated under reduced pressure and distilled water (10 ml) was added to the residue. The mixture was left overnight under refrigeration and the resulting precipitate was filtered. The crude product was recrystallised from ethyl acetate/dichloromethane to yield 7-hydroxy-3 -(4-hydroxyphenyl)chroman-4-one (0.14g, 71%) as a white powder. Example 4: 7-(tert-Butyldimethlysilyloxy)-3-(4-(tert-butyldimethlysilyloxy) phenyl)chroman-4-one HO sO tBMSCI ---- 0 Imidazole OH O-Si 7-Hydroxy-3-(4-hydroxyphenyl)chroman-4-one 42g, imidazole 130g, tert butyldimethylsilyl chloride 127g, and N,N-dimethylformamide (500ml) were combined in a 2L round bottom flask and stirred under nitrogen at room temperature for 16 hours. The reaction was quenched with the addition of chilled H 2 0 (200ml) with the reaction mix cooled in an ice bath. The resultant white solid was filtered and rinsed with water. Recrystallisation from ethanol afforded the product as white fluffy crystals (35.7g). Example 5: 7-(tert-Butyldimethylsilyloxy)-3-(4-(tert-butyldimethylsilyloxy)phenyl)-4 (4-methoxyphenyl)chroman-4-ol P:\WPDOCS\Bah\NOVOGEN\SPEC0l2543451.AUcomplete.doc-03/05/05 -34 Mg Br S -O O 6-0 0 0 0-S HO O-SI OMe 7-(tert-Butyldimethylsilyloxy)-3-(4-(tert-butyldimethylsilyloxy)phenyl)-4-( 4 methoxypenyl)chroman-4-ol 25g was weighed in a 2-neck round bottom flask, and flushed under nitrogen. Anhydrous THF 80ml was added to the reaction vessel to give a clear slightly yellow solution. A condenser was attached and the reaction vessel placed in an ice bath. Commercial 4-methoxyphenylmagnesium bromide (0.5M solution in THF) 225ml was added to the reaction mix dropwise over 10 minutes. The reaction was quenched by the dropwise addition of wet ether (50:50 H 2 0: diethyl ether) while still under nitrogen, with a white precipitate forming as increasing amounts of H 2 0 was added. A further amount of H 2 0 was added to the reaction mix before extraction with diethyl ether. The organic layers were combined and washed with water, brine, dried over anhydrous MgSO 4 and solvent removed on rotovap to give clear yellow oil which solidified overnight to give an off-white solid. The crude product was used in the next step without purification. Example 6: 3-(4-Hydroxyphenyl)-4-(4-methoxyphenyl)-2H-chromen-7-ol -si-O O HO 0 I+ F 0pTsOH H HO O-Si OH OMe OMe 7-(tert-Butyldimethylsilyloxy)-3-(4-(tert-butyldimethylsilyloxy)phenyl)-4-(4 methoxyphenyl)chroman-4-ol (42g), pTsOH (435g), boiling chips and 2.5L of ethanol P:\WPDOCS\Bah\NOVOGEN\SPEC\1254345.AUomple.d-03/05/05 -35 were combined in a 2-neck 5L round bottom flask with condenser attached. The reaction was heated at reflux for 3 hours. The solvent was concentrated in vacuo to -100ml before being poured into chilled, stirred water (700ml). The mixture was then extracted with ethyl acetate, the combined organic layers washed with water (3 x 2L), brine (1 x 500ml), dried over anhydrous magnesium sulphate and filtered and solvent removed in vacuo to give red/ brown oil. The oil was dissolved in methanol (~100ml) and put in freezer overnight. A white precipitate had formed overnight, which was filtered off and rinsed with methanol. The filtrate was concentrated in vacuo to give a brown oil. Example 7: 3-(4-Hydroxyphenyl)-4-(4-methoxyphenyl)-chroman-7-o HO O HO O
H
2 /Pd OH ethanol OH OMe OMe 3-(4-hydroxyphenyl)-4-(4-methoxyphenyl)-2H-chromen-7-o 25,5g (70mmoles), 10% Pd/A1 2 0 3 3.95g and 200ml of ethanol were combined in a 2-neck 500ml round bottom flask. The reaction was hydrogenated at low pressure using standard conditions for 3 hours. The reaction was filtered through Celite to remove the catalyst, rinsed through with ethanol (300ml). The filtrate was concentrated to -50ml before being poured into chilled, stirred water (1.4L). A pale orange precipitate formed which then formed a brown oil. The mixture was then extracted with diethyl ether, the combined organic layers washed with water (3 x 1L), brine (1 x 500ml), dried over anhydrous magnesium sulphate and filtered. The solvent was removed in vacuo to give red/ brown oil. The product was recrystallised from diethyl ether (-100ml), to give brown solid which was rinsed with chilled diethyl ether to give off-white crystals 11.3g. The 1H NMR spectrum and numbering scheme being shown below.
