COSMETIC AND/OR DERMATOLOGICAL COMPOSITION FOR COLOURING THE SKIN

Abstract

The invention relates to a composition which contains an aqueous solution of certain elements of a family of sterol derivatives, which enable improved tanning of the skin due to considerable penetration of the molecules thereof. Preferably, the composition also contains an ionic solution of cationic association complexes constituting an acid amphiphilic carrier.

Claims

1.-20. (canceled)

21. Appropriately applicable cosmetic composition to ensure tanning of the skin of a human subject, with or without irradiation with ultraviolet rays, containing, in a cosmetically acceptable vehicle, an aqueous solution of at least one compound of formula (I): ##STR00005## wherein R.sub.1 designates a hydrogen atom or R.sub.10—CO, where R.sub.10 represents H, CH.sub.3 or C.sub.2H.sub.5, R.sub.2 represents hydrogen or OH, R.sub.3 represents X—(CH.sub.2).sub.n—Y, where n is an integer from 1 and 4, X represents S, O or NH, and Y represents NH.sub.2, imidazol-5-yl, indol-3-yl, piperidin-2-yl, piperidin-3-yl, piperidyn-4-yl, piperazin-2-yl, piperazin-3-yl, pyridin-2-yl, pyridin-3-yl or pyridin-4-yl, R.sub.4 represents hydrogen or OH in position 20, 22, 24, 25, 26 or 27 of the ring shown above in formula (I), wherein OH is positioned so as to obtain an R or S asymmetric centre, Z.sub.1 and Z.sub.2 represent the possibility of having single or double bonds between carbons C7 and C8, on the one hand, and carbons C22 and C23, on the other hand, T.sub.1, T.sub.2, T.sub.3 are, independently from one another, H or CH.sub.3 in α or β, T.sub.4 is H, CH.sub.3 and/or C.sub.2H.sub.5 positioned to form an R or S asymmetric centre, characterized in that it contains an ionic solution of catanionic mixture complexes, where each molecule is formed by a molecule of formula (I) and one or two molecules of a carrier T which is a bolaform surfactant derived from sugar comprising an acid function within its structure and which is obtained by at least one acid-base reaction carried out between the acid group of a carrier (T) and an amino group of substituent R.sub.3 of the carbon in position 6 of the compound of formula (I).

22. Composition according to claim 21, characterized in that it contains a mixture of both compounds of formula (I) wherein R.sub.1=R.sub.4=T.sub.1=T.sub.2=T.sub.3=H, R.sub.2=OH, R.sub.3=NH—(CH.sub.2).sub.2-imidazol-5-yl and T.sub.4=CH.sub.3 or C.sub.2H.sub.5.

23. Composition according to claim 21, characterized in that it contains 0.01 to 500 g/L of compound(s) of formula (I).

24. Composition according to claim 21, characterized in that it contains at least one tanning compound other than compound(s) of formula (I).

25. Composition according to claim 24, characterized in that the tanning compound(s) it contains, independently from the compound(s) of formula (I), is dihydroxyacetone and/or erythrulose and/or at least one water-soluble dye.

26. Composition according to claim 21, characterized in that it contains at least one melanogenesis activator compound other than the compound(s) of formula (I) selected from the group consisting of substrates for melanin biosynthesis and biological activators for melanogenesis able to act by stimulating melanin synthesis and/or the transfer of melanosomes from melanocytes to keratinocytes.

27. Composition according to claim 26, characterized in that the melanogenesis activator it contains, independently from the compound(s) of formula (I), is chosen from the group consisting of L-tyrosine or derivatives thereof such as N-acetyl-L-tyrosine, L-dihydrophenylalanine, aliphatic diols such as propylene glycol, cyclic diols, adenosine-1 receptor agonists, adenosine-2 receptor agonists, α-hydroxyacids and derivatives thereof, β-hyroxyacids and derivatives thereof, retinoids and derivatives thereof, pro-opiomelanocortic peptides, α-MSH or its analogs, MC1R receptor agonists, cAMP analogs, psoralens, PAR-2 receptor activity activators.

28. Composition according to claim 21, characterized in that it is applied to the skin in an amount between 0.0001 and 100 mg/cm.sup.2/day of compound(s) of formula (I).

29. Composition according to claim 21, characterized in that the carrier (T) acid function is selected from the group made up of carboxylic acid COOH, sulfuric acid O—SO.sub.3H, sulfonic acid SO.sub.3H, phosphoric acid O—P(O)(R.sub.5O)OH, wherein R.sub.5 is a C.sub.1-C.sub.6 alkyl group, phosphonic acid O—P(O)R.sub.6OH and phosphinic acid P(O)R.sub.6OH, wherein R.sub.6 is H or a C.sub.1-C.sub.6 alkyl group.

30. Composition according to claim 21, characterized in that the sugar derivative surfactant is a monosaccharide or polysaccharide derivative.

31. Composition according to claim 30, characterized in that the sugar derivative is a glucose or lactose derivative.

32. Composition according to claim 21, characterized in that the sugar acid derivative comprises a sugar structure on which a linear or branched aliphatic chain (CH.sub.2).sub.p is bonded by an NH group, of which the end opposite to the sugar structure carries an acid group, p being an integer having a value from 4 to 10.

