TREA

Method of reducing hair growth employing sulfhydryl active compounds

Follow

Information

  • Patent Grant
  • 5411991
  • Patent Number
    5,411,991
  • Date Filed
    Tuesday, December 22, 1992
    32 years ago
  • Date Issued
    Tuesday, May 2, 1995
    29 years ago
Information
Abstract
A method of reducing the rate of mammalian hair growth includes topically applying a composition containing a sulfhydryl reactive compound to the skin.
Description

The invention relates to reducing hair growth in mammals.
Hair proteins include a fairly large quantity of the amino acid cysteine, which includes a thiol (--SH) group. It is the formation of disulfide bonds between cysteine residues in the hair proteins, to form cystine, that give hair its strength and character.
It is known in the art to use depilatory compositions to remove hair from, e.g., legs. Such compositions, when applied to the skin, digest the hair, in part, by breaking down the disulfide bonds in the hair. Such compositions typically include a chemical agent like calcium thioglycolate that aids the digestion process.
We have discovered that the rate of mammalian (including human) hair growth can be reduced by applying a non-depilatory composition including sulfhydryl active compounds to the skin. Sulfhydryl active compounds, as used herein, are compounds that include a free --SH group, thiols without a free --SH group, and thiols or disulfides that can be converted to a molecule with a free --SH group in cells. Non-depilatory, as used herein, is a composition which after a single topical application does not result in hair removal and/or degradation.
Without being bound to any theory, it is believed that sulfhydryl active compounds reduce hair growth at least in part by one or more of the following mechanisms. During hair growth, cysteine is incorporated into protein chains. The --SH groups of cysteine residues in the protein chains form disulfide bonds (and cystine), binding the protein chains together as part of the normal hair growth. Sulfhydryl active compounds, applied topically, penetrate the hair follicle and interfere with hair growth by (1) reacting with free cysteine to form a mixed cysteine-sulfhydryl active compound disulfide bond, resulting in there being less cysteine available for incorporation into disulfide bonds present in hair proteins; (2) reducing the disulfide bond in cystine in the hair proteins, at the same time forming a mixed cysteine-sulfhydryl active compound disulfide bond; and (3) reducing the disulfide bond in cystine, without concomitant formation of the mixed disulfide bond.
Preferred sulfhydryl active compounds with a free --SH group include thiosalicylic acid, D-cysteine, 2-mercaptoethylamine (cysteamine), captopril, N-acetyl-L-cysteine, cysteinylglycine, 2,3-dimercapto-1-propanesulfonic acid, meso-2,3-dimercaptosuccinic acid, dimethylcysteamine, diethyldithiocarbamic acid, D-penicillamine, L-cysteine methyl ester, and L-cysteine ethyl ester.
Preferred sulfhydryl active compounds without a free --SH group include 3,3'-thiodipropionic acid, isethionic acid, 3-carboxypropyl disulfide, 3,3'-thiodipropionic acid dilauryl ester, sulfasalazine, 3-(methythio)-propylamine, 5'-deoxy-5'-methylthioadenosine, allyl sulfide, DL-.alpha.-lipoic acid (reduced form), and DL-methionine-S-methyl-sulfonium chloride.
Preferred sulfhydryl active compounds that are converted to free thiols in cells include phosphocysteamine, which is dephosphorylated to cysteamine in cells; penicillamine disulfide, which is reduced to free penicillamine in cells; and S-2-aminoethyl-L-cysteine, which is hydrolyzed to cysteamine and serine (inactive) in cells.
The sulfhydryl active compounds should not be of too high a molecular weight (greater than about 1000 daltons), or contain highly charged phosphate groups, or compounds that may not adequately penetrate the skin.
The composition contains, in addition to the sulfhydryl active compound, a non-toxic dermatologically acceptable vehicle or carrier which is adapted to be spread on the skin. The concentration of the compound may be varied over a wide range up to a saturated solution, preferably from 1% to 20% by weight. The reduction of hair growth increases as the amount of sulfhydryl active compound applied increases per unit area of skin; the maximum amount that can be effectively applied is limited primarily only by the rate at which the compound penetrates the skin. Generally, the effective amounts range from 100 to 2000 micrograms or more per square centimeter of skin.