P:\WPDOCS\Bah\NOVOGEN\SPECI 254345 .AUcomplmetedc-03/05/05 -36 HO 4.1 8a 0 2 3 2' 6 4 1' 5 .1241 6" 6 Cd ,,2" 5O 4" 3" O H 8 ppm Peak Shape J Hz Integrates Connnents C2equatorial 4.14 Dd 10.98 1 C2axial 4.35 D 1 Dd is overlapping C3 3.47 Ddd 1 C4 4.20 Dd 5.12 1 C5 6.71 D 8.05 1 C6 6.36 Dd 2.56, 8.42 1 C8 6.41 D 2.20 1 C9 3.71 S - 3 CTC' 66 Doublets overlapping for C2',C3',C2" C3" C3', C ' 6.61 D - 2 Total integration is 8 C2", C6" 6.61 D - 2 C3", C5" 6.61 D - 2 In the above general methods, the structures may be optionally substituted or protected with appropriate substituents, or synthons or derivatives thereof. The compounds may be present as, for example, their salts, acetates, benzyl or silyloxy derivatives as can be determined by a skilled synthetic chemist. Hydroxy groups can be readily alkylated (MelIbase), acylated (Ac 2 0/Py) or silylated (Cl-SiR 3 /base) and likewise deprotected by standard methods known in the art. Example 8: 3-(4-Hydroxyphenyl)-4-(4-hydroxyphenyl)-chroman-7-ol 3-(4-hydroxyphenyl)-4-(4-methoxyphenyl)chroman-7-ol (3.17g) was transferred to a round bottom flask and the flask was purged with nitrogen. 33 wt.% Hydrogen bromide in acetic acid (1 3ml) was added drop-wise to the flask and the contents were heated to reflux at 130*C for 7 hours. The reaction mixture was placed in an ice bath and adjusted to pH 6 using sodium hydroxide solution (40%w/v). The mixture was extracted with ethyl acetate and the ethyl acetate layer was further washed with water and brine prior to drying over P:\WPDOCS\Bah\NOVOGEN\SPEC0I2543451.AUcomplet.doc-03/05/05 - 37 magnesium sulphate. The mixture was filtered and the solvent was removed in vacuo to yield a brown solid (2.89g). The solid was dissolved in minimal ethyl acetate and purified by column chromatography (Silica 60H, 200-400mesh using ethyl acetate:chloroform (40:60) eluant). 3-(4-hydroxyphenyl)-4-(4-hydroxyphenyl)chroman-7-ol was obtained in -80% purity and was further purified by semi-preparative high performance liquid chromatography (HPLC) see Fig. 12. 2.0. Materials and Methods 2.1. Tissue culture The human pancreatic cancer cell line, HPAC (CRL-2119) was routinely cultured in 1:1 mixture DMEM (Dulbecco's Modified Eagle Medium Sigma) plus Ham's F12 (Sigma) medium containing HEPES (15 mM), insulin (0.002 mg/ml), transferrin (0.005 mg/ml), hydrocortisone, (40 ng/ml), epidermal growth factor (10 ng/ml). The ovarian cancer cell lines; CP70 was obtained as a gift from Dr. Gil Mor (Yale University) and cultured in a 1:1 mixture DMEM plus Ham's F12 medium, and SKOV-3 (ovarian cancer cell line) was purchased from ATCC and cultured in McCoys 5a medium. The breast cancer cell line MDA-MB-468 cultured in Leibovitz's L-15 medium. The melanoma cell line MM200 was obtained as a gift from Peter Hersey (University of Newcastle) and A2058 was obtained as a gift from Dr Peter Parsons (QIMR). Both were cultured in DMEM medium. All cultures were supplemented with 10% FCS (fetal calf serum CSL, Australia), penicillin (1 OOU/ml), streptomycin (100mg/ml), L-glutamine (2mM) and sodium bicarbonate (1.2 g/L), and cultured at 37 0 C in a humidified atmosphere of 5% CO 2 . All cell lines were purchased from ATCC (Maryland, USA) except where noted. The normal cell line NFF (neonatal foreskin fibroblasts) was a gift from Dr. Peter Parsons (Queensland Institute of Medical Research). RK (rabbit kidney) cells were obtained from Miller Whalley (Macquarie University). Both cell lines were cultured in RPMI supplemented with 10% FCS (CSL, Australia), penicillin (10OU/ml), streptomycin (100mg/ml), L-glutamine (2mM) and sodium bicarbonate (1.2 g/L), and cultured at 37*C in a humidified atmosphere of 5% CO 2
.
P:\WPDOCS\Bah\NOVOG EN\SPEC\ 1254345L1AUcomplete.doc-03/05/05 - 38 2.2. Proliferation assays IC50 values were determined for each cell line. Cells were seeded in 96-well plates at an appropriate cell density as determined from growth kinetics analysis and cultured for 5 days in the absence and presence of the test compounds. Cell proliferation was assessed after the addition of 20 pl of 3-4,5 dimethylthiazol-2,5-diphenyl tetrazolium bromide (MTT, 2.5mg/ml in PBS, Sigma) for 3-4hrs at 37*C according to manufacturer's instructions. IC50 values were calculated from semi-log plots of % of control proliferation on the y-axis against log dose on the x-axis. 2.3. DHE and HMC Pharmacokinetics - Oral HMC and DHE were prepared as homogenous suspensions in 1% CMC (m:v, water). Both formulations were delivered orally by gavage to female BALB/c mice at a dosage of 50 mg/kg. Three animals were allocated to each timepoint (15 min, 30 min, lhr, 4 hr and 24 hr). At each respective timepoint, animals were euthanased by cervical dislocation and blood collected. Free HMC was analysed by mass spectroscopy. 2.4. HMC Pharmacokinetics - i.v. and i.p. HMC was prepared as a solution in 20% hydroxypropyl-beta-cyclodextrin (m:v, water). The formulation was delivered either orally by gavage or by i.p. injection to female BALB/c mice at a dosage of 50 mg/kg. Three animals were allocated to each timepoint (15 min, 30 min, lhr, 4 hr and 24 hr). At each respective timepoint, animals were euthanased by cervical dislocation and blood collected. Urine was also collected and analysed for HMC. Free HMC was analysed by mass spectroscopy. 2.5 Pilot in vivo efficacy study - HPAC tumour bearing mice Subconfluent (80%) flasks of HPAC cells were trypsinised, washed in Hanks balanced salt solution (Sigma), resuspended in dubellco's minimal essential medium (Sigma) and an equal volume of matrigel m (Becton Dickson) at a density of 3.7 x 107 cells per ml. Athymic nu/nu BALB/c mice were s.c. inoculated with 3.7x 106 HPAC cells bi-laterally midway along the dorsal surface. For the HMC (n=3 per dosage regimen) and control groups (n=2), treatment commenced five days post inoculation to allow tumour formation. HMC was formulated 20% HPBCD and delivered i.p. daily for 15 days. The control group P:\WPDOCS\Bah\NOVOGEN\SPEC 1254345 LAUcomplete.doc-03/05/05 -39 received equivalent (weight:weight) i.p. doses of 20% HPBCD. Tumour measurements commenced on day 5 post inoculation (10 x10 mm 2 ) and were measured in 2 dimensions, length (a) and width (b), using calipers. Tumor weight (W) was calculated by the formula W=ab2 /2, where a, is the longer of the 2 measurements (Odwyer et al., 1994). Tumour proliferation curves were analyzed with respect to maximal tumour inhibition (treated/control, T/C). On sacrifice, liver, kidney, femur, stomach and colon tissue were fixed in buffered formalin, embedded in paraffin, sections cut and stained with H&E. Stained sections were then submitted to Rothwell consulting for histopathology analysis. Serum biochemistry was conducted on bloods taken from control, vehicle control and HMC treatment groups. Serum analysis was conducted by Veterinary Clinical pathology (U. Syd). 2.6 Three-D model analysis of synergy 3-D model analysis of the cytotoxic interaction between drug A and drug B enables the representation of predicted inhibitory effect of two drugs in combination in 3 dimensions to reveal actual regions of synergy or antagonism. The 3D synergy plots are based on a theory of "Theretical Additivity" (TA) as outlined by Kanzawa et al (Int. J. Cancer 71, 311-319 (1997)). Theoretical Additivity was calculated from the cytotoxicities of drug A and drug B as monotherapies using the following formula which assumes the drugs are mutually exclusive inhibitors: (fa)A + (fa)B - 2 (fa)A(fa)B TAol = 1 - (fa)A(fa)B Where: (fa)A = fraction of cells affected by drug A (fa)B = fraction of cells affected by drug B The TA is calculated for each combination of drug concentrations and subtracted from the observed experimental effect for each combination to give a measurement of synergistic action. A positive difference indicates that more cells are affected by the drug combination than would be expected in theory if the two drugs were administered together - hence synergism. A negative difference indicates that less cells were affected than theoretically expected - hence antagonism.
