IE83638B1 - Method of treatment of androgen-related diseases - Google Patents

Abstract

Abstracts of the 7th International Congress of Endocrinology, Excerpta Medica (1984) at page 98 disclose that treatment of prostate cancer patients with LHRH agonists alone causes a transient increase in serum androgen levels lasting for 5 to 15 days before castra- tion levels are reached. While F. Labrie et al. recommend that orchiec— tomy, estrogen and LHRH agonists alone should not be further used for treatment of prostate cancer in the absence of a pure antiandrogen, there still is a need for a method of treatment of prostate cancer that effects more complete androgen blockage at the start as well as during the full period of treatment.

Description

BACKGROUND OF THE INVENTION This invention relates to a method of treatment of androgen-related diseases such as prostate cancer in warm-blooded male animals (including humans) in need of such treatment, and in particular, to a combination therapy comprising administering an antiandrogen in association with an inhibitor of sex steroid biosynthesis to such animals. The invention also includes pharmaceutical compositions and kits useful for such treatment.

Androgen-dependent diseases include diseases whose onset, maintenance or . progress is, at least in part, dependent upon biological activities indu- ced by androgens (e.q. testosterone and dihydrotestosterone). to UI While various investigators have been studying hormone-dependent prostate cancer, none have proposed the combination therapy of this invention.

A.V. Schally et al., Cancer Treatment Reports, 68 (No. 1) 281-289 (1984), summarize the results of animal and clinical studies on growth inhibition of hormone-dependent mammary and prostate tumors by use of analogues of luteinizing hormone-releasing hormones, the so-called LHRH agonists and suggest that LHRH analogs and/or antagonists may have poten- tial for treating breast cancer.

T.W. Redding and A.V. Schally, Proc. Natl Acad. Sci. UA 80, 1459- 1462 (1983), relates to inhibition of prostate tumor growth in rats by chronic use of an LHRH agonist, [D-Trp‘]LHRH.

U.S. Patent Number 4,329,364 relates to use of the antiandrogen, 4'- nitro-3'trifluoromethyl isobutyranilide for treatment of prostatic cancer. _U.S. Patent Number 4,472,382 relates to treatment of prostate adeno- carcinoma, benign prostate hypertrophy and hormone-dependent mammary tumors may with various LHRH agonists and treatment of prostate adenocar- cinema and benign hypertrophy by use of various LHRH agonists and an antiandrogen.

U.S. Patent Number 4,559,695 (Labrie) relates to treatment of prostate cancer in animals whose testicular hormonal secretions are blocked. The method of treatment includes administering an antiandrogen such as flutamide as an inhibitor of sex steroid biosynthesis such as aminoglutethimide and/or ketoconazole.

Some clinical improvement in men with prostate cancer by use of the two LHRH agonists, Buserelin and Leuprolide, is also reported by N. Faure et al. at pages 337-350 and by R.J. Santen et al. at pages 351-364, res- pectively, LHRH and its Analogues - A new Class of Contraceptive and the- rapeutic Agents (B.H. Vickery and J.J. Nestor, Jr., and E.S.E. Hafez, eds), Lancaster, MTP Press, (1984).

R. Santen et al., The Journal of Steroid Biochemistry, volume 20, no 6B, at page 1375 (1984), relates that the use of ketoconazole in combina- tion vith chronic administration of Leuprolide in rodents decreased basal and Leuprolide-stimulated testosterone levels.

One of Applicant's Co-pending U.S. Patent Applications Serial Number /321,926 filed March 10, 1989, relates to a combination therapy for , treatment of estrogen-related diseases by inhibiting ovarian hormonal secretions and administering an antiestrogen in combination with at least one of several enumerated activity blockers, sex steroid formation inhi- bitors and the like.

D. Kerle et al., The Journal of Steroid Biochemistry, volume 20, no. 6B, at page 1395 (1984) relates to the combined use of a LHRH analogue and ketoconazole producing objective responses in some prostate cancer patients who have relapsed or failed to respond to treatment with a LHRH analogue alone.

F. Labrie et al., The Prostate, 4, 579-594 (1983). disclose that use of a combination therapy of an LHRH agonist (Buserelin) and an antiandro- gen (Anandron) to treat advanced prostate cancer in previously untreated patients effects simultaneous elimination of androgens of both testicular and adrenal origin.

F. Labrie et al., J. Steroid Biochem., 19, 999-1007 (1983), disclose the treatment of prostate cancer by the combined administration of an LHRH agonist and an antiandrogen. Labrie et al. disclose animal and cli- nical data in support of the proposition that the combined LHRH/antian- drogen treatment neutralizes the stimulatory influence of all androgens on the development and growth of androgen-dependent prostatic cancer.

F. Labrie et al., Abstracts of the 7th International Congress of Endocrinology, Excerpta Medica (1984) at page 98 disclose that treatment of prostate cancer patients with LHRH agonists alone causes a transient increase in serum androgen levels lasting for 5 to 15 days before castra- tion levels are reached. While F. Labrie et al. recommend that orchiec— tomy, estrogen and LHRH agonists alone should not be further used for treatment of prostate cancer in the absence of a pure antiandrogen, there still is a need for a method of treatment of prostate cancer that effects more complete androgen blockage at the start as well as during the full period of treatment.

There are many data indicating that estrogens have a stimulatory effect on prostatic growth (Lee et al., 1981; J. Androl. 2: 293-299; Belis et al., 1983; J. Androl. 4: 144-149; Walsh and Wilson, 1976; J.

Clin. Invest. 57: -1097; De Klerk et al., 1985; Prostate 7, 1-12‘ Habesucht et al., 1987; Prostate 11: 313-326). Estrogen: have also been found to enhance the growth-promoting effect of androgens (Farnsworth, ; Invest. Urol. 6: 423-427; Groom et al., 1971; Biochem. J. 122: -126; Lee et al., 1973; Steroids 22: 677-683).

Estrogen receptors have been demonstrated in human normal, hyper- plastic and cancer prostatic tissue (Hobbs et al., 1989: 84th Endocrine Soc., Meeting, abst. No. 1410; Hobbs et al., 1983; J. Steroid Proc.

Biochem. 19, 1279-1290; Wagner et al., 1975; Acta Endocrinol. (Kbh). suppl. 193, 52; and also in laboratory animal prostatic tissue (Swaneck et al., 1982; Biochem. Biophys. Res. Commun. 105: 1441-1447).

Moreover, androgen receptor levels were found to be elevated in prostatic tissue of patients treated with estrogen, thus indicating a stimulatory‘ effect of estrogen on the level of androgen receptors in prostatic tissue (Mobbs et al., 1983; J. Ster. Biochem. 19, 1279-1290).

A similar stimulatory effect of estrogen has been observed in the dog prostate (Moore et al., 1979; J. Clin. Invest. 63, 351-357).

In the prostate as well as in many other tissues, testosterone is irreversibly converted by So-reductase into the more potent androgen di- hydrotestosterone (Bruchovsky and Wilson, J. Biol. Chem. 243: 2012-2021, 1968; Wilson, Handbook of Physiology 5 (section 7), pp. 491-508, 1975).

Inhibitors of 5a-reductase have been found to inhibit prostatic growth (Brooks et al., Endocrinology 109: 830, 1981; Brooks et al., Proc. Soc.

Exp. Biol. Med. 169: 67, 1982; Brooks et al., Prostate 3: 35, 1982; Wenderoth et al., Endocrinology 113, 569-573, 1983; McConnell et al., J.

Urol. 141: 239A, 1989): Stoner, E., Lecture on the role of Sc-reductase inhibitor in benign prostatic hypertrophy, 84th AUA Annual Meeting, Dallas, May 8th, 1989.

The inhibitory effect of the 5a-reductase inhibitor Merck L. 652,931 on prostatic and seminal vesicle development in the prepubertal rat was described in Proc. 71st Annual Meeting of Endocrine Society, abst. #1165, p. 314, 1989. The inhibitory effect of MKr906 on dihydrotestosterone formation in men has been described in men by Gormley et al., in Proc. 71st Annual Meeting of Endocrine Society, abst. #1225, p. 329, 1989; Imperato-McGinley et al., in Proc. 71st Annual Meeting of Endocrine Society, abst. #1639, p. 432, 1989; Seller and Franson, in Proc. 71st Annual Meeting of Endocr. Soc., abst. #1640, p. 432, 1989, and Tenover et al., in Proc. 71st Annual Meeting of Endocr. Soc., abst. #583, p. 169, 1989. The activity of the Sn-reductase inhibitors N,N-diethylmethy1 oxoaza-5o-androstane-17B-carboxamide (4-MA) and 6-methylenepreg- nene-3,20-dione (LY207320) has been described by Toomey et al., Proc. st Annual Meeting of Endocr. Soc., abst. #1226, p. 329, 1989.

SUMMARY OF THE INVENTION According to the invention there is provided the use of an antiandrogen in the preparation of a medicament for use, together with an inhibitor of So.-reductase activity, in the treatment of prostate cancer; the use of an antiandrogen in the preparation of a medicament for use, together with an inhibitor of a 17|3 HSD, in the treatment of prostate cancer; or the -use of an antiandrogen in the preparation of a medicament for use, together withan inhibitor of 35-hydroxysteroid dehydrogenase, in the treatment of prostate cancer. Thus, the invention also provides the use of an inhibitor of 5a- reductase activity in the preparation of a medicament for use, together with an antiandrogen, in the treatment of prostate cancer; the use of an inhibitor of a 1713-HSD, in the preparation of amedicament for use, together with an antiandrogen, in the treatment of prostate cancer, or the use of an antiandrogen in the preparation of a medicament for use, together with an inhibitor of 3B-hydrolxysteroid dehydrogenase, in the treatment of prostate cancer.