33. Composition according to claim 21, characterized in that the ratio of the weight amounts A of compound(s) of formula (I) and B of carrier(s) (T) is between 0.001 and 1000.

34. Composition according to claim 21, characterized in that it contains from 0.01 to 150 g of the totality of components A and B per litre of composition.

35. Composition according to claim 21, characterized in that it contains at least one adjuvant selected from the group consisting of at least one thickener and/or water-soluble dye and/or fragrance and/or alcohol and/or vitamin and/or emulsifier, used alone or in mixture with optionally a co-emulsifier and/or oil or another fat and/or preservative and/or antioxidant and/or bactericide.

36. Composition according to claim 21, characterized in that it contains at least one chemical or physical sun filter, or a mixture of such filters.

37. Composition according to claim 21, characterized in that it is packaged as nano capsules or nanosized vesicles suspended in a liquid medium.

38. Composition according to claim 21, characterized in that it is packaged in the form of hydrogels, creams, lotions, emulsions or aerosols.

Description

[0040] In the drawings:

[0041] FIG. 1 shows the IR spectrum for the product obtained in Example 3;

[0042] FIG. 2 shows the NMR spectrum for the product obtained in Example 3;

[0043] FIG. 3 shows the results obtained in Example 5;

[0044] FIG. 4 shows the results obtained in Example 6;

[0045] FIGS. 5a, 5b, 5c show a visualization of melanosomes in cells treated according to Example 7;

[0046] FIG. 6 shows the result of treatment according to Example 8 for gene expression in treated cells;

[0047] FIG. 7 shows the result of treatment according to Example 9 in modulating proteins, this result being visualized by “Western Blot” technique;

[0048] FIGS. 8 and 9 show the result of treatment with compositions in accordance with the invention on reconstituted skin;

[0049] FIG. 10 shows the result of treatment according to Example 10 in modulating proteins involved in melanogenesis;

[0050] FIG. 11 shows the quantities of melanin synthesized on a reconstituted skin sample after application of a composition according to Examples 12 and 13, wherein said quantities and skin samples are defined as described in Example 10.

EXAMPLE 1: SYNTHESIS OF THE COMPOUND OF FORMULA (I) WHEREIN T.SUB.4.=H AND Z.SUB.1.=Z.SUB.2.=SINGLE BOND

[0051] The process described below is extracted from the published patent application WO03/089449. The compound (hereinafter referred to as DDA) corresponds to the systematic name: 5α-hydroxy-6β-[2-(1H-imidazol-4-yl)ethylamino]cholestan-3β-ol. [0052] a) Preparation of 5,6-α-epoxycholestan-3β-ol:

[0053] Meta-chloro-peroxybenzoic acid (0.73 g, 4.25 mmol, purity of 70-75% by weight) was dissolved in methylene chloride (10 ml) and added dropwise, under stirring, to a mixture of cholesterol (1 g, 2.5 mmol) dissolved in methylene chloride (25 ml). Stirring was maintained overnight. The reaction mixture was washed with aqueous sodium sulfite solution (10% by weight) and sodium hydrogen carbonate (5% by weight) and a saturated solution of a mixture of sodium chloride and potassium chloride. The organic phase was dried over anhydrous magnesium sulfate. Vacuum evaporation of the organic solvent gave 0.7 g of white needles (70% yield).

[0054] The proportion of α and β epoxide isomers was determined by proton NMR: 78% of α-epoxide, 22% of β-epoxide were found.

[0055] Characterization of the product: .sup.1H NMR (200 MHz, MeOD) δ ppm 2.89 (d, 1H, J=4.37 Hz, H-6); 3.04 (d, J=2.43 Hz, H-6) 3.91 (m, 1H, H-3); MS DCI/NH.sub.3MH.sup.+ 403] DCI/MNH.sub.4.sup.+, m/z: 403 [MNH.sub.4].sup.+. The α and β isomers were separated by liquid chromatography on silica (toluene/ethyl ether 85/15). The α isomer had a melting point Mp=141-142° C.; the β-isomer had a melting point Mp=131-132° C.

[0056] To complete characterization, thin layer chromatography was performed (ethyl acetate); we obtained: Rf=0.69 (brown colour after developing with a mixture of sulfuric acid-methanol).

[0057] b) Synthesis of the amino sterol from the α-epoxy-sterol obtained in step a)

[0058] Lithium perchlorate (0.75 mmol) and an amine in its basic form (1 mmol), namely, 2-(1H-imidazol-4-yl)-ethylamine, were dissolved in anhydrous ethanol (1 ml). This solution was added under an argon stream to an ethanol solution (3 ml) of the α-epoxy-sterol obtained according to a) above (100 mg, 0.25 mmol). The reaction mixture was stirred and refluxed for 6 days. Progress of the reaction was monitored by thin layer chromatography (TLC). The solvent was removed by evaporation and the residue was washed with ethyl ether (5×3 ml) and hexane (5×20 ml). The residue was dissolved in water and acidified with 2M HCl (2 ml).