P:\WPDOCS\Bah\NOVOGEN\SPEC\2543451.AUcomplte.dc-0 3 /05/05 - 40 3.0. Results 3.1. Normal cell toxicity Dehydroequol (DHE) was less toxic to both NFF and rabbit kidney cells with IC50 values above 150 piM when compared to HMC (86 and 61 pM respectively) (Table 1 and Figure 1). When compared to cisplatin a benchmark chemotherapeutic agent, the degree of toxicity exhibited by HMC is mild (9.9 pM vs 86 pM). Table 1. Relative toxicity of DHE, HMC and cisplatin against Neonatal foreskin fibroblasts (NFF) and rabbit kidney cells. Analogue (IC50 UM) Antineoplastic Tissue/cell Type Designation A (IC50 uM) DHE HMC Cisplatin Fibroblast Neonatal Foreskin Fibroblasts >150 86.12 ± 7.6 9.85 ± 5 (Human, NFF) Kidney Rabbit Kidney >150 1 4.3 Not tested 3.2. In vitro efficacy against cancer cells When compared to DHE IC50 values, HMC demonstrated markedly superior activity (-5 10 fold greater) against the multi-drug resistant, p53 mt ovarian cancer cell line (SKOV-3), the AR negative, p53 Mt prostate cancer cell line (PC3), both ER positive (p53 wt) and negative (p53 mt) breast cancer cell lines (MCF-7 and MDA-MB-468 respectively), p53 Mt Glioma (HTB-138), p53 Mt pancreatic cancer (HPAC) and p53 Mt large cell lung cancer (Table 2). HMC exhibited anti-cancer activity comparable to that of DHE against all other cell lines tested (Table 1). Particular efficacy of HMC was noted against melanoma cells. (Table 2 and Fig 2). This represents a substantial advantage over the prior art. HMC was differentially active against 2 separate colorectal cell lines, with marked activity observed against HT-29 cells and somewhat less activity against HCT-15. It is noted that HT-29 and HCT- 15 are COX-2 positive and deficient respectively. When examined microscopically and compared to cells treated with vehicle only, HMC treated SKOV-3 cells exhibited morphological changes consistent with cells undergoing apoptosis (cell enlargement, granular appearance in cytosol and blebbling of plasma membrane). In P:\WPDOCS\Bah\NOVOGEN\SPECl2543451.AUcompletdc-3/05/05 -41 contrast SKOV-3 cells exposed to 100 tM Dehydroequol after 18 hr retained a relatively normal morphology, comparable with that of vehicle only treated cells. Table 2. Comparison of Dehydroequol and HMC cytoxicity against cell lines representative of different malignancies. Analogue (IC50 uM) Antineoplastic Indication Designation ________ _______ (1C50 uM) DHE HIMC Cisplatin A2780 1.7 ±0.61 1.58 ±0.59 2.10 Ovarian CP70 1.69 ±0.62 1.21 ±0.29 10.30 SKOV-3 21.83 ± 4.65 2.26 5.40 PC3 9.09 ±8.12 2.9 ±0.92 2.11 Prostate LNCaP 4.8 ± 3.8 4.52 >10 DU145 5.95 ± 1.5 3.78 2.07 Breast MCF-7 21.5 ± 13.2 7.15 ± 7 3.69 Breast MDA-MB-468 7.9 ±3.5 1.1 ±0.35 0.58 Glioma HTB-138 7.35 ±0.89 1.9 ±0.27 42.30 Pancreatic CRL-2119 56.62 ± 16.8 14.1± 1.16 9.36 Leukemic RPMI-8226 3.72 ± 0.08 NT NT CCRF-CEM 1.7 ± 0.68 1.90 NT NCI-H23 8.75 ± 7.2 3.75 ± 2.5 NT Lung NCI-H460 10.6 ± 3.8 2.23 ± 0.15 22.29 Colorectal HT-29 50.45 ± 21.9 3.7 ± 1.4 22.7 ± 35 Colorectal HCT-15 24.4 ± 12.57 37.8 ± 33 129.9 ± 39 MM200 2.90 0.7 ± .03 8.3 ± 0.7 Melanoma A2058 NT 1.2 ± 0.65 5.73 ± 2.3 IGR-3 NT 0.53 ±0.02 NT 3.3. HMC Pharmacokinetics - oral When compared with the pharmacokinetic profile of orally dosed DHE, HMC administered via the same route and dosage (50 mg/kg), HMC exhibited a Cmax of 141 pM (achieved after 1 hr) compared to 511 pM for DHE (achieved after 15 min) (Table 3 and Figure 3). Like DHE, HMC is also subject to conjugation with low plasma concentrations of the free form of the molecule observed (1.3 pM after 30 min) (Table 3 and Figure 3). This is less than half the maximum concentration of free dehydroequol achieved using the same dosage regimen (3.3 pM after 15 min) (Figure 3). The ratio of free:total is greater for HMC when compared to DHE (0.92 vs 0.64 respectively). Table 3. Comparison of free and total plasma concentrations achieved in mice dosed with 50 mg/kg of either HMC or DHE p.o.
PAWPDOCS\Bah\NOVOGEN\SPEC\254345 .AUcomplme.dc-03/05/05 -42 Time HMC (uM) DHE (uM)~ Time Total Free Total Free 0.25 72 ±4.4 0.38±0.04 511.5 ±99 3.3 ±0.13 0.5 122 ± 18.4 1.3 ± 0.2 357 ± 82 2.9 ± 0.05 1 141 ± 45.8 0.95 ±0.4 387 ± 22.8 1.5 ± 0.11 4 33.9± 12.7 0.19± 0.08 117.6 ±42 1.3 ±0.07 24 0 0 0.13 ±0.1 0.15 ±0.04 3.4. HMC pharmacokinetics - i.v. and i.p. When formulated in HPBCD and delivered i.v., extremely high levels of HMC were observed in the blood equating to 1 mM of drug, 15 min post administration (Figure 4). Elimination kinetics of i.v. delivered HMC were biphasic with HMC being rapidly excreted from blood at a rate of -1000 uM/hr in the first hr post administration. Assuming linear excretion, this rate slowed to 0.97 uM/hr in hours 1-4 hr post administration. When the same formulation was administered i.p., approximately 1 log less HMC was observed in plasma (131 pM by i.p. administration vs 1069 pM by i.v. administration) up to 1 hour post administration (Fig 4). Elimination kinetics by i.p. administration however, was much slower during this period (112 pM/hr) thus resulting in a serum concentration some 4.5 fold higher at 1 hr post administration (18.7 by i.p. vs 3.98 by i.v.). Conversely, in hours 1 4 post administration, elimination kinetics was faster after i.p. administration when compared to i.v. (4.6 pM/hr by i.p. vs 0.97 pM/hr by i.v.). These data confirm that HMC is highly bioavailable in its free state when administered by i.v. or i.p. routes. In conjunction with oral PK data, these data also suggest that HMC is susceptible to rapid removal by GI detoxification enzymes. Large concentrations of free HMC were observed in urine over 0.5, 1 and 4hr where collected (3.3 mM, 3.9 mM and 0.093 mM). Table 4. Comparison of the pharmacokinetic profile of HMC in serum after i.v and i.p administration of HMC formulated in 20% hydroxypropyl beta cyclodextrin at a dose of 50 mg/kg). Inset shows HMC concentrations in serum.