The following specific examples in Table 1 are intended to illustrate more clearly the nature of the present invention without acting as a limitation upon its scope. The inhibition in hair growth provided by the sulfhydryl active compounds was determined by following the general procedures described in Shander et. al., U.S. Pat. No. 5,132,293, Ahluwalia, U.S. Pat. No. 5,095,007 and Ahluwalia et. al., U.S. Pat. No. 5,096,911, both of which are hereby incorporated by reference herein.
TABLE 1__________________________________________________________________________Inhibition of Hair Growth by Sulfhydryl Reactive Compounds Hair MassCompound Dose Vehicle Treated (mg) Untreated (mg) Percent Reduction__________________________________________________________________________Thiosalicylic acid 20% B 0.18 .+-. 0.04 1.64 .+-. 0.04 89 .+-. 2%2-Mercaptoethylamine (Cysteamine) 20% A 0.30 .+-. 0.09 1.89 .+-. 0.34 86 .+-. 3%L-Cysteine methyl ester 20% A 0.28 .+-. 0.07 1.91 .+-. 0.30 86 .+-. 3%L-Cysteine ethyl ester 20% A 0.49 .+-. 0.08 2.73 .+-. 0.15 82 .+-. 3%N-Acetyl-L-Cysteine 15% A 0.39 .+-. 0.07 2.13 .+-. 0.31 80 .+-. 4%2,3,-Dimercapto-1-propanesulfonic acid 20% A 0.64 .+-. 0.08 3.08 .+-. 0.27 79 .+-. 3%Dimethylaminoethanethiol 20% A 0.34 .+-. 0.05 1.77 .+-. 0.19 78 .+-. 6%Phosphocysteamine 25% E 0.50 .+-. 0.10 1.94 .+-. 0.17 74 .+-. 4%3-Carboxypropyl disulfide 15% A 0.70 .+-. 0.14 2.63 .+-. 0.26 74 .+-. 4%3,3'-Thiodipropionic acid 20% A 0.76 .+-. 0.12 2.80 .+-. 0.25 73 .+-. 4%Diethyldithiocarbamic acid 15% A 0.65 .+-. 0.09 2.28 .+-. 0.25 68 .+-. 7%D-Penicillamine 15% A 0.57 .+-. 0.07 1.87 .+-. 0.3 65 .+-. 5%Sulfasalazine 20% C 0.88 .+-. 0.14 2.32 .+-. 0.21 61 .+-. 6%D-Cysteine 10% A 1.20 .+-. 0.17 2.92 .+-. 0.24 60 .+-. 3%5'-Deoxy-5'-methylthioadenosine 10% A 1.25 .+-. 0.17 2.97 .+-. 0.27 57 .+-. 6%Captopril 10% A 1.49 .+-. 0.20 3.50 .+-. 0.15 57 .+-. 5%DL-.alpha.-Lipoic acid (reduced form) 15% A 0.74 .+-. 0.09 1.73 .+-. 0.19 56 .+-. 6%Cystenyl-glycine 15% A 0.93 .+-. 0.18 2.26 .+-. 0.26 55 .+-. 8%D-Penicillamine disulfide 15% A 1.09 .+-. 0.23 2.36 .+-. 0.30 55 .+-. 4%Isethionic acid 15% A 1.45 .+-. 0.22 3.03 .+-. 0.31 50 .+-. 7%meso-2,3,-Dimercaptosuccinic acid 20% C 1.08 .+-. 0.16 2.23 .+-. 0.28 50 .+-. 5%3,3'-Thiodipropionic acid dilauryl ester 20% D 1.07 .+-. 0.10 2.15 .+-. 0.08 50 .+-. 4%S-2-Aminoethyl-L-cysteine 20% A 0.99 .+-. 0.20 2.15 .+-. 0.35 50 .+-. 11%3,3'-Thiodipropionic acid dilauryl ester 5% D 1.70 .+-. 0.21 2.39 .+-. 0.16 30 .+-. 7%3-(Methylthio)-propylamine 2% A 0.97 .+-. 0.13 1.27 .+-. 0.10 22 .+-. 13%Allyl sulfide 20% B 1.74 .+-. 0.16 2.22 .+-. 0.22 17 .+-. 10%DL-.varies.-Lipoic acid (reduced form) 5% B 2.67 .+-. 0.26 3.22 .+-. 0.32 16 .+-. 5%__________________________________________________________________________ Vehicles Vehicle A: 68% distilled H20, 16% ethanol (100 proof), 5% propylene glycol, 5% dipropylene glycol, 4% benzyl alcohol, 2% propylene carbonate Vehicle B: 80% ethanol (190 proof), 17.5% distilled H 20, 2% propylene glycol dipelargonate (Emerest 2388), 0.5% propylene glycol Vehicle C: Moisturizing lotion containing common cosmetic ingredients which include emulsifiers, detergents, and preservatives Vehicle D: 75% acetone, 20% propylene carbonate, 5% benzyl alcohol Vehicle E: 86% distilled H.sub.2 O, 4% propylene glycol, 4% dipropylene glycol, 4% propylene carbonate, 2% ethanol