[0059] The solution was pre-purified on a grafted silica cartridge (“sep-pack cartridge C18 RP”, 500 mg, Waters); excess polyamine was removed by flushing water on the cartridge (5 ml); the product was eluted with 1/1 CH.sub.3CN/H.sub.2O (5 ml). The product was purified by reverse phase HPLC using a linear gradient of a starting mixture of 95/5/0.1 H.sub.2O/CH.sub.3CN/TFA to 95/5/0.1 CH.sub.3CN/H.sub.2O/TFA achieved over 60 minutes (flow rate=1 ml/min; X=210 nm). The fraction of interest was purified again under isocratic conditions using a mobile phase consisting of a mixture of 44% of (95/5/0.1 CH.sub.3CN/H.sub.2O/TFA) 56% of (95/5/0.1 H.sub.2O/CH.sub.3CN/TFA) (flow rate=1 ml/min; λ=210 nm).

[0060] The product obtained was first characterized by TLC (methanol). Then high performance chromatography (HPLC) was performed on a “Perkin-Elmer LC200 Series” device equipped with “Ultrasep ES100RP10” column (6 μm particles), 250 mm length and 8 mm diameter, manufactured by “Bischoff”.

[0061] HPLC profile: 44% B #=220 nm rt=44-50 min

[0062] Characterization of the product: ESI-MS, m/z 514.5 [M+H].sup.+.

EXAMPLE 2: SYNTHESIS OF COMPOUNDS OF FORMULA (I) WHEREIN T.SUB.4.=CH.SUB.3./C.SUB.2.H.SUB.5 .(70/30 MIXTURE) AND Z.SUB.1.=Z.SUB.2.=SINGLE BOND

[0063] A mixture of sitosterol and campesterol (70/30 by weight) was used as sterol, in step a) of Example 1. For the reaction on the obtained α-epoxysterol, the same amine as in Example 1 step b) was used.

[0064] A mixture of the 2 following compounds was obtained:

[0065] 5α-hydroxy-6β-[2-(1H-imidazol-4-yl)ethylamino]sitostan-3β-ol and

[0066] 5α-hydroxy-6β-[2-(1H-imidazol-4-yl)ethylamino]campestan-3β-ol.

[0067] The product obtained (hereinafter referred to as “AF130”) was characterized by TLC (ethyl acetate): Rf=0.69

Characterization of the product:

[0068] ESI-HRMS m/z: 528.8323 [M+H]+(Δm=0.3 mDa) (campesterol derivative) and 524.8590 [M+H]+(Δm=0.4 mDa) (sitosterol derivative)

EXAMPLE 3

[0069] a) Preparation of the amphiphilic carrier used to prepare the catanionic mixture complex implemented in the subsequent examples. Lactobionic acid was directly reacted with 8-aminooctanoic acid (see Patent Publication WO 2011/039379).

[0070] 1) Synthesis of sodium 8-lactobionamidooctanoate

[0071] To a solution of sodium hydroxide (300 mg, 5.59 mmol) in 50 mL of methanol were successively added 8-aminooctanoic acid (888 mg, 5.59 mmol) and lactobionic acid (2.00 g, 5.59 mmol). The mixture was stirred at 50° C. for 24 h; the solvent was then evaporated under reduced pressure; the residue obtained was purified by chromatography column on silica gel (eluent: CHCl.sub.3/CH.sub.3OH/H.sub.2O: 2.5/7/0.5, Rf=0.8). A white solid was collected at a yield of 56%.

[0072] Characterization of the product:

[0073] IR(neat) cm.sup.−1: 1643 (v.sub.c=o (amide)st);

[0074] 1547 (v.sub.c=o (carboxylate) asymmetric);

[0075] 1405 (v.sub.c=o (carboxylate) symmetric)

[0076] ESI-MS, m/z: 498 [M+Na].sup.+.

[0077] The product obtained has the following formula:

##STR00002##

[0078] 2) Synthesis of 8-lactobionamidooctanoic acid

[0079] To a solution of sodium 8-lactobionamidooctanoate (1.00 g, 2 mmol) in 30 mL of H.sub.2O was added approximately 2 g of proton exchange resin (Dowex 50WX8). The reaction mixture was stirred for 2 h at room temperature, then filtered and concentrated. The residue obtained was purified by column chromatography on silica gel (eluent: acetone/H.sub.2O: 9/1; Rf: 0.5). A white solid was collected at a yield of 57%.

Characterization of the product:

[0080] .sup.1H NMR (300 MHz, MeOD) δ ppm: 1.05-2.15 (m, 10H, CH.sub.2β, CH.sub.2γ, CH.sub.2δ, CH.sub.2ε, CH.sub.2ζ); 2.17 (t, 2H, CH.sub.2α); 3.12 (m, 2H, CH.sub.2η); 3.46-4.12 (m, 10H, CH and CH.sub.2 of the sugar unit); 4.28 (m, 1H, H) 4.30 (m, 1H, H alpha of CONH); 4.54 (d, J=9 Hz, 1′H, anomeric H)

[0081] IR(neat) cm.sup.−1: 1645 (v.sub.c=o (amide) st);

[0082] 1726 (v.sub.c=o (acid) st)

[0083] ESI-HRMS, m/z: 522.2162 [M+Na].sup.+ (Δm=0.1 mDa).

[0084] The product obtained is called L7 and is represented by the following formula:

##STR00003## [0085] b) Preparation of a catanionic mixture complex between the amphiphilic carrier of step a2) of this example and the product of Example 1.