P:\WPDOCS\Bah\NOVOGEN\SPEC\1254345 .AUcompled-03/05/05 - 43 Serum HMC (uM) Time (hr) iv ip 0.25 1069.75 131.37 0.50 198.66 31.78 1 3.98 18.74 4 0.07 0.15 24 0.05 0.17 3.5. Pilot in vivo efficacy study - HPAC tumour bearing mice HMC when dosed daily, i.p. at 100 mg/kg significantly retarded the proliferation of HPAC tumours over the treatment period when compared to vehicle control (Figure5). When the mean terminal tumour mass was assessed a significant reduction in final tumour burden (%T/C = 62) was also noted (Figure 6). Importantly, no signs of toxicity were noted in animals dosed with HMC at 100 mg/kg daily for 15 days as determined by weight loss. Indeed animals treated with HMC appeared to thrive when compared to control (Figure 7). Organs (liver, kidney, spleen, femur, stomach and colon) were collected and submitted for histopathological assessment by Rothwell consulting. A limited serum biochemistry analysis was also conducted. These data confirm that HMC demonstrates antitumorigenic activity against HPAC tumours in vivo. 3.5.1. Histpathological examination of HMC treated groups Histopathological examination of haematoxylin and eosin-stained sections cut from formalin-fixed tissues from two series of experimental mice was made. The liver, kidney, stomach and colon were examined for evidence of toxic damage, the spleen and bone marrow for evidence of myelosuppression and the tumour for degree of necrosis. A score of 0-5 was allocated to each tumour specimen for the degree of necrosis present, a 0 score representing, no necrosis and a score of 5, total necrosis. The sections were scored 'blind' on two separate occasions and the final score given in the results is the mean of these two scores.
P:\WPDOCS\Bh\NOVOGEN\SPEC\I 254345 1.AUcomplete.dc-03/05/05 - 44 Table 5. HMC Toxicology Sample Description Necrosis Score 0-5 4/04 & 1/8 Vehicle control 0.5 4/04 & 2/8 2 4/04 & 4/8 HMC 2 4/04 & 5/8 2 4/04 & 1/11 No treatment control 0.5 3.5.1.1. Overview of results No evidence of toxicity or myelosuppression was detected in sections cut from the tissues of the drug-treated mice. However, in all the drug-treated mice there were patchy mild/moderately severe chronic inflammatory changes affecting the serosa and attached mesentery, as well as reactive changes of the mesothelial cells, in some of the tissues examined. These changes are consistent with the intra-peritoneal injection of a mildly irritant material. Significant necrosis of tumour tissue was not detected in control specimens 1/8 and 1/11. However, there was considerable necrosis in the tumour sections from the drug-treated mice. 3.5.1.2. Serum biochemistry of HMC treated mice in comparison to control Alakalines phosphatase (ALP), alanine transferase (ALT) and creatine (Cre) were assessed in HMC treated vs control animals. ALP and Cre levels were similar to control and fell within normal ranges (for rat) however, ALT levels in vehicle control and HMC treated groups were much lower than no treatment control levels. Table 6 Clinical marker (mice) Sample Group ALP ALT Cre Urea U/L U/L uM mM Control 1/11 116 713 7 6.92 Vechicle control 1/8 152 441 26 9.81 HMC treated 2/8 74 505 17 7.27 HMC threat 4/8 111 482 8 8.11 (100 mg/kg) 5/8 100 494 8 7.79 Normal ranges) 86-246 84-143 1.5-6 6.3-8* * for rat ALP: Alakaline phosphatase ALT: Alanine aminotransferase Cre: Creatinine P:\WPDOCS\Bah\NOVOGEN\SPEC\1254345 .AUompletedoc-03/05/05 - 45 3.6. HMC induced apoptosis in melanoma cells and normal fibroblasts 3.6.1. Melanoma HMC induced apoptosis in all TRAIL-sensitive and -resistant melanoma cells at concentrations down to 2ptM (~7-10% apoptosis) over 24 and 48 hrs of exposure (Table 7 and Figure 8A). At the clinically significant drug concentration of 4 piM, the incidence of apoptotic cells after 24 hr exposure to HMC rose to 25% and 39% in TRAIL sensitive (MEL-RM) and TRAIL negative (IGR3) cell lines respectively (Table 7 and Figure 8A). The incidence of HMC induced apoptosis at 4 tM after 24 hr exposure in the other cell lines was ~9%. In comparison, the incidence apoptosis in DHE- treated cells at a concentratoin of 4 tM after 24 hr exposure was 0-1%. Over 48 hr at the same concentration of HMC (4tM), the incidence of apoptosis rose to 21-42 % in all cell lines examined (Table 7 and Figure 8B). DHE was the only other agent to induce moderate levels of apoptosis after 48 hr exposure at a concentration of 4tM, but only in ME4405 (14%) and Mel-AT (15%) cell lines (Table 7 and Figure 8B). Table 7. Summary of apoptosis incidence in DHE and HMC treated melanoma cells over 24 and 48 hr. Drug Percent Apoptosis Concentration TRAIL sensitive Trail-resistant Trail +ve / (UM) Caspase 8 -ve MEL-RM ME4405 IGR3 Mel-AT DHE HMC DHE ' HMC DHE HMC DHE HMC Control 0 0 0 0 0 0 0 0 1 0 0 0 0 0 8 0 0 2 0 8 2 8 0 11 3 6 0 25 2 9 1 39 4 9 8 2 39 6 11 3 41 8 23 20 5 38 11 19 4 32 10 24 Control 0 0 0 0 0 0 0 0 1 1 1.5 1 1.5 1 1 1.5 1 2 1.5 8 3 8 1 9 5 7 4 3 22 14 42 2 21 15 25 8 10 38 40 20 8 38 43 59 20 12 30 35 18 8 38 40 35 P:\WPDOCSBahNOVOGEN\SPEC 1254345L1AUcomplet.doc-03/05/05 - 46 3.6.2. Normal fibroblasts Studies were conducted on normal fibroblasts (MRC-5) and TRAIL-sensitive melanoma cells (ME4405 and MEL-RM) using 8ptM of either DHE or HMC over 24 and 48 hr of exposure (Figure 9). These data demonstrate that HMC, and to a lesser extent DHE, induced marked levels of apoptosis in both melanoma cell lines over 24 and 48hr. Importantly, while promoting programmed cell death in malignant cells, normal fibroblasts were shown to both HMC and DHE induced apoptosis at 8 ptM drug over 24 and 48 hr of exposure. These data confirm that HMC is selectively cytotoxic to cancer cells. The isoflavan compounds of the invention exhibit a superior efficacy profile against all cancers tested when