LU81836A1 - PROCESS FOR THE PREPARATION OF KERATIN HYDROLYSATES AND OLIGOPEPTIDE COMPOSITION OBTAINED BY THIS PROCESS - Google Patents

Description

PROCESS FOR THE PREPARATION OF KERATIN HYDROLYSATES AND OLIGOPEPTIDE COMPOSITION OBTAINED BY THIS PROCESS.

The present invention relates to a process for the preparation of an oligopeptide composition from a keratinous material which is subjected to enzymatic hydrolysis.

It is known that keratin hydrolysates and, in particular, hydrolysates containing a major proportion of oligopeptides are of great interest in the cosmetic industry for their action on the surface state of the hair or on the skin and in the skin. food industry. However, the advantage of these compositions is essentially a function of their oligopeptide content, that is to say that the protein material consisting of keratin serving as raw material must be fractionated into oligopeptide chains containing several amino acids but having a molecular weight low enough to be water soluble. The advantage of keratin hydrolysates is therefore all the greater as these hydrolysates contain few free amino acids. Furthermore, it has been found that it is very advantageous to preserve in the oligopeptide compositions the cystine bonds existing in keratin, the cystine being more energetic in the form of oligopeptides than in the form of amino acid.

In the state of the art, it has been proposed to prepare keratin hydrolysates either from non-degraded keratin raw materials, for example pig bristles, poultry feathers or horn, or from fibrous residual products and keratinous waste, for example by-products from charcuterie and tanning. These keratins or keratin derivatives are subjected either to partial alkaline or acidic chemical hydrolysis in order to limit the production of free amino acids, or to enzymatic hydrolysis.

It is known that the usual proteolytic enzymes (pepsin, trypsin, chymotrypsin, papain) have no notable activity on natural non-degraded keratins, that is to say keratins which have not undergone any chemical, industrial or cosmetic treatment. Even the enzymes described as possible kera-tinolytics, such as for example the enzymes extracted from the different strains of "Keratomices" (pronase, keratinase, M'zyme, / PSF 2019) have, in fact, very reduced activities if not nullLejs 40 on the main natural keratin materials; for example ^ - //

V

2 pie the digestion yields of human hair subjected to such enzymes are less than 10%. It is certain that industrial keratin waste and by-products can be digested by proteolytic or keratinolytic enzymes 5 but, in this case, this is due to the fact that the starting keratin material is degraded and that most of the cystinic bonds of the keratin has disappeared: the result is that the hydrolysates obtained contain practically no cystine. In fact, all the enzymatic hydrolyses, which have a not insignificant efficiency, are hydrolyses which either apply to a raw material, in which the cystine bonds have already largely disappeared, or else apply to a material which is subjected to a pretreatment intended to remove the majority of cystine bonds. In all other cases, the enzymatic action on keratin has a practically zero yield.

In the state of the art, it has also been proposed, in order to obtain keratin hydrolysates, to carry out acid or alkaline chemical hydrolyses. The acid hydrolyses are difficult to control and the hydrolysates obtained are rich in free amino acids even when the solutions acids are not very concentrated: the yield of oligopeptides is therefore low .-------------------------——---------- ------- 25 -------------------------------- Alkaline hydrolyses are performed in the presence of hydroxides alkaline or quaternary ammonium hydroxides and lead to the destruction of certain amino acids and, in particular, of cystine *: there is * formation of H2S, lanthionine, lysinoalanine and cysteine *, 30 Hydrolysates thus obtained are therefore still very poor in cystine.

It can therefore be seen that, in the state of the art, no method for the preparation of keratin hydrolysates makes it possible to obtain oligopeptides containing an important concentration of cystine. Either the hydrolysates have a low yield of oligopeptides and contain a large number of free amino acids, or else the hydrolysates contain practically no more cystine. ,

The object of the present invention is to propose an AI ^ process for the preparation of an oligopeptide composition with a high concentration.

3 * tration into cystine, this process comprising an enzymatic hydrolysis of keratin after it has undergone a pretreatment which does not destroy the cystine. In the state of the art, all the pretreatments applied to keratinous materials to allow the enzymatic actions were pretreatments destroying cystine. In this regard, there may be mentioned the oxidation processes which irreversibly transform cystine into cysteic acid, the sulfite treatment methods, which partially reduce cystine to cysteine with formation in equivalent amount of S-sulfocys-tei 'ne, the thiol reduction processes, which transform cystine into cysteine but also into lanthionine (with loss of sulfur) and mixed disulfide. In all cases, the enzymatic hydrolysates obtained are, of course, poor in cystine since the action of the enzymes with good yield was considered in the prior art to be essentially incompatible with the presence of cystine bonds in the material to be hydrolyze.