[0086] To a solution of 8-lactobionamidooctanoic acid (330 mg 0.66 mmol) in 30 mL of deionized H.sub.2O was added 339 mg of the product of Example 1 (0.66 mmol). The reaction mixture was then stirred at room temperature for 24 h. This gave a homogeneous solution which, after concentration, quantitatively gave the product represented by the below formula:

##STR00004##

[0087] The resulting product is a pale yellow powder; it is hereinafter referred to as L7DDA as it consists of a L7 molecule combined with a DDA molecule.

Characterization of the product obtained:

[0088] .sup.1H NMR (300 MHz, MeOD) 5 ppm: 0.75 (s, 3H, CH.sub.3(19)); 0.89 (m, 3H, CH.sub.3); 0.91 (m, 3H, CH.sub.3); 1.05-2.15 (m, 45H, CH.sub.2β, CH.sub.2γ, CH.sub.2δ, CH.sub.2ε, CH.sub.2ζ, 35H for CH and CH.sub.2 of DDA); 2.21 (t, 2H, CH.sub.2α); 3.14 (m, 2H, CH.sub.2η); 3.42-4.10 (m, 12H, CH and CH.sub.2 of the sugar unit, +CH.sub.3 and CH.sub.6); 4.21 (m, 1H, H); 4.34 (m, 1H, H alpha to CONH); 4.50 (d, J=9 Hz, 1H, anomeric H); 6.92 (s, 1H, C=CH(NH); 7.80 (s, 1H, HN—CH=N).

[0089] The NMR spectrum is provided in FIG. 2; it shows the formation of the ion pair which combines an L7 molecule and a DDA molecule. The chemical shift of CH.sub.2 group alpha to a carboxylic acid moiety COOH is different from the group alpha to a carboxylate group COO.sup.−; in this example, CH.sub.2—COOH has a chemical shift of 2.17 ppm while CH.sub.2—COO.sup.− has a chemical shift of 2.21 ppm.

[0090] IR(neat) cm.sup.−1: 1643 (v.sub.c=o (amide) st); 1549 (v.sub.c=o (asymmetric carboxylate)); 1403 (v.sub.c=o (symmetric carboxylate)).

[0091] The IR spectrum, provided in FIG. 1, shows that step b) causes the disappearance of the carboxylic acid function characteristic band between 1800 and 1650 cm.sup.−1 in favour of two new bands in the 1610-1550 cm.sup.−1 region (asymmetric elongation of COO.sup.− (carboxylate group)) and 1450-1400 cm.sup.−1 (symmetric elongation of COO.sup.− (carboxylate group)). Thus, in FIG. 1, the disappearance of the characteristic band of the carboxylic acid function characteristic band at 1726 cm.sup.−1 and the appearance of symmetrical and asymmetrical elongation bands of the carboxylate group at 1549 cm.sup.−1 and 1403 cm.sup.−1, respectively can be observed.

[0092] CAC (Critical Aggregation Concentration) (aqueous solution, 25° C.): 2.6×10.sup.−5M.

EXAMPLE 4

[0093] The same process as for step b) of Example 3 can be used to form a combination complex between an amphiphilic acid carrier according to Example 3a2) and any compounds of formula (I) as all these compounds comprise at least one NH group allowing bonding with the carrier acid function. In particular, a complex mixture was obtained by combining the product of Example 2 with that of Example 3a2): this mixture was hereinafter named L7AF130.

[0094] The carrier/active component assembly allows to combine a positive ionization group of the active component with the acid group of the carrier. Therefore, the active component can be combined to the carrier by the R.sub.3 substituent carried by carbon 6 of the compound of formula (I). In the case of AF130 or DDA active components, we can combine two L7 carrier molecules on two amino functions of the R.sub.3 substituent. From the process for obtaining Example 3b, mix in water at room temperature, two equivalents of L7 molecule for one equivalent of active component, as described for example 3b. Once again, the mixture was initially a suspension but became a clear solution, indicating that the resulting complex, hereinafter named (L7).sub.2(AF130) or (L7).sub.2(DDA) depending on the active component, was water soluble.

EXAMPLE 5: STIMULATION OF THE SYNTHESIS OF MELANIN WITH A COMPOUND OF FORMULA (I) NAMED DDA AND A COMBINATION COMPLEX ACCORDING TO EXAMPLE 3A2)

[0095] Quantification of synthesized melanin by healthy murine melanocytes was performed according to the protocol described by Ando et al. (J. Lipid Res., 1999, 40, 1312).

[0096] Cells were seeded and treated for 24 h with the test product or the used vehicle (ethanol) and with, as a positive control, exposure to a dose of 20 mJ/cm.sup.2 of ultraviolet radiation.

[0097] 5 Million cells were isolated after centrifugation at 1500 rpm for 5 min at 4° C. The pellet was washed twice with PBS and then transferred into an Eppendorf tube and centrifuged at 5000 g for 5 min. The supernatant was removed. 200 μL of water and 1 mL of EtOH/ether (1/1) were added (melanin was insoluble in this mixture). After 15 min at room temperature, the totality was again centrifuged at 5000 g for 5 min; the supernatant was removed. The pellet was then taken up with 300 μL of a solution of NaOH(1M) in H.sub.2O/DMSO 90/10 and placed at 80° C. for one hour. Absorbance was measured at 470 nm. The amount of synthesized melanin was expressed based on the control (=100%).