compared to DHE. While HMC is marginally more toxic than DHE in NFF and RK cells, HMC is markedly less toxic than cisplatin. HMC delivered orally in mice is less bioavailable when compared to DHE but the ratio of free:total is greater. HPBCD-formulated HMC was markedly bioavailable in its free form when delivered i.v and i.p. Significant serum concentrations of free HMC post delivery i.p. were some 18 fold above that of orally delivered HMC. It has been demonstrated that HMC, formulated in 20% HPBCD and delivered i.p., exerts a moderate antitumorigenic activity against HPAC tumours in vivo. HMC when delivered at 100 mg/kg to mice is not toxic to major organs as determined by histopathology however, in all the drug-treated mice there were patchy mild/moderately severe chronic inflammatory changes affecting the serosa and attached mesentery, as well as reactive changes of the mesothelial cells which are consistent with the intra-peritoneal injection of a mildly irritant material. HMC induced moderate-strong levels of apoptosis in TRAIL-resistant and TRAIL sensitive melanoma cells after both 24 and 48 hrs of exposure. Normal fibroblast cells were resistant to apoptosis after 48 hrs exposure DHE induces mild-moderate levels of apoptosis in TRAIL-resistant and TRAIL-sensitive melanoma cells after 48 hrs of exposure. Normal fibroblast cells were resistant to apoptosis after 48 hr exposure. The ability of both HMC and DHE to induce apoptosis in caspase negative cells suggest that an operational extrinsic programmed cell death pathway is not essential for HMC and DHE mediated apoptosis.
P:\WPDOCS\Bah\NOVOGEN\SPEC\i254345 LAUcomplete.do-03/05/05 - 47 3.7 In vitro HMC synergistic toxicity in cancer cells when combined with cisplatin, paclitaxel and gemcitabine, camptothecin, topotecan and doxorubicin 3.7.1. HMC combination with cisplatin against the MM200 melanoma cell line. HMC synergy with cisplatin was assessed either in combination over 5 days exposure or in sequence (HMC -+ cisplatin) against the MM200 melanoma cell line. It was difficult to assess for synergisitic toxicity using a change in IC50 as a measure of synergy due to HJMC toxicity as monotherapy (Table 8). 3D analysis of the data reveals that only additive toxicity was apparent using the 5-day combination protocol (Fig. 11). Evidence of synergy using the HMC-cisplatin combination was further assessed using the HMC-* cisplatin sequence (24hr exposure to each compound in sequence) against the melanoma cell line MM200. Using change in IC50 to assess for synergy it was noted that HMC at concentrations of 2 ptM markedly chemosensitised the MM200 cells to cisplatin by >1000 fold (Table 8). HMC induced chemosensitisation of MM200 cells to cisplatin was confirmed using 3D analysis of the data (Fig. 11B). These data demonstrate that HMC is able to chemosensitise cancer cells, in this case melanoma, to cisplatin. Table 8. Comparative assessment of synergy between HMC and the cisplatin against the Mel-RM melanoma cell line. Average IC50 data for each agent when assessed as a monotherapy or in combination are shown TREATMENT (IC50 uM) DRUG Change HMC Change Combined Factor 24 hr first Factor cisplatin 8.82
-
6.32
-
HMC 0.72 -- 20.64
-
HMC 1OuM L.OOE-06 HMC effect -- 1.28E-05 >10000 HMC 5uM 1.OOE-06 "- 2.71E-05 >10000 HMC 2uM 1.OOE-06 "- _1OOE-06 _>1 0000 HMC luM 0.45 " -- 8.29 -1.31 3.7.2 HMC combination with gemcitabine against the Mel-RM melanoma cells. HMC synergy with gemcitabine was assessed either in combination over 5 days exposure or in sequence (HMC -* gemcitabine) against the Mel-RM melanoma cell line. It was P;\WPDOCS\Bah\NOVOGEN\SPEC\ 12543451.AUcomplete.doc-03/05/05 - 48 difficult to assess for synergisitic toxicity using a change in IC50 as a measure of synergy due to HMC toxicity as monotherapy (Table 9). 3D analysis of the data reveals that 5-day combination protocol did not elicit synergisitic toxicity against the Mel-RM cell line. Evidence of synergy using the HMC-gemcitabine combination was further assessed using the HMC- gemcitabine sequence (24hr exposure to each compound in sequence) against the melanoma cell line Mel-RM. Using change in IC50 to assess for synergy it was noted that HMC at concentrations of 2 and 1 ptM markedly chemosensitised the Mel-RM cells. to gemcitabine by >1000 fold. HMC-induced chemosensitisation of Mel-RM cells to gemcitabine was confirmed using 3D analysis of the data. These data demonstrate that HMC is able to chemosesnsitise cancer cells to gemcitabine. Table 9. Comparative assessment of synergy between HMC and gemcitabine against the Mel-RM melanoma cell line. Average IC50 data for each agent when assessed as a monotherapy or in combination are shown. TREATMENT (IC50 uM) DRUG . Change HMC Change Combed Factor 24 hr first Factor HMC 0.51 -- 27.79 -- - HMC 1 uM 1.OOE-06 ?HMC effect -- 1.76E-03 >1000 HMC 2 uM 1.OOE-06 ?HMC effect -- 1.OOE-06 >1000 Gemcitabine 3.88E-03 -- 4.67E-03 -- - HMC 0.51 -- 27.79 _ IIMO 1 uM 1.OOE-06 ?HMC effect -- 1.OOE-06 >1000 HMC 2 uM L.OOE-06 ?HMC effect -- 3.89E-05 >100 3.7.3. HMC combination with paclitaxel against the 4405 melanoma cell line. HMC synergy with paclitaxel was assessed either in combination over 5 days exposure or in sequence (HMC -> paclitaxel) against the 4405 melanoma cell line. It was difficult to assess for synergisitic toxicity using a change in IC50 as a measure of synergy due to HMC toxicity as monotherapy (Table 10). A 30 fold reduction in IC50 was noted in the combination experiment when compared to the paclitaxel monotherapy. However, 3D analysis of the data revealed that the 5-day combination protocol did not elicit synergisitic toxicity against the 4405 cell line. Evidence of synergy using the HMC-paclitaxel combination was further assessed using the