According to the invention there is also provided such a use in which the medicament is foruse together also with the inhibition of testicular hormonal secretion by surgical castration or by administration of a Ll-IRH agonist or antagonist and such a use in which the medicament for use together also with a compound selected from a 50:- reductase inhibitor, a 1713-hydroxysteroid dehydrogenase inhibitor, an antiestrogen, an ‘ LHRH agonist or antagonist, or with surgical castration, where such compound or castration is not already indicated The foregoing active ingredients may also be mixed in any of the foregoing combinations to form pharmaceutical compositions (with or without diluent or carrier) which, when administered, provide simultaneous adnilinistr-ation of a combination of active ingredients resulting in the combination therapy of the invention. Preferably, when LHRH antagonist or agonist is used, it is administered parenterally. For this reason, it may be administered separately in instances where the other active ingredients are formulated for oral ingestion.

A combination therapy for prostate cancer includes administering active ingredients effective to inhibit a variety of different mechanisms which may, directly or indirectly, lead to prostatic cancer growth. Desirably, the inhibition of biological activity which leads to prostatic cancer growth proceeds selectively, without I-H substantially inhibiting other desirable biological activity. Side effects of the treatment are therefore minimized.

Activation of prostatic androgen receptors stimulates growth of prostatic cancer cells. Growth may be inhibited by blocking these recep- tors with antiandrogens as explained herein. Growth may also be inhibited by reducing the concentration of androgens available to activate the receptors by administering at least one sex steroid synthesis inhibitor.

An inhibitor of So-reductase catalyzes conversion of testosterone to dihydrotestosterone (DHT). This is a particularly preferred sex steroid synthesis inhibitor because it selectively reduces DHT levels without reducing testosterone levels. DHT stimulates prostatic cancer growth to a much greater extent than does testosterone. Also absence of DHT forecloses fewer desirable biological functions than does absence of testosterone. For many patients, blocking of testosterone production is also appropriate.

. It is believed that estrogen: may also increase prostatic cancer growth. Without intending to be bound by theory, estrogens appear to at least be involved in increasing the number of androgen receptors, and may stimulate prostatic cancer growth directly by binding estrogen receptors. Regardless of the mechanism by which estrogens contribute to prostatic cancer growth, it has now been found that a combination therapy which includes inhibition of estrogen activity can enhance effectiveness of treatment without inhibiting desirable biological functions which, in males, are largely independent of estrogen.

There is shown in Figure l a schematic representation of the site(s) of action of various drugs, enzymes and hormones. The following abbre- viations are used: ER: estrogen receptor; AR: androgen receptor; DHEA: dehydroepiandrosterone; A5-diol: androstene-38,178-diol; A‘-dione: androstenedione; DHT: dihydrotestosterone; Anti-A: antiandrogen; Anti-E: antiestrogen; ARO: aromatase; 3B-HSD: 3B-hydroxysteroid dehydrogenase, A5-A‘ isomerase; 17B-HSD: 17B-hydroxysteroid dehydrogenase; l: antiandro- gen; 2: inhibitor of So-reductase activity; 3: inhibitor of l7B-hydro- xysteroid dehydrogenase activity; 4: antiestrogen; 5: inhibitor of aroma- tase activity; 6: inhibitor of 3B-HSD activity.

Referring to Figure l, + means increase in androgen receptor levels.

As may be seen from Figure 1, stimulation of the androgen receptor is shown to stimulate prostatic cancer growth, and is therefore to be prevented. In addition, stimulation of the estrogen receptor leads to increased levels of androgen receptors and thus may, in addition, exert direct stimulatory effects on prostatic cancer growth. The action of estrogens is therefore to be prevented. Blockers of sex steroid formation from DHEA and A‘-dione in peripheral tissues does not cause inhibition of adrenal glucocorticoid formation. For example, cortisol and aldosterone production is not inhibited and significant complications which could result from their inhibition are avoided. The desired inhibition of sex steroid formation is thus aimed selectively at androgens and estrogens.

A method of inhibiting activation of the androgen receptor is treat- ment with an effective antiandrogen compound having an affinity for the receptor site such that it binds to the receptor site and prevents andro- gens from binding and activating the site. It is important to select antiandrogens which tend to be pure antagonists and which have no agonis- tic activity. Otherwise, the antiandrogen which blocks the receptor site from androgens, may itself activate the site. Preferred antiandrogens are discussed in detail below. Because it is extremely difficult to block all receptor sites, it is desirable to simultaneously decrease the concentration of androgens available to activate androgen receptors in the prostatic cancer tissue. Hence, it is desirable to inhibit secretion of androgens by the testis. This may be accomplished by a variety of known techniques including but not limited to surgical orchiectomy or by administering LHRH agonists or antagonists. For example, LHRH analogues act in a manner effective to stop the production of bioactive luteinizing hormone, the hormone necessary to cause the testis to produce and secrete androgens and other hormones which may be converted to androgens in peri- pheral tissues. For some patients, it may be unnecessary to inhibit tes- ticular hormonal secretions where sufficiently potent antiandrogens and sex steroid biosynthesis inhibitors are administered.

As may be seen from the scheme of Figure l, a number of hormones (especially DHEA and A‘-dione) released by the adrenals may be converted by a variety of biological pathways into androgens and estrogens in peri- pheral tissues. The most potent androgen produced is DHT. fore highly desirable to include an inhibitor of Sc-reductase which pre- It is there- vents the conversion of testosterone into the more potent androgen DHT.

In peripheral tissues, in addition to DHT, the precursors DHEA and A‘-dione can be converted into the estrogens A5-diol and estradiol. It is desirable to have an inhibitor of 175-hydroxysteroid dehydrogenase which prevents the formation of testosterone as well as of A5-diol and estra- diol. In addition, since A‘-androstenedione can be converted into estrone and then to estradiol, it may be useful to block the activity of aromata- se, the enzyme responsible for such conversion. Other sex steroid for- mation inhibitors, such as inhibitors of 3B-HSD can also be used. How- ever, as mentioned earlier, when 3B-HSD is blocked in peripheral tissues, it is also likely that a similar inhibition will take place in the adre- nals, thus leading to low secretion of glucocorticoids and mineralocorti- coids. When such compounds are used, essential glucocorticoids and some- times mineralocorticoids should be added back as part of the therapy.

Estrogens, at physiological concentrations, are known to stimulate the growth of the human prostatic cancer cell line LNCaP. This effect of estrogen may be inhibitedjhowever, by antiestrogenic compounds described herein.

In certain embodiments, the antiandrogen utilized in the present invention may be represented by the general formula: . ",1, "RH-B-Rzlxc-D wherein the dotted lines represent optional double bonds; wherein R1° is hydrogen or lower alkyl, R13 is absent, hydrogen or methyl in B position, R17 is selected from the group consisting of hydrogen, hydroxyl, lower alkanoyloxy, lower alkyl, lower alkenyl, lower alkynyl, halo(lower)alky1, halo(1ower)alkenyl, halo(lower)alkynyl and fluoro- substituted aromatic ring, and a moiety which, together with R17 forms . C) III \u"" R17(B) is selected from the group consisting of hydroxyl, (C1-C,°) alkanoyloxy, (C,-C,)alkenoyloxy, (C3—C,)alkynoyloxy, aroyloxy, alkenoy1o- xy, cycloalkenyloxy, l-alkyloxy-alkyloxy, 1-alkyloxycycloalkyloxy, alkyl- silyloxy, carboxyl, alkanoyl and a moiety which together with R1’(a) forms (3 III / \\\"" Antiandrogens useful in the combination therapy of the invention also include but are not limited to flutamide (available from Schering-Plough Corp., Kenilworth, New Jersey, under trade name EULEXIN), Nilutamide (available from Roussel of Paris, France, under trade name ANANDRON), cyproterone acetate (available from Schering AG, Berlin under trade name ANDROCUR), Casodex available from ICI Pharmaceuticals, Macclesfield, England. Preferably, the antiandrogen has, as part of its 'molecular structure, a substituted or unsubstituted androgenic nucleus, and as another part of its molecular structure, the side-chain -R‘[-B-R1-]x L—G as defined above. Numerous syntheses of the preferred compounds set forth in the U.S. patent application of Labrie and Mérand entitled "Androgen Derivatives for use in the inhibition of sex steroid activity" which is being executed on even date herewith, the entire disclosure of which is hereby incorporated by reference as though fully set forth herein. A preferred antiandrogen is EM 101 OH ca, 0 ,coN: CAH9 (x = 10) which may be synthesized as set forth below.

Example 1 Synthesis of H-butyl, N-methyl-11—(17'fl-hydray-4'-androsten-3'-on-7'a- yl) undecanamide (EM 101) (5, x=10) (Scheme 1) B-acetay-7a-(1l'-hydroxy udecanyl)-4—androstenone (2) Under argon atmosphere, in a flame dried apparatus with nmgnetic stirrer, a solution of ll-bromo undecanol tetrahydropyranyl ether (25 g, _ 74 mmol) in anhydrous THE (150 ml) was added dropwise to iodine-activated magnesium (1.9 g).The mixture was kept at room temperature overnight and then was cooled to -30°C and anhydrous cuprous chloride (0.3 g) was added quickly. After 45 min of strirring at this temperature, commercial 4,6- androstadienolone acetate (1) (10 g, 30.5 mmol) in anhydrous THE (100 ml) was added dropwise during 4 h. After 35 min, acetic acid (6 ml) and water (100 ml) was added. The mixture was allowed to reach room temperature and was stirred overnight. Afterwards, the organic com- pound was extracted with ether (3X). The organic layers were washed with water, dried on magnesium sulfate and evaporated. The residue was dissol- ved in acetic acid (35 ml) and water (100 ml) and kept 48 h at room tem- perature. And then, the organic compounds were extracted with ether (3X).

The organic layers were washed with saturated sodium bicarbonate solution and water, dried on magnesium sulfate and evaporated. The product was purified by Silica gel dry column chromatography (Kieselgel, 6OF254, Merk, 0.063- 0.200 mm, 150 g). Elution with a mixture of methylene chlo- ride and ethyl acetate (20:l v/v) gave 17B-acetoxy-7a-(ll'-hydroxy-unde- canyl)androsten-3—one (2a, 1.46 g, 2.8 mol, 9.2%) as a C°1°r1e53 oil; IR vmax neat 3450, 1740, 1685, 1620 and 1245 cm'1; NHR 0.84 (5. 3H.