[0098] The results are shown in FIG. 3. It shows that the addition of a DDA compound of formula (I), with or without carrier, results in an increase of the synthesis of melanin in the investigated cells.

EXAMPLE 6

Study of the Synthesis of Melanin by Studying the Stimulation of Tyrosinase Activity

[0099] The study was conducted on healthy murine melanocytes. The results were compared with those obtained with a positive control subjected to a dose of 20 mJ/cm.sup.2 of ultraviolet radiation. The cells were treated for 24 h with either the vehicle used (ethanol) or with the test product. The tyrosinase activity was quantified according to the protocol described by Ando et al. (J. Lipid Res. 1999, 40, 1312) as explained below.

[0100] 5 Million cells were isolated after centrifugation at 1500 rpm for 5 min at 4° C. The pellet was washed twice with PBS and then transferred into an Eppendorf tube and centrifuged at 5000 g for 5 min. The supernatant was removed. 1 mL of 0.5% by mass sodium deoxycholate solution was added (cell lysis). After 15 min at 0° C., 3 mL of a solution of 0.1% by mass of L-DOPA in 0.1M phosphate buffer (pH 6.8) were added. The whole was placed at 37° C. for 10 min. Tyrosinase activity was spectrophotometrically analysed by following the oxidation of L-DOPA to DOPAchrome. Absorbance was measured at 475 nm. The tyrosinase activity was expressed based on the control (=100%), which determines the cell basal tyrosinase activity.

[0101] The results are illustrated in FIG. 4. It shows that the tyrosinase activity in cells increased when cells were treated with a composition containing the DDA active component, with or without L7 carrier or containing AF130 active component combined, for each molecule, with two molecules of L7 carrier, with respect to the control. It also shows that an increase in tyrosinase activity is associated with an increase in melanin synthesis in the cell.

EXAMPLE 7: STUDY OF THE SYNTHESIS OF MELANIN BY MELANOSOME VISUALIZATION

[0102] Healthy murine melanocytes were treated as described in Example 6 by using untreated cells or cells treated with 1 μM of AF130 or 1 μM of (L7).sub.2AF130. The melanin synthesis was visualized by staining according to the DAPI technique: the nuclei of cells fluoresce in blue and, by contrast, melanosomes are highlighted, which are visualized in black. FIG. 5a corresponds to the visualization of untreated cells, FIG. 5b corresponds to the visualization of cells treated with 1 μM of AF130 and FIG. 5c corresponds to the visualization of cells treated with 1 μM of (L7).sub.2AF130: it is observed that the quantity of melanosomes and, therefore, melanin synthesis is greatly enhanced by treatment according to example 6 (comparison with FIG. 5a).

[0103] The DAPI technique is performed as follows: cells are seeded on previously sterilized slides by washing with ethanol; they are treated with the studied active molecule or with a vehicle (ethanol).

[0104] After 24 hours of treatment, cells were fixed using a formaldehyde solution diluted to one tenth (3.7% by weight) in PBS for 15 min at room temperature. Formaldehyde was then removed and the cells were washed with PBS. 10 μl of a DAPI solution to 1/500.sup.th in Mowiol (mounting solution) were deposited on a slide. The cover slip was placed on the drop, cells being present between the slide and the cover slip. The slides were placed at 4° C. overnight before being observed. For each sample, an image in “DAPI” mode was performed, only allowing visualization of nuclei as well as the same image in “visible” mode. The two images were then superimposed.

EXAMPLE 8

[0105] This example shows in healthy murine melanocytes, that treatment with compositions according to the invention allows to increase the expression of genes corresponding to tyrosinase and TRP-1 and TRP-2 enzymes (TRP=Tyrosinase Related Protein), which are involved in melanogenesis.

[0106] Cells were seeded and treated for 24 h with the molecules the action of which we want to study, that is to say here, with DDA (1 μM), on the one hand, and with L7DDA (0.1 or 1 or 2.5 or 5 μM) on the other. The results were compared with irradiated ultraviolet cells as in Example 6. FIG. 6 shows, as ordinate, the expression of genes corresponding to tyrosinase, TRP-1 and TRP-2.

[0107] To quantify the expression of these genes, RNA extraction from cells was performed. Melanocytes were treated for 24 h with the active molecule or the control agent. 1 mL of Trizol® was added; after 5 min at room temperature, the totality was placed in an Eppendorf tube. 200 μL of CHCl.sub.3 were added at 4° C. The Eppendorf tubes were stirred manually, by turning them during 15 sec, left for 5 min at room temperature and then centrifuged at 16000 g at 4° C. for 10 min. The colourless aqueous phase was isolated. 500 μL of isopropanol (−20° C.) were added. The Eppendorf tubes were stirred manually, by turning them during 15 sec, left for 15 min at room temperature and then centrifuged at 16200 g at 4° C. for 10 min. The supernatant was removed. The pellet was washed with 1 mL of 75% ethanol (−20° C.). After centrifugation at 16000 g at 4° C. for 5 min, the supernatant was removed. 10 min after drying, the pellet was resuspended with 30 μL of RNAase-free water. The quantity and purity of RNA were estimated by spectrophotometry (230, 260 and 280 nm).