HMC-> paclitaxel sequence (24hr exposure to P:\WPDOCS\Bah\NOVOGEN\SPEC\l2543451.AUcomplete.dc-03/05/05 - 49 each compound in sequence) against the melanoma cell line 4405. Using change in IC50 to assess for synergy it was noted that HMC at concentrations of 2 piM markedly chemosensitised the 4405 cells to paclitaxel by >1000 fold (Table 10). HMC-induced chemosensitisation of MM200 cells to paclitaxel was confirmed using 3D analysis of the data. These data demonstrate that HMC is able to chemosesnsitise cancer cells to pacltaxel. Table 10. Comparative assessment of synergy between HMC and paclitaxel against the 4405 melanoma cell line. Average IC50 data for each agent when assessed as a monotherapy or in combination are shown. TREATMENT (IC50 uM) DRUG Combined Change 24 hr HMC Change Factor first Factor HMC 1 uM 0.006 1.00 -- 0.03 -4.44 HMC2uM 1.OOE-06 5964.400 -- 0.01 -1.035 Paclitaxel 1.25E-07 -- 5.84E-04 -- - HMC 1.26 -- 55.50 -- - HMC 1 uM 4.12E-09 30.36 -- 5.31E-05 11.00 HMC 2 uM 3.91E-10 ?HMC effect -- 5.48E-09 106633.75 3.7.4. HMC combination with topotecan against the MM200 melanoma cell line. HMC synergy with topotecan was assessed either in combination over 5 days exposure or in sequence (HMC -) topotecan) against the MM200 melanoma cell line. It was difficult to assess for synergisitic toxicity using a change in IC50 as a measure of synergy due to HMC toxicity as monotherapy (Table 8). 3D analysis of the data confirmed that the 5-day combination protocol did not elicit synergisitic toxicity against the MM200 cell line. Evidence of synergy using the HMC-gemcitabine combination was further assessed using the HMC-* topotecan sequence (24hr exposure to each compound in sequence) against the melanoma cell line MM200. Using change in IC50 to assess for synergy it was noted that HMC at a concentration of 2 piM markedly chemosensitised the MM200 cells to topotecan by >1000 fold (Table 11). HMC-induced chemosensitisation of MM200 cells to topotecan was confirmed using 3D analysis of the data. These data demonstrate that HMC is able to chemosesnsitise cancer cells to topotecan. From the 3D analysis the optimum combination P:\WPDOCS\Bah\NOVOGEN\SPECOI2543451.AUcomplete.dc-0 3 /05/05 -50 of HMC and topotecan against the MM200 melanoma cell line would appear to be 2 tM HMC and between 1 and 0.1 ptM topotecan. Table 11. Comparative assessment of synergy between HMC and topotecan against the MM200 melanoma cell line. Average IC50 data for for each agent when assessed as a monotherapy or in combination are shown. TREATMENT (IC50 uM) DRUG . Change HMC Change Combined Factor 24 hr first Factor HMC 1 uM 0.115 -14.145 -- 0.009 9.304 HMC 2 uM 1.OOE-06 ?HMC effect -- 7.85E-05 >1000 Topotecan 0.095 -- 2.216 -- - HMC 0.702 -- 17.952 -- - HMC I uM 0.000 ?HMC effect -- 0.044 50.656 HMC2uM .OOE-06 ?HCM effect - 1.OOE-06 >10000 3.7.5. HMC combination with camptothecin against the Mel-RM melanoma cell line. HMC synergy with doxorubicin was assessed either in combination over 5 days exposure or in sequence (HMC -> doxorubicin) against the Mel-RM melanoma cell line. It was difficult to assess for synergisitic toxicity using a change in IC50 as a measure of synergy due to HMC toxicity as monotherapy (Table 12). 3D analysis of the data confirmed that the 5-day combination protocol did not elicit synergisitic toxicity against the Mel-RM cell line, indeed evidence of antagonism was noted. Evidence of synergy using the HMC doxorubicin combination was further assessed using the HMC-> doxorubicin sequence protocol (24hr exposure to each compound in sequence) against the melanoma cell line Mel-RM. Using change in IC50 to assess for synergy it was noted that HMC at a concentration of 2 tM chemosensitised the Mel-RM cells to camptothecin by ~12 fold (Table 12). 3D analysis of the data, however, reveal a marked degree of synergy between HMC and doxorubicin against Mel-RM cells. These data demonstrate that HMC is able to chemosesnsitise cancer cells to pacltaxel. From the 3D analysis the optimum combination of HMC and camptothecin against the MM200 melanoma cell line would appear to be 2 p.M HMC and between 1 and 0.1 p.M doxorubicin.
P:\WPDOCS\Bah\NOVOGEN\SPEC\l2543451.AUcomplete.doc-03/05/05 -51 Table 12. Comparative assessment of synergy between HMC and doxorubicin against the Mel-RM melanoma cell line. Average IC50 data for each agent when assessed as a monotherapy or in combination are shown. TREATMENT (IC50 uM) DRUG . Change HMC Change Combed Factor 24 hr first Factor Doxorubicin 0.19 -- 0.100 -- - HMC 0.54 -- 50.515 -- - HMC 1 uM 0.40 -2.06 -- 0.062 1.62 HMC 2 uM 0.18 ?HMC effect -- 8.16E-03 12.22 3.8 Inhibition of TNFa in murine macrophages (RAW 264.7) by compounds 4, 6 & 7 The mouse macrophage cell line RAW 264.7 was cultured in DMEM supplemented with FCS, 2mM glutamine and 50U/ml penicillin/streptomycin. Subconfluent cells were detached from the flask by gentle scraping and 24-well plates seeded at 5 x 105 cells per well and allowed to adhere for lhr. Cells were treated with either test agent (in 0.025% DMSO) or vehicle alone, lhr prior to the addition of 50ng/ml LPS. After incubation for 16 hrs, culture media was collected and stored at -80*C for TNFa measurement using an enzyme immunometric assay (Becton Dickinson). Compound 6 and compound 7 of the present invention were tested and the results are shown in Figure 12, which indicated that the compounds tested inhibit TNFa in murine macrophages in a dose dependent manner over the concentration ranges tested. The raw data for compounds 6, 7 and additionally compound 4 is shown in Table 13 below. Table 13 Concentration Compound 6 Compound 7 Compound 4 pM 10 -48.7 -26.2 -6.1 1 -13.0 -25.4 -11.9 0.1 -10.4 -1.4 -6.3 0.001 1.0 19.2 -14.3 0.01 - -11.3 P:\WPDOCS\BahNOVOGEN\SPEC\12543451.AUpet.do-0 