'-CH3), 1.21 (s, 3H, 19'-CH3), 2.05 (s,3H, OCOCH3), 3.61 (t. 2H.

J=6.59 Hz, H-C.1'), 4.61 (t, 1H, J=7.69 Hz, H-C.17) and 5.73 (s, 1H, H—C . 1+) and l7B-acetoxy-7B- (11 ’-hydroxy undecanyl) -1+-androstenone (2b, 0.9 g, 1.7 mmol, 5.6%) as a colorless oil. - ( 17 ' B-acetoxy-19 ' —androsten-3 ' -on-7 ' a—y1) undecanoic acid (3) To 17B-acetoxy-7a-(11'-hydroxy undecanyl) -l+—androsten-3—one (Za, 800 mg, 1.6 mmol) dissolved in acetone (50 ml) and cooled to 0°C was added under stirring during 5 min, a solution of Jones‘ reagent (8N chromic acid solution) (0.283 ml). After 15 min, isopropanol (0.5 ml) was added followed by water and the mixture was extracted with ethyl acetate (3X). The organic layers were washed with brine, dried on magnesium sulfate and evaporated to dryness under reduced pressure. The crude -(17'B-acetoxy-4'-androsten-3'-on-7'a-yl) undecanoic acid (3) (740 mg) was used in the next step without purification.

N—butyl, H-methyl(17'B-acetoxy-4'-androstan-3'-on-7'6-yl) tmdecanr mide (41) To a solution of the above undecanoic acid derivative 3 (390 mg, 0.78 mmol) in anhydrous methylene chloride (8 ml) cooled at —10°C was added, under stirring, triisobutylamine (2100 1.11) and isobutylchlorofor- mate (140 pl). After 30 min, N-methylbutylamine (1.8 ml) was added and the mixture was stirred at room temperature for 1 h. Methylene chloride was added. The organic: solution was washed with 1N hydrochloric acid, water, saturated sodium bicarbonate solution and finally with water. dried on magnesium sulfate and evaporated to dryness. The residue was chromatographed on silica gel (Kieselgel, 60F2S4, Merck, 0.063-0.200 m, g). Elution with a mixture of diethyl ether and methylene chloride (1:20, v/v) gave N—buty1, N-methyl—11-(17'B-acetoxy-4'-androsten-3'—on- 7'a~yl) undecanamide # (230 mg, 0.39 mol, 46% for the alcohol ( 2a )) as a colorless oil; IR vmax neat 1740, 1680, 1640 and 1240 N-CH3), 3.26 and 3.36 (Zt, 2H, J=7.86 Hz, N-CH C H ), 4.61 (t, 1H, J=8.42 -137 Hz, H-C.l7') and 5.72 (s, 1H, H-C.4').

Nebutyl, H-methyl-ll-(l7'B-hydroxy~4'—androsten-3'—on—7'a-yl) udec- anamide (5) (E! 101) The above acetoxy amide 4 (170 mg, 0.29 mmol) was dissolved in methanol (20 ml) and 6% potassium carbonate (2 ml) and heated at 65°C for 200~min. After cooling, acetic acid (1 ml) and water (150 ml) were added and the mixture was extracted with ethyl acetate (3X). The organic layers were washed with water, dried on nmgnesium sulfate and evaporated to dryness. The residue was purified by Silica gel dry column chromatography (Kieselgel, 60F254, Merk, 0.063-0.200 mm, 20 g). Elution with a mixture of diethyl ether and methylene chloride (1:9, v/V) gave N-butyl-N-methyl- 11-(17'B-hydroxy-4'-androsten—3'-on-7'a-yl) undecanamide (EM 101, 94 mg, 0.17 mmol, 58%) as a colorless oil; IR umax (neat) 3400, 1670 and 1640 cm‘1; mm 0.80 (s, 3H, 18'-CH3), 0.95 (t,3H, J=6.75 Hz, N-(cH,),C_H_,). 1.21 (s, 3H, 19'-CH3), 2.91 and 2.97 (25, 3H, N-CH3), 3.25 and 3.35 (Zt.

OAC 0:5 : OAC CIO3 ‘ 1) C1COOIBu.NGBu)3 Acetone O "'4 2H 2 CH3NHC4H9 O KQCO3 CH3OH EM 101 CH ,c»« 0 ’(CH2),CON\ (x = 10) SCHEME I OAc Cucl. IHF 2’A°0" o (CH¢)x+1OH 78+! b 7a—H . / CH 3 "’(CH2)xCON\ C4!-‘<2 C41 Sex steroid formation inhibitors useful in the combination therapy of the invention include but are not limited to inhibitors of 5a-reducta— se activity, inhibitors of 17B-hydroxysteroid dehydrogenase activity, inhibitors of 3B-hydroxysteroid dehydrogenase activity and inhibitors of aromatase activity.

A typically suitable 5a-reductase inhibitor is MK-906, a product of Merck, Sharp & Dohme (Hc Connell et al., J. Urol. 141: 239A, 1989).

Another inhibitor of 5a-reductase is 17B-N,N-diethylcarbamoylmethyl aza-5c-androstanone (4-MA) (Brooks et al., Endocrinology 109: 830, 1981; Liang et al., Endocrinology 112: 1460, 1983). Other 4-azasteroids acting as 5a-reductase inhibitors can be formed in Liang et al., J. Biol. chem. 259: 734-739, 1984; and in Brooks et al., Steroids 47: 1-19, 1986, 6-methylenepregnene-3,20-dione has also been described as Sc-reductase inhibitor (Petrov et al., J. Endocrinol. 95: 311-313, 1982). Similar properties have been described for 4-methyloxoaza-5a-pregnane-30(s) carboxylate (Kadohama et al., J. Natl. Cancer Inst. 74: 475-486, 1985).

Trilostane and epostane have been described as inhibitors of 3B-hy- droxysteroid dehydrogenase activity (Ernshaw et al., Clin. Endocrinol. 21, 13-21, 1984; Robinson et al., J. Steroid Biochem. 21, 601-605, 1984; Lambert et al., Ann. Clin. Biochem. 23, 225-229, 1986; Potts et al., Ste- roids 32, 257-267, 1978) and have been successfully used for the treat- ment of breast cancer in combination with corticosteroids (Beardwell et al., Cancer Chemother. Pharmacol. 10: 158-160, 1983; Williams et al., Cancer Treat. Rep. 71, 1197-1201, 1987).

-MA, (178-N,N-diethylcarbamoy1methylaza-5a-androstanone) has been found to inhibit 38-hydroxysteroid dehydrogenase activity in granulosa cells (Chan et al., Biochem. Biophys. Res. Commun. 144 -171, 1987). Epostane has been shown to inhibit 3B-hydroxysteroid dehydrogenase activity in pregnant goats (Taylor, J. Endocrinol. 113, -493, 1987).

Preferred inhibitors of 17B-hydroxysteroid dehydrogenase activity include but are not limited to: N-butyl, N-methyl-11—(16'a—chloro—3',l7'B—dihydroxy estra~l',3',5'(l0')— trien-7'a—y1) udecanamdde ("EM 139').

W (CHz)'°C0N(CH3)c‘H' N-n-butyl-N-methy1(l6'a-chloro-3',l7'a-dihydroxy-estra-1',3',5'(l0')- trien-7'u-yl) udecanamide ("EM 170') v (cH¢)..cou(cu3)¢4H' N-n—buty1—N-methyl(l6'a-brao-3',l7'a-dihydroxy-estra-1',3‘,5'(10')— trien-7'a—yl) undecanamide ("EM 171') Ho w(cHz)‘°coN(cH5)c‘Hg Examples of certain synthesis schemes for EM 139, EM 170 and EM 171 are set forth below (see example 2 and schemes 2 and 3). Those of skill in the art will recognize analogous schemes for synthesizing analogous compounds.

Exaple 2 SYNTHESIS OF PREFERRED SEX STEROID ACTIVITY INIBITORS Synthesis of a starting compound, N-n—buty1, N—methyl(3'-benzoy1oxy— '-oxo—estra-1',3',5'(10')—trien- 7'a—yl)udecanamide (14a) (SCHEME 2) -nor-testosterone acetate 3-enolacetate (7) In an apparatus supplied with a drierite drying tube, a solution of l9-nor-testosterone (6) (100 g; 0.365 mole) in acetic anhydride (200 ml). pyridine (32 ml) and acetylchloride (320 ml) was heated at reflux under magnetic stirring, for 3 h and then concentrated to dryness under vacuum. The dry residue was triturated in absolute ethanol, filtered and washed with little portions of absolute ethanol. After drying, 19-nor- testosterone acetate 3—enolacetate was obtained as a white powder (121.4 , yield 93%) mp. 176-177°C. The structure was confirmed by spectroscopic me ans .

B-acetoxy—estra-4,6-dienone (8) To a cooled suspension of enolacetate (121 g; 0.337 mole) in a mixture of DH (330 ml) and water (7.2 ml) at 0°C was added, under nitro- gen, over a period of 1 h, N-bromosuccinimide (63 g). The resulting solu- tion was stirred for an additional 0.5 h at 0°C. Then lithium carbonate (60.8 g) and lithium bromide (30.4 g) were added. The mixture was heated at 95°C for 3 h and then poured into 1.7 1 of ice-cold water containing 165 ml of glacial acetic acid. After stirring during 15 hours, the crude B-acetoxy-estra—4,6-dienone (8) was filtered, washed with water, dried in a desiccating apparatus and recrystallized twice from isopropyl ether (72 g, yield 68%, mp llO°C). The structure was confirmed by spec- troscopic means. a-(ll'-acetoxy-undecyl) 175-acetoxy estraenone (9) A. Preparation of reagents and solvents ll-bromo undecanol tetrahydro pyranyl ether ll-bromo-undecanol (100 g, 398 mmol) was dissolved in dry ether (768 _ ml) and the solution was cooled to 0°C using an ice/H30 bath. To this solution was added HCI gas (2.13 g, 58.4 mmol, 26 ml of HC1/ether).