The following biochemical properties of some of the sulfhydryl reactive compounds were tested: (1) the percent reduction in hair shaft cysteine caused by the compounds; (2) the ability of the compounds to form a cysteine-mixed disulfide in vitro; (3) the ability of the compound to form a cysteine-mixed disulfide in hair shafts; and (4) the ability of the compounds to reduce cystine.
The percent reduction in hair shaft cysteine caused by the sulfhydryl reactive compounds was measured according to the following procedure. Amino acid analysis of hamster flank organ hairs was carried out using a commercially available amino acid analysis system (Pico-Tag system, available from Waters Associates, Inc., Milford, Mass.). The hairs were thoroughly washed, then hydrolyzed by HCL vapors at 115.degree. C. overnight. The hydrolyzed hairs (now free amino acids) were derivatized with phenylisothiocyanate to yield the phenylthiohydantion derivatives of the respective amino acids, which were then separated by C-18 reverse phase chromatography (HPLC), and quantitated by an in-line UV spectrophotometer. It is believed that the reduction of cysteine levels in hair shafts caused by some of the sulfhydryl active compounds is at least in part responsible for the reduction in hair growth caused by these compounds.
The ability of the sulfhydryl reactive compounds to form cysteine-mixed disulfides in hair shafts was determined according to the following procedure. Groups of eight (8) Golden Syrian hamsters were treated topically with a sulfhydryl active compound on one flank organ (treated site) and the carrier vehicle without the sulfhydryl active compound on the other flank organ (control site). The carrier vehicles were the same as for the results achieved in Table 1. Following thirteen (13) treatments (Mon-Fri, over 18 days), hair shafts from the treated flank organs were harvested and analyzed for the presence of cysteine-mixed disulphides. It is believed that the ability of some of the sulfhydryl reactive compounds to form the cystein-emixed disulfides in the hair shaft is at least in part responsible for the reduction in hair growth caused by these compounds, as the hair shaft proteins fail to undergo final post-translational maturation (disulfide formation).
The ability of the sulfhydryl reactive compounds to form cysteine-mixed disulfides in vitro was determined by incubating the sulfhydryl reactive compounds in test tubes, with either cystine or cysteine, under physiological conditions (i.e. pH 7.4 and at a temperature of 37.degree. C.). The reaction of these compounds with cysteine or cystine was evaluated by HPLC analysis. It is believed that the ability of a sulfhydryl reactive compound to form a cysteine-mixed disulfide in vitro provides an indication that the compound is capable of forming cysteine-mixed disulfides with free cysteine present in hair follicle bulbs prior to cysteine incorporation into protein of the hair shaft when applied topically to the skin.
The ability of sulfhydryl reactive compounds to reduce cystine was determined by incubating the respective sulfhydryl compound with cystine at physiological conditions of temperature and pH (37.degree. C., pH 7.4). Following the incubation, the samples were derivatized and analyzed on HPLC as given above. For cysteamine, phosphocysteamine and dimethylcysteamine the samples were analyzed without derivatization, using an electrochemical detector instead of the UV detector used in amino acid analysis. The determination of cystine reduction by the compounds was based on generation of cysteine (free thiol) in the incubation mixture. It is believed that reducing the disulfide bond in cystine in hair proteins results in reduced hair growth.