3 /0 5 /05 - 52 The invention has been described herein, with reference to certain preferred embodiments, in order to enable the reader to practice the invention without undue experimentation. However, a person having ordinary skill in the art will readily recognise that many of the components and parameters may be varied or modified to a certain extent without departing from the scope of the invention. Furthermore, titles, headings, or the like are provided to enhance the reader's comprehension of this document, and should not be read as limiting the scope of the present invention. The entire disclosures of all applications, patents and publications, cited herein, if any, are hereby incorporated by reference. Throughout this specification and the claims which follow, unless the context requires otherwise, the word "comprise", and variations such as "comprises" or "comprising", will be understood to imply the inclusion of a stated integer or step or group of integers or steps but not the exclusion of any other integer or step or group of integers or steps. Those skilled in the art will appreciate that the invention described herein is susceptible to variations and modifications other than those specifically described. It is to be understood that the invention includes all such variations and modifications. The invention also includes all of the steps, features, compositions and compounds referred to or indicated in this specification individually or collectively, and any and all combinations of any two or more of said steps or features. The reference to any prior art in this specification is not, and should not be taken as, an acknowledgment or any form of suggestion that that prior art forms part of the common general knowledge in the field of endeavour. Selected Reference Articles Constantinou Al, Mehta R, Husband A. 2003 Phenoxodiol, a novel isoflavone derivative, inhibits dimethylbenz[a]anthracene (DMBA)-induced mammary carcinogenesis in female Sprague-Dawley rats. Eur J Cancer. 39, 1012-8. Constantinou Al, Husband A. 2002 Phenoxodiol (2H-1-benzopyran-7-0,1,3-(4- P\WPDOCS\Bah\NOVOGEN\SPEC 254345 1. AUcompletedo-03/05/05 - 53 hydroxyphenyl)), a novel isoflavone derivative, inhibits DNA topoisomerase II by stabilizing the cleavable complex. Anticancer Res. 22, 2581-5. Gamble, JR., Xia, P., Hahn, C., Drew, J., Drogemuller, C., Carter, C., Walker, C., Brown, DM., Vadas, MA. 2003 Phenoxodiol, a derivative of plant flavanoids, shows potent anti tumour and anti-angiogenic properties. Nature Medicine. Submitted. Hersey, P and Zhang, X. D. 2001 How melanoma cells evade Trail-induced apoptosis. Nature reviews, Cancer, 1, 142-150. Kamsteeg, M., Rutherford, T., Sapi, E., Hanczaruk, B., Shahabi, S., Flick, M., Brown, D.M and Mor, G. 2003 Phenoxodiol-an isoflvone analogue- induces apoptosis in chemo resistant ovarian cancer cells. Oncogene, ;22, 2611-20. O'Dwyer PJ, Moyer JD, Suffness M, Harrison SD Jr, Cysyk R, Hamilton TC, Plowman J. 1994 Antitumor activity and biochemical effects of aphidicolin glycinate (NSC 303812) alone and in combination with cisplatin in vivo. Cancer Res. 54, 724-9 Todorov PT, Field WN, Tisdale MJ 1999 Role of a proteolysis-inducing factor (PIF) in cachexia induced by a human melanoma (G361). Br J Cancer. 80,1734-7. Bellisarii, F. L., S. Gallina, et al. (2001). "Tumor necrosis factor-alpha and cardiovascular diseases." Italian Heart Journal: Official Journal of the Italian Federation of Cardiology. 2(6): 408-17. Szlosarek, P. W. and F. R. Balkwill (2003). "Tumour necrosis factor alpha: a potential target for the therapy of solid tumours." Lancet Oncol 4(9): 565-73. Nakata E, Hunter N, Mason K, Fan Z, Ang KK, Milas L. 2004 C225 antiepidermal growth factor receptor antibody enhances the efficacy of docetaxel chemoradiotherapy. Int J Radiat Oncol Biol Phys. 59(4):1163-73.

Claims (17)

1. A compound of the general formula (I): Rx R10 0 (I) R3. 0 R2 R5 R6 R4 wherein RI is hydrogen, R 2 and R 3 are independently hydrogen, hydroxy, alkoxy, alkyl, cycloalkyl, halo or OC(O)R 7 , with the exception that R 2 and R 3 are not both hydrogen, R 4 , R 5 and R 6 are independently hydrogen, hydroxy, alkoxy, alkyl, cycloalkyl, acyl, NH 2 , NHCI-C 4 alkyl or N(CI-C 4 alkyl) 2 , OC(O)R 7 or OR 8 , R 7 is hydrogen, alkyl, cycloalkyl, aryl, arylalkyl or amino, R 8 is phenyl or benzyl, and Rx is hydrogen, hydroxy, alkoxy, alkyl, cycloalkyl or halo, or a pharmaceutically acceptable salt thereof.
2. A compound of formula (I) according to claim I of the general formula (I-X): (I-X) I-R3 R2 R5 R6 R4 wherein C:\NRPonbIl\DCCMD134150213_ .DOC-22A)22012 - 55 R, is hydrogen, R 2 and R 3 are independently hydrogen, hydroxy, alkoxy, alkyl, cycloalkyl, halo or OC(O)R 7 , with the exception that R 2 and R 3 are not both hydrogen, R 4 , R 5 and R 6 are independently hydrogen, hydroxy, alkoxy, alkyl, cycloalkyl, acyl or OC(O)R 7 , and R 7 is hydrogen, alkyl, cycloalkyl, aryl, arylalkyl or amino, or a pharmaceutically acceptable salt thereof.
3. A compound of formula (I) according to claim 1 wherein the compound is selected from: 3-(4-hydroxyphenyl)-4-(4-methoxyphenyl)chroman-7-ol; 3-(4-hydroxyphenyl)-4-phenylchroman-7-ol; 3-(4-hydroxyphenyl)-4-(3-methoxyphenyl)chroman-7-ol; 3-(3,4-dimethoxyphenyl)-4-(4-methoxyphenyl)chroman-7-ol; 3-(4-hydroxyphenyl)-4-(4-methylphenyl)chroman-7-ol; 3-(4-hydroxyphenyl)-4-(2,6-dimethoxy-4-hydroxyphenyl)chroman-7-ol; 3-(4-hydroxyphenyl)-4-(2-hydroxyphenyl)chroman-7-ol; 3-(3-hydroxyphenyl)-4-(3-methoxyphenyl)chroman-7-ol; 3 -(4-hydroxyphenyl)-4-(4-hydroxyphenyl)chroman-7-ol; 3-(4-bromophenyl)-4-(4-methoxyphenyl)chroman-7-ol; 3 -(4-hydroxyphenyl)-4-(3 -methoxyphenyl)chroman-7-ol; 3-(4-hydroxyphenyl)-4-(3-aminophenyl)chroman-7-ol; and 3-(4-hydroxyphenyl)-4-(4-phenoxyphenyl)chroman-7-ol.