To this mixture, a solution of 3,4-dihydro-2H-pyran (39.9 g, 43.3 ml) freshly distilled in dry ether (218 ml) was added over a period of 90 min. The solution was then stirred over a period of 16 hours at room temperature. Afterwards, sodium bicarbonate was added to the mixture.

The residue was filtered and the solvent was evaporated under vacuum.

The product was then filtered through basic alumina (250 3, Woelm, grade II) using petroleum ether (30-60) as solvent (112 3, 81%).

B. Grignard reagent In a dry three-neck flask (1000 ml) under dry argon, magnesium (12.0 g, 494 mmol) was placed and activated with iodine. Magnesium was heated with the flame to remove iodine and to dry the apparatus. The system was then cooled to -20°C, and a solution of ll-bromo-undecanol tetrahydro pyranyl ether (73.8 g, 211 mmol) in dry THE (420 ml) was added dropwise.

The mixture was stirred under dry argon during one day at -20°C.

The mixture was cooled to —35°C (i2°C) using a dry ice/CCL~/acetone bath. The anhydrous cuprous chloride (1.18 g, 12 mmol) was added and the mixture was stirred over a period of 0.5 h.

C. Addition of Grignard reagent After 0.5 h, using the same apparatus mentioned above (Ar, -35°C), a solution of 17 B-acetoxy estra-4,6-dieneone (8) (32.0 g, 102 mmol) in dry THE (300 ml) was added dropwise over a period of 6 h to the Grignard reagent (red coloration appeared and disappeared). The mixture was stirred for an additional 1 h and, after removal the cooling bath, acidified (about 0°C) with acetic acid (40 ml), diluted with water and extracted with ether (3x). The ether solution was washed with a saturated : sodium bicarbonate solution and water. The organic layer was dried over anhydrous magnesium sulfate and evaporated under reduced pressure to dryness.

The residue was dissolved in MeOH (660 ml) and SN HCl (180 ml), refluxed for l h and 45 min, then concentrated under reduced pressure and cooled in an ice bath. The mixture was then filtered to remove the white precipitate. After the solution had been diluted with water and extracted with methylene chloride (3x). the organic layer was dried over anhydrous Mgso, and evaporated under reduced pressure to dryness. Finally, the pro- duct (55.9 g, brown oil) was chromatographed on silica gel (Kieselgel 6OF254, Merck, 0.063-0.200 mm, 1500 g). Elution with mixtures of methyle- ne chloride and ethyl acetate (4:l to 1:2 v/v) and then pure ethyl aceta- te gave crude 7d-(ll'-hydroxy-undecyl)—l7B-hydroxy estraenone (34.8 g) which was dissolved in dry pyridine (200 ml) and dry acetic anhydride (200 ml), stirred 17 h at room temperature and then poured in ice-water.

The product was extracted with methylene chloride (3X), washed with 1N hydrochloric acid, water, saturated sodium bicarbonate and water (3X), dried on anhydrous magnesium sulfate and filtered. After evaporation of solvent, the mixture (35 g) of 7a- and 7B—diacetoxyenones and degradation products of Grignard reagent were separated by flash chromatography on silica gel (Kieselgel 60, Merck, 230 mesh ASTM, 2.0 kg) developed with a mixture of hexane and diethyl ether (2:3 v/v). The first product eluted was pure amorphous 7a-(11'-acetoxy undecyl) 17B-acetoxy-estraenone, (9) (20.8 g, 39.4 mol, yield from dienone was 39.0%). Further elu- tion gave the 7 B-isomer (10) (5.4 g, 10.3 mmol, 10%). All structures were determined by spectroscopic means. 7a-(11'-hydroxy-undecyl) estra-1,3,5(10)-trien-3,173-diol (lla) Under dry argon, a solution of 7a-(l1'-acetoxy undecyl) 17B-acetoxy- estraenone (9) (17.0 g, 32.4 mol) in dry acetonitrile (150 ml) was added rapidly to a suspension of cupric bromide (14.8 g, 66.2 mol) and mol) and lithium bromide (2.89 g, 33.6 mmol) in warm acetonitrile (75 ml). The mixture was heated to reflux over a period of 30 min and stirred vigorously, and then cooled to room temperature. A saturated aqueous solution of sodium bicarbonate (50 ml) was added, and then the organic compound was extracted with ethyl acetate (3x 150 ml). The orga- nic layers were washed with water, dried over anhydrous magnesium sulfa- te, filtered and evaporated under vacuum to dryness. The residue was’ chromatographed on silica gel (Kieselgel 60F254 Merck 0.063-0.200 mm; 1000 g). Elution with hexane-ethyl acetate (l:1 v/v) gave the 7a-(11'- acetoxy-undecyl) estra-1',3',5'(l0')-trien-3,175-diol, 17B-acetate (llb) (8.51 g; 50.3%) and the starting product (1.33 g; 15%).

The above diacetate phenol (8.51 g, 16.2 mmol) was dissolved in me- thanol (90 ml) and sodium hydroxyde 30% (w/v) (9 ml). The mixture was refluxed for 90 min under dry nitrogen. The solution was then concentrat- ed under vacuum and diluted with hydrochloric acid (10% V/V). The mixture was extracted using ethyl acetate (4 x 150 ml) and the ethyl ace- tate extract was washed with water, dried over anhydrous magnesium sulfa- te, filtered and evaporated under vacuum. The evaporation gave 7a-(ll'- hydroxy undecyl) estra-1,3,5(lO)-trien-3,178-diol (113) (6.99 g, 98% brut) as a yellow foam, the structure of which was confirmed by spectros— copic means. -benzoyloxy 7a-(ll'-hydroxy undecyl) estra-1,3,5(10)-trienol (12) The above triol (6.99 g; 15.8 mmol) was dissolved in acetone (25 ml) and an aqueous solution of sodium hydroxyde (IN, 19.1 ml). The mixture was cooled to 0°C using an ice/water bath. Benzoyl chloride (2.22 ml, 19.1 mmol) was then added dropwise. The mixture was stirred for 40 min at 0°C and then diluted with water. The solution was extracted using ethyl acetate (3K) and the organic layers were washed with a saturated aqueous solution of sodium bicarbonate and finally with water. The ethyl acetate solution was dried over anhydrous magnesium sulfate, filtered and evapo- rated under vacuum to dryness. Then. the residue was immediately chroma- tographed on silica gel (Kieselgel, 6OF2S4, 0.063-0.200 mm; 500 g). The chromatography was carried out, first, using methylene chloride as sol- vent (about l liter) and secondly the pure 3-benzoyloxy 7a-(ll'-hydroxy undecyl) estra-1,3,5(lO)—trien-17B-ol (12), colorless oil (6.50 g, %) was eluted with methylene chloride-ethyl acetate (5:l about 1 liter and 4:1; v/v). The structure was confirmed by spectroscopic means. ll-(3'-benzoyloxy-l7‘-oxo—estra-1',3‘,5'(10')-trien-7'a-yl) undecanoic acid (13) To a cooled solution of 3-benzoyloxy-7a-(ll‘-hydroxy undecyl)estra- l,3,5(10)-trien-17B-ol (12) (4.3 g) in acetone (100 ml) was added dropwise Jone's reagent (8N-chromic acid solution, 6.7 ml). After 30 min, isopropanol (40 ml) was added and the mixture was concentrated under vacuof Water was added and the mixture was extracted four times with ethyl acetate. The organic layers were washed twice with brine, dried ; over magnesium sulfate and evaporated to dryness. The crude 11-(3'-ben- zoyloxy-17’-oxo-estra-1',3’,5'(l0')-trien-7'd-yl) undecanoic acid (13) (3.94 g) was used in the next step without purification.

Scheme 2 O OH o’C-CH3 H H 0 H3CO2 / 7 <3 / 9 /C—CH3 /C-CH3 O _._:_._).

QHEEE H O O (CH2)10CH2OCOCH3 7*BH / 10 7-aH on / OH >- > HO "'(CH2)1QCH2OH C6H5CO2 ."(CH2)10CH2OH 110 R = H 12 11 b R = COCH3 / o o C(,H5CO2 "’(CH2)mCO2H redo "'(CH2)10CO2H 13 14:1 R0 = C6H5CO b RQ=H N-n-butyl,n-methyl—1l— (3'-hydroxy—l7'—oxo-estra-1',3',5'(10')-trienr 7'a—yl) undecanamdde (l4b) To 11-(3'-benzoyloxy-17'-oxo-estra-1',3',5'(l0')-trien-7‘a-yl) unde- canoic acid (13) (3.94 g, 7.22 mmol), dissolved in anhydrous CH,Cl, (100 ml) and cooled at -10°C was added tributylamine (2.18 ml, 9.15 mmol) and isobutylchloroformate (1.30 ml, 10.0 mmol). The solution was stirred during 35 min. and N-methylbutylamine (13 ml, 109.7 mmol) was added. The mixture was warmed to room temperature and stirred during 1 h. Afterward, CHZCII was added and the organic phase was washed with lN HCl, water, saturated sodium bicarbonate solution and finally with water, dried with anhydrous Mgso‘ and the solvent was removed under reduced pressure. The residue was purified by chromatography on silica gel. Elution with mixtu- re of Et0Ac/hexane (1.5:8.5 v/v) yielded N-butyl, N-methyl-ll-(3'- ben- zoyloxy-17'-oxo-estra-1',3‘,5‘(10')-trien-7'a-yl) undecanamide (lha) (4.25 g, 96%) as colorless oil; IR u (neat) 1750, 1725 and 1640 cm-1. The above described benzoyloxy amide (341 mg, 0.54 mmol) was dissolved in methanol (10 ml) and cooled at 0°C. Following this ZN NaOH (5 ml) was added and the mixture was stirred during 60 min. at 0°C. The solution was neutralized with 1N HCl and extracted with CH,Cl,. The organic phase was dried with anhydrous MgS0. and the solvent was removed under reduced pressure. The residue was purified by chromatography on silica gel.