According to the invention, it has surprisingly been found that it is possible to obtain an enzymatic hydrolysis action with good yield without destroying the cystine sounds initially present in the keratin material subjected to the hydrolysis , provided that the material to be hydrolyzed is subjected beforehand to an awareness-raising action carried out either with hydrogen bonding agents or with polar solvents which dissolve the interfibril cements existing between the bundles of fibrils made up of micro-. fibrils themselves formed protein chains of keratin, that is, in the case where the keratin material 30 comprises a cuticle enveloping the keratin product itself, with a decuticulating agent.

In all cases, the sensitization treatment proposed according to the invention has no significant action at the level of the cystine bonds of keratin, so that the hydrolyzates obtained always comprise more than 30% of the cystine bonds existing in the starting keratin material. On the contrary, in analogous compositions of the prior art, rich in oligopeptides, never / more than 10% of the cystine bonds of the starting keratin material were found. / iy 4

The present invention therefore relates to a new process for the preparation of an oligopeptide composition by hydrolysis of a keratin material, this process comprising a treatment with proteolytic and / or keratinolytic enzymes, characterized in that before the enzymatic treatment, the keratin material is subjected to an sensitization treatment allowing the subsequent enzymatic action and practically not destroying the cystine bonds initially existing in the keratin material treated.

In a first embodiment of the method according to the invention, the sensitization treatment is carried out by means of at least one sensitizing agent taken from the group formed by the agents which break hydrogen bonds and the solvents. polar. In the case where a hydrogen bond breaking agent is used, said agent can advantageously be taken from the group formed by electrolytes and urea or its derivatives, these agents acting in an aqueous medium at a concentration greater than or equal to 8 moles per liter. Among the particularly interesting electrolytes, lithium bromide should be mentioned below. When the sensitizing agent consists of one or more polar solvents, it is preferred that this or these solvents constitute (s) at least 75% by weight of the medium in which the sensitization treatment is carried out. Among the solvents which can be particularly used, mention should be made of dimethylformamide and methanol.

When the sensitization treatment is carried out using at least one hydrogen bond-breaking agent and / or at least one polar solvent, said treatment is preferably carried out for a time greater than 30 mm and at a temperature 30 rature between room temperature and the reflux temperature of the medium at atmospheric pressure.

When the keratin material, which constitutes the raw material, consists of cuticle keratins, the sensitization treatment can also be carried out by means of at least one decuticulating agent taken from the group formed on the one hand, the ultra- on the other hand, formic acid at a concentration greater than 90% by weight in the treatment medium. If formic acid is used as decuticulating agent, the sensitization treatment is carried out, preferably at 40 ° C., for a time greater than 30 minutes and at a temperature between 5 and 5 ambient temperature. and the reflux temperature at atmospheric pressure.

When the decuticulating agent is an emission of ultrasound, it has been found that satisfactory results are obtained when the ultrasound has a frequency between 20 KHz and 70 KHz and a longer action time. at 30 min, the power dissipated being between 50 and 150 watts per dm? treaty.

When the keratin material used as raw material has undergone the abovementioned sensitization treatment, an enzymatic hydrolysis can be carried out using proteolytic and / or keratinolytic enzymes and very satisfactory hydrolysis yields can be obtained. The enzymatic treatment is advantageously carried out at a pH less than or equal to 9 and at a temperature below 50 ° C to avoid disturbing alkaline hydrolysis, so that the enzymes are not necessarily at the pH corresponding to their optimum kinetics. The concentration of enzymes used depends on the operating conditions and is sufficient to obtain an enzymatic action in the medium. The enzymatic treatment generally lasts between 20 h and 90 h.

The hydrolyzate obtained can be either used in the form of a solution after adjusting the pH, or lyophilized, can be dialyzed, or atomized without raising the temperature, or recovered in the form of a dry residue in a rotary evaporator at approximately 40 ° C. provided to have neutralized the medium, or precipitated in a solvent medium. In all cases, it can be seen that the oligopeptide composition obtained contains few free amino acids, is rich in oligopeptides having a molecular weight between 1000 and 5000 and contains more than 30% of the cystine bonds contained in the starting keratin material. .

The present invention also relates to the new industrial product that constitutes an ovopeptidic composition obtained by the process defined above, characterized in that more than 75% by weight of the oligopeptides, which it contains, have a molecular weight included between 1000 and 5000, the composition containing, in addition, more than 30% by weight of the cystine groups contained in the keratin material used, as raw material. / 40 The present invention also relates to the use of the oligopeptide composition defined above for the treatment of hair or skin or in the food industry.

To better understand the object of the invention, we will now describe, by way of purely illustrative and nonlimiting examples, several modes of implementation.

In these examples, the yield of the enzymatic digestion is calculated by analysis (chromatography on ion exchange resin), after hydrolysis, of an aliquot of the filtered and centrifuged supernatant. In each example, the enzymatic digestion yield was compared for the keratin material treated with or without prior sensitization. In addition, the level of cystine initially present in the treated natural keratin was compared with the level of cystine in the hydrolyzate obtained (protein analysis).