4. A compound of formula (I) or (I-X) according to claim 1 or claim 2, wherein the compound is: 3-(4-hydroxyphenyl)-4-(4-methoxyphenyl)chroman-7-ol; or 3-(4-hydroxyphenyl)-4-(4-hydroxyphenyl)chroman-7-ol.
5. A process for the preparation of a compound of formula (I-X) according to claim 2 comprising the step of reacting the 4-keto group of a compound of the formula (II): CANRPortbl\DCC\MDT151213_ DOC-22 12/20 12 -56 R10 O (II) 0 / , R2 wherein R 1 , is alkyl or Si(RA) 3 , R 2 and R 3 are independently hydrogen, alkoxy, halo or OSi(RA)3, with the exception that R 2 and R 3 are not both hydrogen, and RA is independently alkyl or aryl, with an arylating agent W~M*, wherein W~ is a benzene ring optionally substituted with the groups R 4 , R 5 and R 6 , wherein R 4 , R 5 , R 6 and R 7 are as defined in claim 2, and M* is one or more counter ions, to form the intermediate tertiary alcohol (III): R10 O (III) HO - R3 R2 or a salt thereof and which is dehydrated to form a compound of formula (IV): (IV) -R3 R2 which is subsequently hydrogenated and deprotected to form a compound of formula (I-X).
6. Use of one or more compounds of formula (I) or (I-X) as defined in any one of C:RNorb\DCC\MDT\41502 _ .DOC-22t212012 - 57 claims 1 to 4 in the treatment of cancer or a tumour mass.
7. A method for the treatment or amelioration of cancer or a tumour mass, which comprises administering to a subject one or more compounds of the formula (I) or (I-X) as defined in any one of claims I to 4 or a pharmaceutically acceptable salt or derivative thereof, optionally in association with a carrier and/or excipient.
8. Use of one or more compounds of formula (I) or (I-X) as defined in any one of claims 1 to 4 or a pharmaceutically acceptable salt or derivative thereof, in the manufacture of a medicament for the treatment of cancer or a tumour mass.
9. An agent for the treatment, prophylaxis or amelioration of cancer or a tumour mass, which agent comprises one or more compounds of formula (I) or (I-X) as defined in any one of claims I to 4, or a pharmaceutically acceptable salt or derivative thereof.
10. A pharmaceutical composition which comprises one or more compounds of formula (I) or (I-X) as defined in any one of claims 1 to 4 or a pharmaceutically acceptable salt thereof, in association with one or more pharmaceutical carriers, excipients, auxiliaries and/or diluents.
11. A drink or food-stuff, which contains one or more compounds of formula (I) or (I X) as defined in any one of claims I to 4 or a pharmaceutically acceptable salt thereof.
12. A compound of formula (I) or (I-X) as defined in claim I or claim 2, or a pharmaceutically acceptable salt thereof, substantially as hereinbefore described with reference to the Examples and/or accompanying drawings.
13. The method of claim 7, wherein the compound is administered in combination with radiotherapy or chemotherapy. C :NRPortbI\DCCVAfl h I50)213_I.DOC-22A2/212 - 58
14. The method of claim 13, wherein the compound radiosensitises or chemosensitises the cancer or tumour mass.
15. The method of claim 14, wherein the compound chemosensitises the cancer or tumour cell, and wherein the subject is undergoing chemotherapy with cisplatin, dehydroequol or taxol.
16. The method of claim 14, wherein the cancer or tumour mass is of epithelial origin, of mesenchymal origin or of neural origin.
17. The method of claim 16, wherein the cancer is prostate, ovarian, cervical, breast, gall-bladder, pancreatic, colorectal, renal, non-small cell lung, melanoma, mesothelioma, sarcoma or glioma.
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AU2005201855A AU2005201855B2 (en) 2004-09-21 2005-05-03 Chroman derived compounds and formulations thereof for use in therapy
MX2007003215A MX2007003215A (en) 2004-09-21 2005-09-21 Chroman derivatives, medicaments and use in therapy.
EP05779877A EP1794141B1 (en) 2004-09-21 2005-09-21 Substituted chroman derivatives, medicaments and use in therapy
EP20110175917 EP2407462B1 (en) 2004-09-21 2005-09-21 Substituted chroman derivatives, medicaments and use in therapy
ES11175917.1T ES2516067T3 (en) 2004-09-21 2005-09-21 Substituted Chroman Derivatives, Medicines and Therapy
ES05779877T ES2377073T3 (en) 2004-09-21 2005-09-21 Substituted Chroman Derivatives, Medicines and Therapy Use
PCT/AU2005/001436 WO2006032086A1 (en) 2004-09-21 2005-09-21 Chroman derivatives, medicaments and use in therapy
PCT/AU2005/001435 WO2006032085A1 (en) 2004-09-21 2005-09-21 Substituted chroman derivatives, medicaments and use in therapy
CN2005800380156A CN101094844B (en) 2004-09-21 2005-09-21 Chroman derivatives, medicaments and use in therapy
HK07113859.6A HK1108685B (en) 2004-09-21 2005-09-21 Substituted chroman derivatives, medicaments and use in therapy
ES11180383.9T ES2586847T3 (en) 2004-09-21 2005-09-21 Chroman derivatives, medications and therapeutic use
AT05779877T ATE532777T1 (en) 2004-09-21 2005-09-21 SUBSTITUTED CHROMEDER DERIVATIVES, MEDICATIONS AND APPLICATIONS IN THERAPY
NZ553834A NZ553834A (en) 2004-09-21 2005-09-21 7-hydroxy-3,4-diphenyl-chroman and chromene derivatives
HK08101549.6A HK1112617B (en) 2004-09-21 2005-09-21 Chroman derivatives, medicaments and use in therapy
EP05787045.3A EP1809618B1 (en) 2004-09-21 2005-09-21 Chroman derivatives, medicaments and use in therapy
EP11180383.9A EP2436680B1 (en) 2004-09-21 2005-09-21 Chroman derivatives, medicaments and use in therapy
MX2007003216A MX2007003216A (en) 2004-09-21 2005-09-21 Substituted chroman derivatives, medicaments and use in therapy.
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CA2581316A CA2581316C (en) 2004-09-21 2005-09-21 Substituted chroman derivatives, medicaments and use in therapy
NZ553835A NZ553835A (en) 2004-09-21 2005-09-21 7-hydroxy-3,4-diphenyl-chroman derivatives
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CN2005800381178A CN101056868B (en) 2004-09-21 2005-09-21 Substituted chroman derivatives, medicaments and use in therapy
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IL182034A IL182034A (en) 2004-09-21 2007-03-20 Substituted chroman derivatives, a process for their preparation, pharmaceutical compositions comprising them and their use in the manufacture of medicaments
NO20071578A NO20071578L (en) 2004-09-21 2007-03-26 Chromium derivatives, drugs and use in therapy
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