The results of the testing of these properties are recorded in Table 2.
TABLE 2__________________________________________________________________________Biochemical Properties of Select Sulfhydryl Reactive Agents Percent reduction in Formation of Cysteine mixed disulfide ReductionSulfhydryl reactive agent hair shaft cysteine in-vitro in hair shaft of Cystine__________________________________________________________________________D-Penicillamine 50% YES YES ND*Cysteamine 50% YES YES YESDimethyl cysteamine 28% YES YES YESPhospho cysteamine 24% YES* YES* ND*Dimercaptopropanesulfonic acid 40% YES NO YESMeso-dimercaptosuccinic acid 22% NO ND* YESCaptopril 26% YES ND* YES5'-Deoxy methylthioadenosine 11% NO ND* NODiethyl dithiocarbamicacid 18% NO ND* NOThiosalicylic acid 14% NO ND* NOSulfasalazine (-2%) NO ND* NOCystienyl-glycine ND* ND* ND* YES.varies.-Lipoic acid ND* NO ND* NO__________________________________________________________________________ ND-: Not Determined
Other embodiments are within the claims.
Claims
  • 1. A process of reducing the rate of mammalian hair growth, comprising
  • selecting an area of mammalian skin from which a reduced rate of hair growth is desired; and
  • applying a non-depilatory composition including a hair growth reducing effective amount of a sulfhydryl active compound to said area of mammalian skin, said sulfhydryl active compound penetrating into the hair follicles in said area of mammalian skin to interfere with the formation of new hair causing a reduction in the rate of hair growth from said area of mammalian skin.
  • 2. The process of claim 1 wherein said compound reacts with free cysteine in hair follicle cells to form cysteine-mixed disulfides.
  • 3. The process of claim 1 wherein said sulfhydryl active compound reduces disulfide bonds in cystine in hair proteins.
  • 4. The process of claim 3 wherein said sulfhydryl active compound also forms a mixed disulfide bond with one of the cysteine moieties in hair shaft proteins.
  • 5. The process of claim 1 wherein said sulfhydryl active compound is cysteamine.
  • 6. The process of claim 1 wherein said sulfhydryl active compound is D-penicillamine.
  • 7. The process of claim 1 wherein said sulfhydryl active compound is dimethyl cysteamine.
  • 8. The process of claim 1 wherein said sulfhydryl active compound is phosphocysteamine.
  • 9. The process of claim 1 wherein said sulfhydryl active compound is captopril.
  • 10. The process of claim 1 wherein said sulfhydryl active compound is meso-dimercaptosuccinic acid.
  • 11. The process of claim 1 wherein said sulfhydryl active compound is cysteinyl-glycine.
  • 12. The process of claim 1 wherein said sulfhydryl active compound is D-cysteine.
  • 13. The process of claim 1 wherein said sulfhydryl active compound is N-acetyl-cysteine.
  • 14. The process of claim 1 wherein said sulfhydryl active compound is thiosalicylic acid.
  • 15. The process of claim 1 wherein said sulfhydryl active compound is lipoic acid.
  • 16. The process of claim 1 wherein said sulfhydryl active compound is 5'-deoxy-5'-methyl-thioadenosine.
  • 17. The process of claim 1 wherein said sulfhydryl active compound is L-cysteine methyl ester.
  • 18. The process of claim 1 wherein said sulfhydryl active compound is sulfasalazine.
  • 19. The process of claim 1 wherein said sulfhydryl active compound is L-cysteine ethyl ester.
  • 20. The process of claim 1 wherein said sulfhydryl active compound is 3-carboxypropyl disulfide.
  • 21. The process of claim 1 wherein said sulfhydryl active compound is applied to the face.
  • 22. The process of claim 1 wherein said sulfhydryl active compound has a free --SH group.
  • 23. The process of claim 1 wherein said sulfhydryl active compound is a thiol without a free --SH group.
  • 24. The process of claim 1 wherein said sulfhydryl active compound is a thiol or disulfide that can be converted to a molecule with a free --SH group in cells.
  • 25. The process of claim 1 wherein said hair growth that is reduced is androgen-stimulated hair growth.