Elution with mixture of Et0Ac/hexane (3:7 v/v) yielded N-butyl, N-methyl- 11-(3'- hydroxy—l7'-oxo—estra-1',3',4'(10)-trien-7'a-yl) undecanamide (14b) (284 mg, 97%) as colorless oil; ‘H-NMR 6 (CDC13) 0.91 (s,3H,18‘-CH3), 2.76 app(d,1HJ=l6,3Hz, part of ABX system, 6’-H) 2.96 and 2.98 (2s,3H N-CH3), 3.27 and 3.38 (2tapp,2H,J=7.5Hz,N-CH,-), 6.63 (broad s,lH,4‘-H), 6.70 (broad d,1H,J= 8.5 Hz,2'-H), 7.12 (d,lH,J=8.4 Hz,l‘-H); IR vmax (neat) 3270, 1730, 1615 cm~1; MS m/e 523 (M*,100%), 508 (M'-CI-13,322), 142 (c,H_coN(cH,)c H ‘ 47%).

-HALO-ESTRADIOL UNDECANAMIDE (SCHEME 3) N—nrbutyl, Rsmethyl-ll-(3',17'—diacetoxy-estra-1',3’,5'(l0'),l6'—tetraen- 7'ary1) undecanamide (15) The ketone amide 1#b (163 mg, 0.50 mmol) was dissolved in isoprenyl acetate (10 ml). p-toluenesulfonic acid (44 mg) was then added and the solution was distilled to about two-thirds of the original volume in 7 h and was then stirred at reflux for 12 h. Afterwards, the solution was cooled with an ice-water bath and extracted with 50 ml of cooled ether. The ether was washed with a cooled satured sodium bicarbonate and water. The organic phase was dried with anhydrous MgS0. and the solvent was removed under reduced pressure. The residue was filtered through alur mina (l5m x 50 m alumina Woehlm neutral, activity II) using a mixture of benzene-diethyl ether (3:7 V/v) as eluant. The solvent was removed under reduced pressure and, the residue was purified by flash chromato- graphy on silica gel. Elution with mixture of Et0Ac/hexane (l:4 v/v) yielded the N-butyl, N-methyl(3'.17’-diacetoxy~estra-1',3‘,5'(lO'). 16'-tetraen-7'a-yl) undecanamide (15) (244 mg, 80%) as colorless oil; 1H-NHR 6m(CDC1,) 0.92 (s,3H,18'-CH3), 0.92 and 0.95 (2t,3H,J=7.0 Hz,N(cH,),cg,), 2.18 (s,3H,17'-ococH,). 2.28(s,3H,3'-ococH,), 2.75 app (d,lH,J=l6.l Hz, part of ABX system,6'-H), 2.90 and 2.96 (2s,3H,N-CH,). 3.26 and 3.35 (2taPP,2H,J=7.6 Hz,N—CH,-), 5.52 (m,lH,l6'-H). 6.80 (broad s,lH,4'-H), 6.85 (dd,lH,J1=9.l Hz and J,=3.0 Hz,2'-H), 7.27 (d,lH,J=9.l Hz,l'-H): IR UmaX(neat) l750, 1635, 1200 cm-1; MS m/e 607 (M‘,2%).

S(M*~COCH,,lO0%).

(M’-COCK:-CH3,l3%), 523 (M’-2COCH1,45%), 142 (C2H,CON(CH3)C.H,’,55%). 129 (c,H,(cH,)NcocH3-,38%), 114 (c,H,(cH,)Nco*, 50%), 86 (c,H,(cH,)N*, %); EXACT MASS calcd for c,,H5,o5N 507.4239, found 507.4234.

N—buty1, N—methy1(16'a—ch1oro-3'acetaxy-17'-oxo—estra-1',3',#' (10')-triene-7'a—yl) umdecanamde (16, X = C1) cm-1; HS m/e 601, 599 (M’,24%, 68%), 142 (C,H~C0N(CH3)C H ‘ %). 114 (c,H,(cH,)Nco~,93%).

N—butyl, N-methyl-ll-(160.-chloro-3 ' , 17 ’-dihydxaxy-estra-1' ,3 ' ,5 ' (10' )- trien-7'u.-yl) undecanamide ("EM 139'‘) and ("E11 170'‘) A stirred solution of haloketone amide (16, X=Cl) in anhydrous tetrahydrofuran (THF) (10 ml) under argon was chilled to —70°C with 2-propanol/dry ice bath. A solution of 1.0 M of lithium aluminium hybride (2 eq.) was then added dropwise. After 30 min, the reaction was allowed to return slowly at 0°C for 5 min, ‘then was quenched by the dropwise addition of a mixture of THE-Et0Ac (5 ml) (1:l v/v) and acidified at pH N 4 with (10%) H01. The mixture was stirring for 5 min at room temperature and then extracted with Et0Ac. The organic phase was washed with water, dried on anhydrous Na,S0. and evaporated under reduced pressure. The residue was chromatographed on silica gel with a mixture of Eto0Ac/hexane (4:6 v/v) as eluant: N-butyl, N-methyl-ll-(l6’a—chloro-3‘l7'u-dihydroxy-estra-1',3’,5‘(10‘)- trien-7'a-yl) undecanamide ("EM 170') (15 mg, 29%) as colorless oil; analytical sample was obtained by HPLC purification; 1H-NMR 6 (CDCI3, 400 MHz) 0.79 (s,3H,l8'-CH3), 0.93 and .96 (2t, 3H,J=7.3 Hz,N(cH,),cH,), 2.80 (2H,J,,,=17.1 Hz and J,,, .5 Hz, A6=24.34 (Hz, system ABX, 6"H), 2.94 and 2.99 (25, 31-I,N-CH,), .26 (dd,J1 = 7.6 Hz and J: = 7.4 Hz) and 3.32-3.43 (m)-[2H,-N—CH,-], .71 (d,lH,J=4.5 I-Iz,l7'B-H), 4.63 (ddd, 1H, J 10.2 Hz, J .15 16.17. =a.5 Hz and J15,15 3.9 Hz, l6'B-H), 6.50 (d, 1H, J=24 Hz, 3'—OH). 6.60 (d, lH,J=2.5 Hz, 4'—H), 6.66 (dd,lH,J1=8.4 Hz and J,=2.5 Hz, 2'-H). 7-14 (d,lH,J=8.5 Hz, l’-H); IR umax(neat) 3300, l615, 1495 cm‘1; MS m/e ,559 (M*, 40%, 100%), 523 (M‘-HCl, 20%). 142 (C,H‘C0N(CH3)C,H,’, 44%), (C‘H9(CH3)CN0*, 37%); Exact mass calculated for C3,H5,03N35C1 .3785, found 559.3821; — and - -N-butyl, N-methyl(16'a—chloro—3',17’B-dihydroxy—estra-1'3',5'(l0‘)- trien-7'a-yl) undecanamide ("EM 139") (25 mg, 55%) as a colorless oil; analytical sample was obtained by HPLC purification; 1H-NMR 6 (C001,, 400 MHZ), 0.81 (s,3H, 18'—CH,), 0.93 and 0.96 (Zt, 3H,J=7.3 Hz, (CH,)3CH,), 2.78 (2H, J,,5=16.2 Hz and J5,, = 4.5 Hz, A5=24.34 Hz, systan ABX, 6'-H), 2.94 and 2.99 (25, 3H,N-CH3), .27 (dd, J1=7.6 Hz and J,=7.5 Hz) and 3.31-3.45 (M)[2H, -N-CH,-1, 3.86 (dd, 1H, J,,,,,-OH=3.4 Hz and J,,,,, -5.9 Hz, 17’a-H), 4.11 (ddd, 1H, J,,,,, =1o.a Hz, J,,,,,=5.9 Hz and 4.11 (ddd, 1H, J = 10.8 Hz, J,,,,, = 5.9 Hz and J,,,,,=2.5 Hz, 16'B-H), 6.56 (d, 1H, J=19.7 Hz, 3'- oa), 6.61 (d, 1H, J=2.5 Hz, 4'-H), 5.55 (dd, 1H, J,=a.4 Hz and J,=2.5 Hz, ‘-H), 7.13 (d, 1H, J=8.4 Hz, 1'-H); IR V max(neat) 3320, 1615, 1490 cm‘1; MS m/e 561,559 (M‘, 38%, 100%), 523 (M’-HCl, 16%), 142 (C,H,C0N(CH3)C,H,‘, 80%), 114 (C,H,(CH,)NCO‘,76%): exact mass calculated for c,_H,,o,N==c1 559.3785, found 559.3825.