[0108] A RT-qPCR was performed; in an Eppendorf tube, were added: 1 μL of reverse transcriptase, 4 μL of 5× reaction mixture “iScript®5×”, the amount of RNAase-free water needed to reach a total volume of 20 μL and the corresponding volume for 1 μg of RNA. The Eppendorf tubes were then vortexed, centrifuged for a few seconds and then placed in the thermocycler (program: 5 min at 25° C., then 30 min at 42° C., then 5 minutes at 85° C. and then back to 4° C.)

[0109] An amplification was then performed. The reference genes were: glyceraldehyde 3-phosphate dehydrogenase and Cyclophilin A1. Genes of interest were: Tyrosinase, TRP-1 and TRP-2. For each gene (reference or of interest), a mixture was prepared with RNAase-free water, Sybr Green® and the corresponding primer.

[0110] The resulting cDNAs were taken up with 180 μL of RNAase-free water. 5 μL of cDNA were added at the bottom of each well. 20 μL of mixture were added on the edge of each well. The plate was then covered with an adhesive plastic and centrifuged at 4000 rpm until no more bubbles were observed.

[0111] The plate was then placed in the thermal cycler: 95° C. for 3 min, followed by 50 amplification cycles of 15 sec at 95° C. and one minute at 60° C. At the end of these 50 cycles, the melting curves were generated at 95° C. for 1 min and 95° C. for 10 sec (80 cycles). One can thus refer, in FIG. 6, to the stimulation of gene expression for the different tested products. The digital results are provided in the table below.

TABLE-US-00001 ΔΔCT ΔΔCT ΔΔCT (tyrosinase) (TRP-1) (TRP-2) L7DDA 0.1 μM 4.98 13.93 9.57 L7DDA 1 μM 5.76 14.00 7.75 L7DDA 2.5 μM 6.83 16.58 12.13 L7DDA 5 μM 10.25 13.53 13.47 DDA 1 μM 6.09 13.45 6.97 UV 20 mJ/cm.sup.2 2.99 3.54 2.83

[0112] It was found that the treatment of cells with DDA and L7DDA products provided results showing that the enzymes involved in melanogenesis are stimulated as much as with UV irradiation.

EXAMPLE 9: EFFECT ON THE MODULATION OF PROTEINS INVOLVED IN MELANOGENESIS (WESTERN BLOT)

[0113] In this example, the test treatment was carried out on healthy murine melanocytes. Treatments were performed with 1 μM of the DDA compound and also with 1 μM of L7DDA and (L7).sub.2DDA and (L7).sub.2AF130 compounds. The positive control was carried out with cells that had received a dose of 20 mJ/cm.sup.2 of UV radiation. The reference protein was actin (43KDa). After 24 hours of treatment, cells were scraped into cold PBS (4° C.) and then centrifuged at 1500 rpm at 4° C. for 5 min. The supernatant was removed.

[0114] The pellet was taken up with 100 μL of lysis buffer (0.1M of TRIS-HCl, pH=7.4, 1% Igepal, 0.01% SDS, to which mixture were added protease inhibitors (1% by volume of the mixture)) and vortexed for several seconds. After 30 min at 4° C., the mixture was vortexed again and subjected to ultrasound for 5 sec. The Eppendorf tubes were finally centrifuged at 10000 rpm at 4° C. for 10 min. The supernatant (=protein extract) was transferred to a new Eppendorf tube. A Bradford assay was performed to quantify the proteins.

[0115] Based on the results of this assay, samples were prepared for deposit on SDS-PAGE gel (samples prepared at 1 μg/μL): 10 μL, i.e. 10 μg, of proteins were deposited for each sample.

[0116] After gel transfer in liquid phase of the proteins on a polyvinylidene fluoride membrane, membranes were incubated with the primary antibodies of interest (Tyrosinase: 1/2000.sup.th, Actin: 1/10000.sup.th, TRP-2: 1/2000.sup.th) and then with the secondary antibody directed against the gene of interest (in all cases, at 1/1000.sup.th), coupled with HRP (horseradish peroxidase). Finally, after an incubation of 5 min with 1 ml of ECL (enhanced chemiluminescence)/membrane, the membranes were developed in a darkroom. This information was also used to perform the dosages as described in Example 11 below (results in FIG. 10).

[0117] The result of the Western Blot thus preformed is shown in FIG. 7. It is observed that the treatment of cells with compositions according to the invention generates a tyrosinase production stimulation similar to that obtained with ultraviolet irradiation; stimulation is stronger for the treatment with (L7).sub.2AF130. This result confirms the one described in Example 8.

EXAMPLE 10: TREATMENT OF RECONSTITUTED SKIN

[0118] In this example, test treatment was carried out on “RHE/MEL light tanned” reconstituted skin epidermis marketed by the “StratiCELL®” company. The medium of the epidermis was changed every day before the test treatment. The treatment consists of adding 1 μM of the treatment product in the medium, twice a day for five days. The epidermi were isolated and placed in an Eppendorf tube with 400 μL of “Solvable” reagent (supplied by Perkin-Elmer) and then heated at 100° C. for 1 h. Absorbance was measured at 490 nm. The amount of melanin synthesized was expressed based on the control (=100%). The results are shown in FIG. 8. The epidermis tanning at the end of treatment were studied by histology highlighting the evidence of melanin deposits in treated skins. At the end of treatment, tissues were placed in a 4% formaldehyde solution and embedded in paraffin and cut. A Fontana-Masson staining (argentaffine method based on silver nitrate) highlights melanin deposits in black. Cut observation through an optical microscope provides the images of FIG. 9.