  • 26. The process of claim 1 wherein said mammalian skin is human skin and said area of human skin to which said composition is applied is an area of skin comprising beard hair.
  • 27. The process of claim 1 wherein said composition, when tested in the Golden Syrian hamster assay, provides a reduction in hair growth of at least 16%.
  • 28. The process of claim 1 wherein said composition, when tested in the Golden Syrian hamster assay, provides a reduction in hair growth of at least 30%.
  • 29. The process of claim 1 wherein said composition, when tested in the Golden Syrian hamster assay, provide a reduction in hair growth of at least 50%.
  • 30. The process of claim 1 wherein said non-depilatory composition further comprises a non-toxic, dermatologically acceptable vehicle.
  • 31. The process of claim 30 wherein said composition comprises between 1% and 20% of said sulfhydryl active compound by weight.
US Referenced Citations (31)
Number Name Date Kind
3426137 Philpitt et al. Feb 1969
4039669 Beyler et al. Aug 1977
4098802 van der Vies Jul 1978
4139638 Neri et al. Feb 1979
4161540 Neri et al. Jul 1979
4191775 Glen Mar 1980
4207315 Voorhees et al. Jun 1980
4228163 Bliss Oct 1980
4269831 Ferrari et al. May 1981
4272508 Tamm Jun 1981
4310523 Neumann Jan 1982
4344941 Wiechert et al. Aug 1982
4367227 Bingham Jan 1983
4370315 Greff et al. Jan 1983
4439432 Peat Mar 1984
4456586 Van der Berghe et al. Jun 1984
4457925 Bittler et al. Jul 1984
4463016 Burgess Jul 1984
4525344 Tutsky Jun 1985
4684635 Orenstresch et al. Aug 1987
4720489 Shander Jan 1988
4775530 Perricone Oct 1988
4885289 Breuer et al. Dec 1989
4912120 Castelhano et al. Mar 1990
4929630 Castelhano et al. May 1990
4935231 Pigiet Jun 1990
4944939 Moore Jul 1990
5095007 Ahluwalia Mar 1992
5096911 Ahluwalia et al. Mar 1992
5143925 Shander et al. Sep 1992
5362748 Schwen et al. Nov 1994
Foreign Referenced Citations (8)
Number Date Country
2840144 Mar 1980 DEX
53-127432 Feb 1978 JPX
58-57308 Apr 1983 JPX
61-210021 Sep 1986 JPX
61-289016 Dec 1986 JPX
63-243017 Oct 1988 JPX
1458349 Dec 1976 GBX
9110421 Jul 1991 WOX
Non-Patent Literature Citations (74)
Entry
Plewing, The Journal of Investigative Dermatology, 62:308-315 (1974).
Chemical Abstracts 111:120611g, 1989.
Chemical Abstract 118(14):131764e, 1992.
Gahl et al., Biochem. J., 228:545-550 (1985).
Theone et al., J. Clin. Invest., 58:180 (1976).
Maiorino et al., The J. of Pharmacology and Experimental Therapeutics, 259:808 (1991).
Walshe, Clinical Studies, pp. 487-495 (Oct. 1956).
Levine, Nature, 187:940 (1960).
Schneider, NE J. Med., 313:1473 (1985).
Porter et al., Adv. Enz. Res., 27:57-59 (1988).
Pegg, Cancer Res., 48:759-74 (1988).
Luk et al., Am. J. Physiol., 254:G194-G200 (1988).
Alhonen-Hongisto et al., Biochem. Biphys. Res. Comm., 144:132-137 (1987).
Casero et al., Cancer Res., 47:3964-67 (1987).
Henry et al., Br. J. Derm., 105:33-34 Supplement 20 (1981).
Luk et al., Cancer Res., 42:3070-3073 (1982).
Rupniak et al., Eur. J. Cancer Clin. Oncol., 18:1353-9 (1982).
Peterson et al., Biochem. Biophys. Acta., 657:268-276 (1981).
Kousa et al., Acta Dermatovener, 62:221-224 (1982).
McCullough et al., J. Invest. Dermatol., 85:518-521 (1985).
McCullough et al., J. Invest. Dermatol., 81:388-392 (1983).
Splinter et al., Eur. J. Cancer Clin. Oncol., 22:61-67 (1986).