Scheme 3 -9,’ ¢ X=C1,Br an an an 139 171 ~W"(CH > cnNc H 2 1o 3 4 9 X=Br, Rb=0H, R==H X=Br, Rb=H, Rc=0H x=c1, Rb=0H, R¢=H x=c1, Rb=H, Rc=0H x=1, Rb=0H, Rc=H N—n-butyl, N-methyl(16'u-broo-3'-acetoxy-17'-oxn-estra-1',3',5'— (l0'),trienr7'a-yl) udecanamide (16, X=Br) To the above diacetate 15 (244 mg, 0.40 mol) dissolved in 10 ml of acetic acid was added dropwise with stirring within 10 minutes and at room temperature, a brominating solution composed of 50 mg (0.6 mmol) of sodium acetate, 1.6 ml of acetic acid, 0.04 ml of water and 63.9 mg (0.02 ml, 0.40 mmol) of bromine. During the course of this reaction, a red coloration appeared and disappeared. To the solution, 50 ml of ether was added and the organic phase was washed with water (4 x 50 ml) followed by a saturated sodium bicarbonate solution (2 x 50 ml) and finally with water (3 x 50 ml). The combined phase was dried over anhydrous magnesium sulfate and the solvent was removed in vacuo. The residue was chromato- graphed on silica gel (Kieselgel, 60F254, Merck, 0.063-0.200 mm). Elu- tion with a mixture of hexane-ethyl acetate (4:l v/v) yielded N-butyl, N-methyl-ll-(16c-bromo-3'-acetoxy-17‘-oxo-estra-1',3‘,5'(10'),trien-7'-c- yl) undecanamide (16, X-Br) (201 mg, 78%) as colorless oil (201 mg. %), as colorless oil; ‘H-NMR o (CDCl,), 0.94 (s, 3H,l8'-CH,), 2.28 (s, 3H, 3'-0COCH,). 2.82 app (d,lH,J-16.4 Hz, part of ABX system, 6'-H), 2.90 and 2.96 (25, 3H,N-CH3), 3.24 and 3.35 (Zta 2H, J=7.7 Hz, -N-CH,‘). pp’ 4.58 (t,lH,J-3.6 Hz, 16$-H), 6.82 (broad s,lH,4'-H), 6.88 (dd,lH, J-8.0 Hz and 3,: 4.0 Hz,2'-H), 7.29 (d,lH,J=B.0 Hz, l'—H); MS m/e 544 (n~.7z). 555 (M* — Br, 77:), 522 (M*-Br-cocH,, 55%). 142 (C,H,CON(CH,)C,H,‘, 57:), (C,H,(CH,)NCO*, 66%), 88 (100%).

N-butyl, N-methy1—l1—(16'a-broo-3',17'—dihydroxy—estra-1',3,#'(l0‘)- trien-7'a-yl) undecanamdde ("EM 105") and ("EH 171") A solution of bromoketone amide l6 (X=Br) (295 mg, 0.46 mmol) in anhydrous tetrahydrofuran (10 ml) under argon was chilled to -70°C and a solution of 1.0 M of lithium aluminium hybride in ether (0.92 ml, .92 mmol) was added dropwise with rapid magnetic stirring. After 30 min, the reaction was quenched by the dropwise addition of a mixture of THE- ethyl acetate (l:l v/V) and acidified by 10% hydrochloric acid. The mix- : ture was stirring for 5 min at room temperature and then extracted with ethyl acetate. The organic phase was washed with water, dried on anhy- drous sodium sulfate and evaporated to dryness under reduced pressure.

The residue was purified by chromatography on silica gel. Elution with a mixture of hexane-ethyl acetate (7:3 v/v) gave: N-n-butyl, N-methyl-ll-(15‘d-bromo-3',l7'a-dihydroxy-estra- l',3',5'(l0')-trien-7'd-yl) undecanamide ("El 171') (63 mg, 21%) as colorless oil; 1H-NMR 6 (CDC1,, 400 M2) 0.81 (3, 3H. l8'—CH,). 0.93 and 0.96 (Zt, 3H,J=7.3 uz,N(ca,),cn,), 2.79 (2H,J5’6=l6.6 Hz, J6’7=4.7 Hz, = A6=24.34 Hz. system ABX,5‘-H), 2.94 and 2.99 (2S,3H,N~ CH3), 3.27 (dd,2H,J1=7.7 Hz and J,=7.5 Hz, -N-CH,-), 3.31-3.44 (m,2H.-N- CH,-), 3.55 (dd,lH,Jl7,l7=1.4 Hz, 317,16 =4,3 Hz, m, J16 l5=9.7Hz,l6'B-H), 6.60 (d,lH,J=2.4 Hz, = 4,3 Hz, 17'B-H), 4.68 (dt,lH,Jl6’17 '-H), 6.65 (dd, lH,J=8.5 Hz and J2=2.5 Hz, 2'-H), 7.14 (d,lH,J=8.5 Hz, l‘-H); IR vmax (neat) 3300, 1515, 1495 cm'1; MS m/e 605,603 (M’, 17%).

(M‘-HBr, 81%), 142 (c,n.coN(cH,)c H ~ 100%). 114 (C‘H,(CH,)NCO’, %)} Exact mass calculated for C3‘H O N"Br 603.8289, found 603.3304.

N—n-butyl, N-methyl—1l-(l6'a-brao—3',17'B-dihydray-estra-l',3',- '(10')—trien-7a-yl) umdecanamide ("EM 105") (170 mg, 50%) as a colorless oil; analytical sample was obtained by HPLC purification; ‘H-NMR 6 (CDCIJ, 400 MHZ), 0.80 (s,3H,l8,-CH3), 0.93 _ A6=24.34 Hz, system ABX, 6'-H), 2.94 and 2.99 (2s,3H,N-CH3), 3.27 (dd, H,J1=7.7 Hz and J,=7.5 Hz, -N-CH,-), 3.31-3.45 (m,2H,—N—cH,-), 4.02 (dd,lH,Jl7’l7= 3.7 Hz, and Jl7’16=6.1 Hz, l7'a-H), 4.15 (ddd,lH,Jl6’15= .2 Hz, J15'l7= 6.1 Hz and Jl6’l5 =2.9 Hz, l6'B-H). 5.61 (d,lH,J=2.5 Hz, 4'-H), 5.66 (dd,lH,J=8.# Hz and J, 2.5 Hz, 2'*H), 7.12 (d,lH.3=8.4 Hz, 1'-H); IR vmax (neat) 3320, 1610, 1490 cm'1; MS m/e 605, 603 (M’, 29%), 523 (M'-HBr, 100%), 142 (c,H,coN(cH,)c,H,~, 70%), 114 (C‘H,(CH,)NCO’, 60%); Exact mass calculated for C,‘H5.0,N7'Br 603.3289, found 603.3289.

Antiestrogens useful in the combination therapy of the invention include but are not limited to Tamoxifen, commercially available from Imperial Chemical Industries, and EM 139, EM 170 and EM l7l whose synthe- sis are set forth above. Some steroidal antagonists also function as in- hibitors of sex steroid formation. The antiestrogens EM l39, EM 170 and EM l7l, for example, exhibit the dual function of acting as sex steroid formation inhibitors. For this reason, a combination therapy requiring both an inhibitor of sex steroid formation and a steroidal antagonist may be produced by administering a single active compound (alone or together with diluent) capable of performing both functions. Another example of a dual function active ingredient is the antiandrogen EM 101 which has also shown an inhibitiory effect on sex steroid formation.

The inhibitor of sex steroid biosynthesis is preferably capable of acting at least in peripheral tissues (extra-testicular and extra-adre- nal)~ In preferred embodiments, it is used in association with an antian- drogen, and with an LHRH agonist or LHRH antagonist. The use of an LHRH agonist is the more preferred method of chemical castration. Surgical castration may alternatively be used as a means of inhibiting testicular hormonal secretions, but chemical castration is preferred.

By the term "LHRH agonist" is meant synthetic analogues of the natu- ral luteinizing hormone-releasing hormone (LHRH), a decapeptide of the structure: L-pyroglutamyl-L-histidyl-L-tryptophyl-L-seryl-L-tyrosyl- gly- cyl-L-leucyl-arginyl-L-prolylglycyl-NH1.

Typical suitable LHRH agonists include nonapeptides and decapeptides represented by the formula: L-pyroglutamyl-L-histidyl-L—tryptophyl-L- seryl—L-tyresyl—X—Y-L—arginyl-L-prolyl-Z wherein X is D-tryptophyl, D- leucyl, D-alanyl, iminobenzyl—D~histidy1, 3-(2-naphthyl)-D—alanyl, O-ter- butyl—D-seryl, D—tyrosyl, D-lysyl, D-phenylalanyl or N-methyl—D- alanyl and Y is L—leucyl, D—leucyl, N"-methyl—D-leucyl, N"-methyl-L— leucyl or D-alanyl and wherein Z is glycyl-NHR, or NHR1 wherein R, is H, lower alkyl or lower haloalkyl. Lower alkyl includes, for example, methyl.

Haloloweralkyl includes, for example, -CF-3, -CHZCFJ, -CF,CH,, and the like. Fluorine is a preferred halogen.

Preferred nonapeptides wherein Y is L—leucyl and X is an optically active D-form of selected amino acids and Z is NHC1H5 are [D-Trp‘, des- Gly-NH,1°]LHRH ethylamide (X=D-Trp‘); [D-Ser-t-Buo)‘, des-Gly-NH,1°]LHRH ethylamide [X-D-Ser(t-BuO‘)l; [D-Leu°, des-Gly-NH,1°]LHRH ethylamide (X=D-Leu‘, [D-His(Bzl)‘, des—G1y—NH,1°]LHRH ethylamide (X=iminobenzyl-D- His‘) and [D-Ala‘, des-Gly-NH,1°]-LHRH ethylamide (X=D-Ala‘).

Preferred decapeptides include [D-Trp‘]LHRH wherein X=D-Trp, Y=L- leucyl, Z=glycyl-NHZ, [D-Phe‘]-LHRH wherein X=D—phenylalanyl, Y=L-leucyl and Z=glycyl-HN2) or [D-Nal(2)‘LHRH which is [93-3—(2-naphthyl)—D—Ala‘]- LHRH wherein X=3(2-naphthyl)-D-alanyl, Y=L-leucyl and Z=glycyl-NH,.

Other LHRH agonists useful within the scope of this invention are the a-aza analogues of the natural LHRH, especially. [D-Phe‘, Azgly‘°]- LHRH, [D-Tyr(-Me)‘, Azgly‘°]LHRH, and [D-Ser-(t-BuO)‘. Azgly1°]LHRH dis- closed by A.S. Dutta et al. in J. Med. Chem., 21, 1018 (1978) and U.S.

Pat. No. 4,100,274 as well as those disclosed in U.S. Pat. Nos. 4,024,248 and 4,118,483.

Typical suitable LHRH antagonists include [N-Ac-D-p~Cl-Phe1,', D—Phe3, D-Arg‘, D-A1a1°]-LHRH disclosed by J. Ercheggi et al., Biochem.