EXAMPLE 11: STUDY OF THE MODULATION OF DIFFERENT PROTEINS INVOLVED IN MELANOGENESIS ON A RECONSTITUTED SKIN MODEL

[0119] “RHE/MEL light tanned” reconstituted skin samples marketed by the “StratiCELL®” company were used. The sample was treated according to the procedure of Example 9 with the same UV positive control and the same control with actin. The sample was treated twice a day by action of 1 μM of DDA, L7DDA, (L7).sub.2DDA and (L7).sub.2AF130 products.

[0120] Details of the method used have already been provided in Example 9 (GP100: 1/500.sup.th, TRP-1 1/1000.sup.th, Rab27a: 1/500.sup.th).

[0121] The results are shown in FIG. 10 and show that the tyrosinase and proteins involved in melanogenesis TRP-1 and GP100 (key protein of melanosomes biogenesis) are more highly stimulated by the treatment with a composition according to the invention than by UV exposure. Moreover, Rab27a, a protein involved in the transfer of melanosomes from melanocytes to keratinocytes, is more strongly stimulated by treatment with catanionic combinations.

[0122] Examples 12-22 describe compositions according to the invention used for application on human reconstituted skin such as those used in Examples 10 and 11. The compounds are, depending on the case, described with their chemical names or INCI names (International Nomenclature of Cosmetic Ingredients) and the quantities indicated are percentages by weight (percentage of active material for the DDA and catanionic mixtures). Models of reconstituted skin were treated twice a day for three days with 2 mg/cm.sup.2 of the formulations described below (Examples 12-22). The results are illustrated in FIG. 11.

EXAMPLE 12: THE COMPOSITION, WHOSE FORMULATION IS GIVEN BELOW, IS A HYDROALCOHOLIC GEL PREPARED AS FOLLOWS: WATER AND ETHANOL WERE FIRST MIXED, HYDROXYPROPYL CELLULOSE WAS ADDED, STIRRING WAS PERFORMED UNTIL COMPLETE DISSOLUTION THEN THE OTHER COMPONENTS WERE ADDED WHILE STIRRING

[0123]

TABLE-US-00002 Ethanol 50 Glycerin (sold under the name “Pricerine 9091 ®” by the 5 company “Croda”) Hydroxypropyl cellulose (sold under the name “Klucel H 1 CS ®” by the company “IMCD” DDA dilactate Powder (as active molecule) 1 Water up to 100

EXAMPLE 13: THE COMPOSITION, WHOSE FORMULATION IS GIVEN BELOW, IS A HYDROALCOHOLIC GEL PREPARED AND USED AS IN EXAMPLE 12

[0124]

TABLE-US-00003 Ethanol 50 Glycerin (sold under the name “Pricerine 9091 ®” by the 5 company the company “Croda”) Hydroxypropyl cellulose (sold under the name “Klucel H 1 CS ®” by the company “IMCD” (L7).sub.2(DDA) Powder (as active molecule) 1 Water up to 100

EXAMPLE 14: THE COMPOSITION, WHOSE FORMULATION IS GIVEN BELOW, IS A HYDROGEL PREPARED AS IN EXAMPLE 12 WITHOUT ETHANOL, WHICH WAS ABSENT IN THE FORMULATION

[0125]

TABLE-US-00004 Hydroxyethyl cellulose (sold under the name “Natrosol 1.5 250 HR ®” by the company “IMCD”) Glycerin (sold under the name “Pricerine 9091 ®” by the 5 company “Croda”) DDA dilactate Powder (as active molecule) 1 Water up to 100

EXAMPLE 15: THE COMPOSITION, WHOSE FORMULATION IS GIVEN BELOW, IS A HYDROGEL PREPARED AS IN EXAMPLE 14

[0126]

TABLE-US-00005 Hydroxyethyl cellulose (sold under the name “Natrosol 1.5 250 HR ®” by the company “IMCD”) Glycerin (sold under the name “Pricerine 9091 ®” by the 5 company “Croda”) Propylene glycol 5 DDA dilactate Powder (as active molecule) 1 Water up to 100

EXAMPLE 16: THE COMPOSITION, WHOSE FORMULATION IS GIVEN ABOVE IS A HYDROGEL PREPARED AS IN EXAMPLE 14

[0127]

TABLE-US-00006 Hydroxyethyl cellulose (sold under the name “Natrosol 1.5 250 HR ®” by the company “IMCD”) Glycerin (sold under the name “Pricerine 9091 ®” by the 5 company “Croda”) Propylene glycol 5 L7DDA Powder (as active molecule) 1 Water up to 100

EXAMPLE 17: THE COMPOSITION, WHOSE FORMULATION IS GIVEN BELOW, IS A HYDROGEL PREPARED AS IN EXAMPLE 14

[0128]

TABLE-US-00007 Hydroxyethyl cellulose (sold under the name “Natrosol 1.5 250 HR ®” by the company “IMCD”) Glycerin (sold under the name “Pricerine 9091 ®” by the 5 company “Croda”) Propylene glycol 5 (L7).sub.2DDA Powder (as active molecule) 1 Water up to 100