Ebling J. of Investigative Dermatology, 67:98-106 (1976).
Cardo et al., Hair Research 244-250 (1981).
Lucky, Arch Dermatol., 121:55-56 (1985).
Lucky et al., J. Investig. Dermatology, 86:83-86 (1986).
Goldbarg, "A Method for the Colorimetric Determination of Gamma-Glutamyl Transpepidase in Human Serum; Enzymatic Activity in Health and Disease", 44:2:127 (1963).
Minato, Arch. of Biochemistry and Biophysics, 192:235-240 (1979).
Gardell et al., Febs Letts, 122:2:171-174 (1980).
Reed et al., Biochemistry and Biophysical Research Communications, 94:4:1273-1277 (1980).
Kim et al., J. of Dermatology 6:39-45 (1979).
Kaszynski, Brit. J. Dermatology, 109:565-569 (1983).
Richards et al., Cancer Research, 42:4143-4151 (1982).
Chase et al., Physiological Zoology, 24:1-8 (1951).
De Young et al., Cancer Research, 38:3697-3701 (1978).
Kinoshita et al., Bull. Chem. Soc. Jpn., 54:2219-2220 (1981).
Chem. Abst. 95:143848, p. 20 (1981).
Gale et al., Biochem. Pharmacology 17:2495-2498 (1968).
Jayaram et al., Biochem. Pharmacol., 24:1787-1792 (1975).
Cooney et al., Int. J. Biochem. 11:519-539 (1980).
Van Scott et al., The Journal of Investigative Dermatology, vol. 27 pp. 405-428 (1956).
Rieger, Cosmetics and Toiletries, 101:63-66 (1986).
Downing et al., J. Am. Acad. Dermatol., 14:2:221-222 (1986).
De Young, The Journal of Investigative Dermatology, 82:3:275-279 (1984).
Marsen et al., Pharmacology of the Skin II, Chapter 35, pp. 473-481.
Mills et al., Cosmetics and Toiletries, vol. 104, (1989).
Tyms, The Physiology of Polyamines, vol. II, Chapter I, pp. 4-33 (1989).
Spencer, Cosmetics & Toiletries, 100:47-49 (1985).
Dunn, AFP, 39:3:169-174 (1988).
Kligman et al., Arch. Dermatol., 107:551-552 (1973).
Brown, Cutis, 32:373-375 (1983).
Splinter et al., Eur. J. Cancer and Clin. Oncol., 22:61-67 (1986).
Matthews et al., NPha Journal, pp. 6-12 (Jan. 1982).
Ogawa et al., Curr. Prob. Dermatol., 11:159-170 (1983).
Martinent et al., J. Biol. Chem. 263:4236-4241 (1988).
Folk et al., Adv. Enzymol., 38:109-191 (1973).
Chung et al., Proc. Natl. Acad. Sci. U.S.A., 69:303-307 (1972).
Harding et al., Biochemistry, 11:2858-2863 (1972).
Harding et al., Biochemistry, 10:624-630 (1971).
Goldsmith, Hair Research, pp. 29-35 (1981).
Hattori et al., J. of Dermatology, 10:45-54 (1983).
Killackey et al., Molecular Pharmacology, 35:701-706 (1989).
Scott et al., Transactions, 15:1167-1168 (1987).
Straile, Biology of the Skin and Hair Growth, pp. 35-57 (1965).
Heby, The Physiology of Polyamines, 1:5:83-94 (1988).
Ogawa et al., J. Invest. Dermatol., 68:32-35 (1977).
Chem. Abstracts, vol. 100 (1984) 172302z Ogawa et al.
Burdick et al., Br. J. Derm. (1970) 82, Supplement 6.
Girard et al., Arch. Dermatol. Res. 269-281-290 (1980).
Goos et al., Arch. Dermatol. Res. (1982) 273:333-341.
Simpson et al., "Bristish Journal of Dermatology", 100:687-692 (1979).
Theone et al., Brief Clin. and Lab. Observations, 96:1043-44 (1980).
Kanerva et al., Arch. Toxicol. Suppl (9)455-59 (1986).
Pegg et al., The American Physiological Society, pp. C212-C221 (1982).