Biophys. Res. Commun. 100, 915-920 (1981); [N-Ac-D-p-Cl-Phe1,’, D-Trp’, D-Arg‘, D-Ala1° JLHRH disclosed by D.H. Coy et al., Endocrinology, ll0: l445—l447 (1982); [N-Ac-D-(3—(2—naphthyl)—0Ala)1, D-p-Cl-Phe‘, D-Trp3, D-hArg(Et,)‘, D-Ala1°]LHRH and [N-Ac—Pro1v D-pF-Phe3, D-(3-(2-naphthyl)- Ala3,‘l-LHRH disclosed by J.J. Nestor et al. J. Steroid Biochem., 20 9no.

B), 1366 (1984); the nona— and decapeptide analogs of LHRH useful as LHRH antagonists disclosed in U.S. Pat. No. 4,481,190 (J.J. Nestor et al.); analogs of the highly constrained cyclic antagonist, cycle [A’ Pro‘, D-p-C1-Phel, D-Trp3,‘, N-Me-Leu7, B—Ala1°]-LHRH disclosed by J.

Rivier, J. Steroid Biochem., 20 (no. 68), 1365 (1984); and [N-Ac-D-(3- (2-naphthpyl)~Ala1, D-p-F-Phe3, D-Trp3, D-Arg‘]LHRH disclosed by A.

Corbin et al., J. Steroid Biochem. 20 (no. 6B) 1369 (1984).

Preferred nonapeptides wherein Y is L-leucyl and X is an optically active D-form of selected amino acids and Z is NHCZHS are [D-Trp‘, des- Gly-NH,1°]LHRH ethylamide (X=D-TIP‘); [D-Set-t—BuO)‘, des-Gly-NH,1°]LHRH ethylamide [X-D-Ser(t-BuO‘)]; [D-Len‘, des-Gly-NH,1°]LHRH ethylamide (X=D-Leu‘, [D-His(Bz1)‘, des—Gly-NH21°]LHRH ethylamide (X=iminobenzyl-D- ‘ His‘) and [D-Ala‘, des-Gly-NH,1°]-LHRH ethylamide (X=D-Ala‘).

Preferred decapeptides include [D-Trp‘]LHRH wherein X=D-Trp, Y=L- leucyl, Z=glycyl-NH,, [D-Phe‘]-LHRH wherein X=D-phenylalanyl, Y=L-leucyl and Z=glycyl-HN,) or [D-Nal(2)°LHRH which is [93(2-naphthyl)-D-Ala‘]- LHRH wherein X=3(2-naphthyl)~D-alanyl, Y=L-leucyl and Z=g1ycyl-NH,.

Other LHRH agonists useful within the scope of this invention are the a-aza analogues of the natural LHRH, especially, [D-Phe‘, Azgly‘°]- LHRH, [D-Tyr(~Me)‘, Azgly1°]LHRH, and [D-Ser-(t-Buo)‘, Azgly1°]LHRH dis- closed by A.S. Dutta et al. in J. Med. Chem., 21, 1018 (1978) and U.S.

Pat. No. 4,100,274 as well as those disclosed in U.S. Pat. Nos. ,024,248 and 4,118,483.

Typical suitable LHRH antagonists include [N-Ac-D-p-Cl-Phe1,‘, D-Phe3, D-Arg‘, D-Ala‘°]-LHRH disclosed by J. Ercheggi et al., Biochem.

Biophys. Res. Commun. 100, 915-920 (1981): [N-Ac-D-p-C1-Phe1,‘, D-Trp3, D—Arg°, D—A1a1° ]LHRH disclosed by D.H. Coy et al., Endocrinology, 110: 1445-1447 (1982); [N-Ac-D-(3—(2—naphthyl)-OAla)1, D-p-C1—Phe3, D-Trp’, D-hArg(Et2)5, D-Ala1°]LHRH and [N-Ac—Pro1, D-pF-Phe', D-(3-(2-naphthyl)~ A1a3,‘]-LHRH disclosed by J.J. Nestor et al. J. Steroid Biochem., 20 9no.

B),~l366 (1984); the nona- and decapeptide analogs of LHRH useful as LHRH antagonists disclosed in U.S. Pat. No. 4,481,190 (J.J. Nestor et al.); analogs of the highly constrained cyclic antagonist, cycle [A3 Prol, D-p-Cl-Phez, D-Trp3,°, N-Me-Leu7, B—Ala1°]-LHRH disclosed by J.

Rivier, J. STeroid Biochem., 20 (no. 6B), 1365 (1984); and [N-Ac-D-(3-(2- naphthpyl)-Ala‘, D-p-F-Phe’, D-Trp3, D-Arg‘]LHRH disclosed by A. Corbin et al., J. Steroid Biochem. 20 (no. 68) 1369 (1984).

Other LHRH agonist and antagonist analogs are disclosed in LHRH and its Analogs (B.H. Vickery et al. eds, at pages 3-10 (J.J. Nestor), 11-22 (J. Rivier et a1.) and 22-33 (J.J. Nestor et al.) as well as in The Case for LHRH agonists (Clinical Oncology, Furr and Denis, eds), Bailliére Tindall, vol. 2, no. 3, pp. 559-570, 1988).

The LHRH agonists and antagonists useful in this invention may con- veniently be prepared by the method described by Stewart et al. in "Solid Phase Peptide Synthesis" (published in 1969 by Freeman & Co., San Francisco, page 1) but solution phase synthesis may also be used.

The nona- and decapeptides used in this invention are conveniently assembled on a solid resin support, such as 1% cross-linked Pro-merri- field resin by use of an automatic peptide synthesizer. Typically, side- chain protecting groups, well known to those in the peptide arts, are used during the dicyclohexylcarbodiimidecatalyzed coupling of a tert-bu- tyloxycarbonylamino acid to the growing peptide attached to a benzhydry1- amide resin. The tert-butyloxycarbonyl protecting groups are removed at each stage with trifluoroacetic acid. The nona- or decapeptide is cleaved from the resin and deprotected by use of HF. The crude peptide is puri- fied by the usual techniques, e.g., gel filtration and partition chroma- tography and optionally lyophilization. See also D.H. Coy et al., J.

Med. Chem. 19, pages 423-425 (1976).

‘In this invention, the LHRH agonist or antagonist, the 5a-reductase inhibitor, the antiandrogen, the antiestrogen, and, where applicable, the inhibitor of 38- and 175-hydroxysteroid dehydrogenase activities are administered as pharmaceutical compositions via topical, parenteral or oral means. The LHRH agonist or antagonist is administered parenterally, i.e., intramuscularly, subcutaneously or intravenously by injection or infusion by nasal drops or by suppository. The LHRH agonist or antagonist may also be microencapsulated in or attached to a biocompatable, biode- gradable polymer, e.g., poly(d,l-lactide-co-glycolide) and subcutaneously or intramuscularly injected by a technique called subcutaneous or intra- muscular depot to provide continuous, slow release of the LHRH agonist or antagonist over a period of 30 days or longer. The most preferred route of administration of the LHRH agonist or antagonist is subcutaneous or intramuscular depot injection. Preferably the antiestrogen will be admi- nistered orally. Preferably, the Sa-reductase inhibitor, the antiandro- gen, the antiestrogen, the inhibitor of 3B-HSD and the inhibitor of 17B- HSD can also be administered orally. The antiestrogen, an inhibitor of 3B-HSD and inhibitor of 17B-BSD can also be administered in a slow release formulation, e.g. poly(d,l-lactide-coglycolide) or as implants.

The amount of each component administered is determined by the attending clinicians taking into consideration the etiology and severity of the disease, the patient’s condition and age, the potency of each component and other factors. According to this invention, the following dosage ranges are suitable.

The LHRH agonist or antagonist is generally administered at from about 10 to 5000 pg per day with contemplated dosage ranges of about 10 to 1500 pg per day and about 250 (preferably 50 ug to 500 pg per day) for the LHRH agonist and to about 100 to 2000 pg per day for the LHRH antago- nist being preferred.

In the most preferred embodiment of this invention, the LHRH agonist or antagonist is administered subcutaneously in a daily dose of 500 ug for the first 30 days and thereafter subcutaneously in a daily dose of 250 ug regardless of the patients‘ body weight. When the LHRH agonist or antagonist is administered, once every 30-day period is used, with a dose of 750 to 15,000 pg per 30-day period being preferred. Similar daily delivery doses are used for longer-term controlled release formulations.

The inhibitors of 3B-HSD and 17B-HSD are preferably administered in dosages ranging from about 0.1 to 25 mg/kg per day with 200 mg per day in two equally divided doses being preferred.

The antiestrogen compositions are administered in a dosage range of about 0.05 to 25 mg/kg body weight per day, with 20 mg, especially 40 mg, in two equally divided doses being preferred.

The 5a—reductase inhibitor compositions are administered in a dosage ranging from 0.1 to 25 mg/kg per day with 50 mg per day in two equivalent doses being preferred.

' The antiandrogen and aromatase inhibitor compositions are administe- red in a dosage range of 0.5 to 25 mg/kg body weight per day with 750 mg per day in three equally divided doses being preferred.

The LHRH agonist or antagonist, antiestrogen, antiandrogen, an inhi- bitor of aromatase, 17B-HSD and 3B-HSD each may be administered separate- ly or when the modes of administration are the same, all or at least two of them may be administered in the same composition, but in any case the preferred ratio of LHRH agonist to antiestrogen, to antiandrogen to inhi- bitor of 17B-HSD and administered daily will be about 250 pg of LHRH ago- nist to about 750 mg of antiandrogen, about 40 mg of antiestrogen, to about 40 mg of inhibitor of 17B-HSD and about 1+0 mg of inhibitor of 38-HSD.