EXAMPLE 18: THE COMPOSITION, WHOSE FORMULATION IS GIVEN BELOW IS A HYDROGEL PREPARED AS IN EXAMPLE 14

[0129]

TABLE-US-00008 Hydroxyethyl cellulose (sold under the name “Natrosol 1.5 250 HR ®” by the company “IMCD”) Glycerin (sold under the name “Pricerine 9091 ®” by the 5 company “Croda”) Propylene glycol 5 (L7).sub.2(AF130) Powder (as active molecule) 1 Water up to 100

EXAMPLE 19: THE COMPOSITION, WHOSE FORMULATION IS GIVEN BELOW IS A HYDROGEL PREPARED AS IN EXAMPLE 14

[0130]

TABLE-US-00009 Hydroxyethyl cellulose (sold under the name “Natrosol 1.5 250 HR ®” by the company “IMCD”) Ethanol 5 Glycerin (sold under the name “Pricerine 9091 ®” by the 5 company “Croda”) Propylene glycol 5 DDA dilactate Powder (as active molecule) 1 Water up to 100

EXAMPLE 20: THE COMPOSITION, WHOSE FORMULATION IS GIVEN BELOW IS AN EMULSION PREPARED AS FOLLOWS

[0131] Preparation of aqueous phase A:

TABLE-US-00010 Hydroxyethyl cellulose (sold under the name “Natrosol 1.5 250 HR ®” by the company “IMCD”) Water up to 100
Preparation of oil phase B:

TABLE-US-00011 Paraffin oil 7.5 Dicaprylyl carbonate (sold under the name “Cetiol CC ®” 4 by the company “BASF”) Coco caprylate (sold under the name “Cetiol C5 ®” by the 4 company “BASF”) Sterate sorbitan and sucrose cocoate (sold the name under 3 the name “Arlacel 2121 ®” by the company “CRODA”)

Preparation of Phase C:

[0132]

TABLE-US-00012 DDA dilactate powder (as active molecule) 0.5 Water up to 100

[0133] Phase B was heated at 80° C. and phase A at the same temperature. Phase B was slowly introduced while under fast stirring into phase A. The mixture was homogenized and cooled under slow stirring: phase C was added when the temperature was below 40° C.

EXAMPLE 21: THE COMPOSITION, WHOSE FORMULATION IS GIVEN BELOW, IS AN EMULSION PREPARED AS FOLLOWS

[0134] Preparation of aqueous phase A:

TABLE-US-00013 Hydroxyethyl cellulose (sold under the name “Natrosol 1.5 250 HR ®” by the company “IMCD”) Water up to 100
Preparation of oil phase B:

TABLE-US-00014 Vegetable oil (sold under the name “Cegesoft PS6 ®” by 5 the company “BASF”) Dicaprylyl carbonate (sold under the name “Cetiol CC ®” 3 by the company “BASF”) Coco caprylate (sold under the name “Cetiol C5 ®” by the 5 company “BASF”) Cocoglycerides (sold under the name “Myritol 331 ®” by 3 the company “BASF”) Isoceteth-3- Acetate (sold under the name “Hetester 8 PHA ®” by the company “SACI-CFPA”)

Preparation of Phase C:

[0135]

TABLE-US-00015 DDA dilactate powder (as active molecule) 1 or 0.1 Water up to 100

[0136] Phase B was heated at 70° C. and phase A at the same temperature. Phase B was slowly introduced while under fast stirring into phase A. The mixture was homogenized and cooled under slow stirring. Phase C was added when the temperature was below 40° C.

EXAMPLE 22: THE COMPOSITION, WHOSE FORMULATION IS GIVEN BELOW, IS A DRY OIL PREPARED AS FOLLOWS

[0137] Preparation of phase A:

TABLE-US-00016 Propylene glycol 5 Dicaprylyl carbonate (sold under the name “Cetiol CC ®” 34.5 by the company “BASF”) Coco caprylate (sold under the name “Cetiol C5 ®” by the 30 company “BASF”) Propylheptyl Caprylate 30 (sold under the name “Cetiol 5 Sensoft ®” by the company “BASF”) Cocoglycerides (sold under the name “Myritol 331 ®” by 10 the company “BASF”) Vegetable oil (sold under the name “Cegesoft PS6 ®” by 10 the company “BASF”) Passiflora incarnata (sold under the name “Cegesoft 2 PFO ®” by the company “BASF”)
Preparation of phase B:

TABLE-US-00017 Ethanol 4.5 basic DDA Powder (as active molecule) 1
Phase B was introduced into phase A under stirring and homogenized.

[0138] In all cases corresponding to Examples 12-22, the skin samples show a tanned, uniform and durable natural coloration. The self-tanning effect intensities are obtained by the Fontana-Masson coloration of histological sections and are summarized in the table below.

TABLE-US-00018 Self-tanning Examples effect 1% by weight DDA Aqueous solution + in H.sub.2O UV (20 mJ/cm.sup.2) / + 12 Hydroalcoholic + gel 13 Hydroalcoholic + gel 14 Hydrogel + 15 Hydrogel ++ 16 Hydrogel ++ 17 Hydrogel +++ 18 Hydrogel +++ 19 Hydrogel ++ 20 Emulsion + 21 Emulsion + 22 Dry oil ++