In the therapy of prostate cancer, combining the administration of an LHRH agonist or antagonist, an antiestrogen, an antiandrogen and an inhibitor of l7B‘HSD, the dosages preferable are as follows: the LHRH [*0 U1 agonist or antagonist is generally administered at from about 10 to 2000 pg per day, with contemplated dosage ranges of 10 to 500 pg per day, 50- 250 pg per day and 250 to 500 pg per day being preferred. In the most preferred embodiment of this aspect of this invention, the LHRH agonist or antagonist is administered subcutaneously in a daily dose of 500 pg for the first 30 days and thereafter subcutaneously in a daily dose of 250 pg regardless of the patients’ body weight. When the LHRH agonist or antagonist is administered, once every 30-day period, by intramuscular or subcutaneous depot injection, a dose from about 300 to 60000 (occasional- ly 10000) pg per 30-day period is used, with a dose of 750 to 2000 pg per ‘ 30-day period being preferred. The antiandrogen composition is generally administered in a dosage range of about 0.5 to 25 mg/kg (body weight) per day with 400 especially 750 mg per day in three equally divided doses being preferred. The antiestrogen and inhibitor of 17B-HSD and 3B-HSD activities are administered in a dosage range of about 0.1 to 25 mg/kg body weight per day, with 100 mg in two, preferably with 50 mg in two, equally divided doses being preferred.

The LHRH agonist or antagonist, antiandrogen, antiestrogen, 5a-re- ductase inhibitor, inhibitor of 178-350, inhibitor of 3B-HSD, inhibitor of aromatase, each may be administered separately or when the modes of administration are the same, all or two or three of them may be adminis- tered in the same composition, but in any case the preferred ratio of LHRH agonist to antiandrogen to antiestrogen administered daily will be about 750 pg of LHRH agonist to about 250 mg of antiandrogen to prefera- b ly 40 mg of antiestrogen.

In the therapy of prostate cancer, according to this invention, it is preferred that the LHRH agonist is [D-Trp‘, des-Gly-NH,1°]LHRH ethyl- amide be administered subcutaneously in single daily dose of 500 pg for the first thirty (30) days of treatment and thereafter in a single daily dose of 250 pg.

In the combination therapy of prostate cancer according to this invention, the administration of the antiandrogen, antiestrogen, inhibi- tor of l7B—HSD, inhibitor of 5o-reductase, inhibitor of aromatase, and inhibitor of 38-HSD, LHRH agonist or LHRH antagonist can be started in any order of sequence. Preferably, the administration of the antiandrogen and 5a-reductase inhibitor, are started before (preferably two to four hours before) the administration of the LHRH agonist or LHRH antagonist is started. Orchiectomy can replace LHRH agonist or antagonist.

Preferably, the administration of the inhibitor of 175-HSD and inhibitor of 38-HSD is started on the same day as the administration of the LHRH agonist or LHRH antagonist. However, the attending clinician may elect to start adminsitration of the LHRH agonist or antagonist simultaneously with the antiandrogen, antiestrogen inhibitor of 17B-HSD and inhibitor of -HSD.

When patients whose testes have already been surgically removed are treated according to this invention, the administration and dosage of the antiandrogen and the other components of the therapy (except the LHRH agonist or antagonist which is not used) are the same as indicated for the therapy in which the LHRH agonist or antagonist is used.

The LHRH agonists or antagonists useful in the present invention are typically amorphous solids which are freely soluble in water or dilute acids, e.g., HCl, H250‘, citric, acetic, mandelic or fumaric. The LHRH agonist or antagonist for subcutaneous injection is supplied in vials containing 5 ml of sterile solution with the LHRH agonist or antagonist at a concentration of about 1.0 mg/ml.

A typical pharmaceutical composition of the LHRH agonist or antago- nist includes the LHRH agonist or antagonist or a pharmaceutically acceptable acid salt thereof, benzyl alcohol, a phosphate buffer (pH .0-6.5) and sterile water.

The LHRH agonist or antagonist for intramuscular or subcutaneous depot injection may be microencapsulated in a biocompatible, biodegrada- ble polymer, e.g., poly (d,l-lactide-co-glycolide) by a phase separation process or formed into a pellet. The microspheres may then be suspended in a carrier to provide an injectable preparation or the depot may be injected in the form of a pellet. See also European patent application EPA No. 58,481 published Aug. 25, 1982 for solid compositions for subder- mal injection or implantation or liquid formulations for intramuscular or subcutaneous injections containing biocompatible, biodegradable polymers ; such as lactide-glycolide copolymer and an LHRH egonist, e.g. D-Ser-t- Buo‘, Azgly*°-LHRH. These formulations permit controlled release of the peptide.

The inhibitors of 17B-HSD, 3B-HSD, aromatase and Sc-reductase are typically compounded in customary ways for oral administration, e.g., in tablets, capsules and the like. These compounds useful in the present invention are typically formulated with conventional pharmaceutical exci- pients, e.g., spray dried lactose and magnesium stearate into tablets or capsules for oral administration. The antiestrogens, when used with the invention, are typically compounded in customary ways for oral administr- ation, e.g., in capsules, tablets, as dragees or even in liquid form, e.g., suspensions or syrups. One or more of the active substances, with or without additional types of active agents, can be worked into tablets or dragee cores by being mixed with solid, pulverulent carrier substan- ces, such as sodium citrate, calcium carbonate or dicalcium phosphate, and binders such as polyvinyl pyrrolidone, gelatin or cellulose derivati- ves, possibly by adding also lubricants such as magnesium stearate, sodium lauryl sulfate, "Carbowax" or polyethylene glycols. Of course, taste-improving substances can be added in the case of oral administra- tion forms.

The therapeutically active antiestrogen compound should be present in a concentration of about 0.5-90% by weight of the total mixture, i.e., in amounts that are sufficient for maintaining the above-mentioned dosage range.

As further forms, one can use plug capsules, e.g., of hard gelatin, as well as closed soft-gelatin capsules comprising a softener or plasti- cizer, e.g. glycerine. The plug capsules contain the active substance preferably in the form of granulate, e.g., in mixture with fillers, such as lactose, saccharose, mannitol, starches, such as potato starch or amylopectin. cellulose derivatives or hightly-dispersed silicic acids. In soft-gelatin capsules, the active substance is preferably dissolved or suspended in suitable liquids, such as vegetable oils or liquid polyethy- lene glycols.

In place of oral administration, the active compounds may be admini- stered parenterally. In such case, one can use a solution of the active substance, e.g., in sesame oil or olive oil. One or more of the active substances (antiestrogen or inhibitor of 17$-HSD and 3B-HSD can be microencapsulated in or attached to a biocompatible, biodegradable polymer, e.g. poly(d,1-lactide-co-glycolide) and subcutaneously or intra- muscularly injected by a technique called subcutaneous or intramuscular depot to provide continuous slow release of the compound(s) for a period of 2 weeks or longer.

In the most preferred aspect of this invention, the LHRH agonist is [D~Trp°,des-G1y—NHz1°] LHRH ethylamide which is administered subcuta- neously in single daily dose of 500 pg for the first thirty (30) days of treatment and thereafter in a single daily dose of 250 ug: the antian- drogen is EM 101 which is administered orally in three equally divided daily doses of 250 mg; and the inhibitor of sex steroid biosynthesis is EM 139 and/or MK 906 administered orally in two equally divided doses of 50 mg every 12 hours.

The inhibitor(s) of sex steroid biosynthesis and the antiandrogen are preferably administered to a male in need of the prostate cancer treatment of this invention two to four hours before the LHRH agonist or antagonist is administered, but the at tending clinician may elect to start administration of the LHRH agonist or antagonist, the antiandrogen and the inhibitor of steroid biosynthesis simultaneously. When the antiandrogen and sex steroid inhibitor are particularly effective, both chemical (LHRH agonist or antagonist) and surgical castration may be avoided. Especially, when patients whose testes have already been surgically removed are treated according to this invention, no LHRHp agonist or antagonist need to be used but other dosages remain the same.

The terms and descriptions used herein are preferred embodiments set forth by way of illustration only, and are not intended as limitations on the many variations which those of skill in the art will recognize to be possible in practicing the present invention as defined by the following claims.

Claims (1)

1.CLAIMS: Use of an antiandrogen in the preparation of a medicament for use, together with an inhibitor of Sot-reductase activity, in the treatment of prostate cancer. Use according to claim 1, in which the antiandrogen has no agonistic activity. Use of an antiandrogen in the preparation of a medicament for use, together with an inhibitor of a 17B HSD, in the treatment of prostate cancer. Use of an antiandrogen in the preparation of a medicament for use, together with an inhibitor of 313-hydroxysteroid dehydrogenase, in the treatment of prostate cancer. Use of an inhibitor of Soc-reductase activity in the preparation of a medicament for use, together with an antiandrogen, in the treatment of prostate cancer. Use according to claim 5, in which the antiandrogen has no agonistic activity. Use of an inhibitor of a 1713-HSD, in the preparation of a medicament for use, together with an antiandrogen, in the treatment of prostate cancer. Use of an inhibitor of 3B-hydroxysteroid dehydrogenase, in the preparation of a medicament for use, together with an antiandrogen, in the treatment of prostate cancer. Use according to any of the preceding claims in which the medicament is for use together also with the inhibition of testicular hormonal secretion by surgical castration or by administration of a LHRH agonist or antagonist. is Use according to any of the preceding claims in which the medicamenyfor use together also with a compound selected from a 5a-reductase inhibitor, a 17(3- hydroxysteroid dehydrogenase inhibitor, an antiestrogen, an LHRH agonist or antagonist, or with surgical castration, where such compound or castration is not already indicated in said claim. Use of an antiandrogen according to claim 1, 3 or 4, substantially as herein described. Use of an inhibitor of 5(1—reductase activity according to claim 5, substantially as herein described. Use of an inhibitor of a 17[3—HSD according to claim 7, substantially as herein descried. Use of an inhibitor of 3 B~hydroxysteroid dehydrogenase according to claim 8, substantially as herein described. MACLACHLAN & DONALDSON, Applicants’ Agents, 47 Merrion Square, DUBLIN