Example 1: a) First step: Sensitization 100 g of cut hair (2 cm long portions) are immersed in two liters of pre-5 dimethylformamide heated to 120 ° C.

The solution is left for two hours at 120 ° C. The hair is then filtered; they are rinsed several times with demineralized water, then with alcohol and ether. They are dried at room temperature.

10 b) Second step: Enzymatic digestion

An enzyme solution containing Proteinase "PSF 2019" (Company 0RIL - PARIS) is prepared just before use. Its formula is as follows: - Proteinase "PSF 2019" purified 15 (11,000 Anson units / mg) 3.2 g - Boric acid 22.5 g - Normal soda 130 ml - MgCl2, 6H20 0.03 g - Demineralized water. ..qsp ... 2000.00 ml 20 Hair presensitized with dimethylformamide is immersed in the enzyme solution brought to 40 ° C.

A paddle stirrer ensures continuous agitation.

Digestion lasts four days. After filtration of the insoluble residue, the solution is neutralized.

25 The results obtained are as follows: performance_ of_ the enzymatic di ges tion: - non-sensitized control hair: 5% - sensitized hair: 38% 2) karatinization of keratin: 30 - cystine in hydrolyzate level: 56 x 10 ~ 3 mole per 100 g of total protein material - cystine level in the initial keratin: _o 62 x 10 mole per 100 g of total protein material

Example 2: a) First step; Sensitization

A procedure identical to that of Example 1 is used, but the sensitization is maintained for A / 40 four hours. / dd 8 b) Second step: Enzymatic digestion

A procedure identical to that of Example 1 is used.

The results obtained are as follows: 5 1) yield_of_the_ <management ,, enzymatic:

- control hair not sensitized 5 X

- hair sensitized 95% - rate of cystine in the hydrolyzate: _o 10 50 x 10 mole per 100 g of total protein material - rate of cystine in the initial keratin: 62 x 10 ”J mole per 100 g of total protein material 15 Example 3: a) First step: Awareness

A procedure identical to that of Example 1 is used, but the sensitization is maintained for six hours.

B) Second step: Enzymatic digestion

A procedure identical to that of Example 1 is used.

The results obtained are the following: 1) enzymatic_digit_dig§stion:

25 - non-sensitized control hair 5 X

- sensitized hair 98 X

2) ǧï§Çtérisati2n_de_l ^ hydrolyzate_de_kératine: - level of cystine in the hydrolyzate: _q 35 x 10 mole per 100 g of proteinaceous 30 total - rate of cystine in the initial keratin:

.O

62 x 10 mole per 100 g of total protein material

Example 4:35 a) First step: Sensitization 100 g of cut cheveix (2 cm long portions) are immersed in two liters of dimethylformamide preheated to 140 ° C. j

The solution is brought to the boil and the refluA / 40 is maintained for one hour. fJf 9

The hair is filtered; they are rinsed several times with demineralized water, then with alcohol and ether. They are dried at room temperature.

b) Second Step: Enzymatic Digestion 5 A procedure identical to that of Example 1 is used,

The results obtained are the following: 1) enzymatic_digestation_of_digestion_ that: - non-sensitized control hair 5% 10 - sensitized hair 81% 2) 9§cracterisation_de_l2hydrolysat_de_kératine: - cystine in hydrolyzate: 25 x 10 mole per 100 g of material total protein 15 - cystine level in the initial keratin:

_ O

62 x 10 mole per 100 g of total protein material

Example 5: a) First step: Sensitization 20 100 g of cut hair (portions of 2 cm long) are immersed in two liters of a solution consisting of 1500 ml of dimethylformamide and 500 ml of demineralized water.

This solution is brought to the boil and the reflux is maintained for three hours.

The hair is filtered; they are rinsed several times with demineralized water, then with alcohol and ether. They're dried at room temperature.

b) Second step: Enzymatic digestion A procedure identical to that of Example 1 is used.

The results obtained are as follows: 1) yield_of_the_digestion_enzymaticjue_: - non-sensitized control hair 5% 35 - sensitized hair 59% 2) keratin hydriglysate: - cystine in the hydrolyzate: / 42 x 10 “3 mole per 100 g of total protein material / day 10 - cystine level in the initial keratin: 62 x 10 “3 mole per 100 g of total protein material

Example 6: 5 a) First step: Sensitization 100 g of cut hair (portions of 2 cm long) are immersed in two liters of methanol,

The solution is brought to a boil and the reflux is maintained for twelve hours.

10 The hair is filtered; they are dried at room temperature.

b) Second step: Enzymatic digestion

A procedure identical to that of Example 1 is used.

15 The results obtained are as follows: 1) ï§5 ^ ®5§? £. ^ §_L§. ^ Î: S§§Îign_enzymatigue: - non-sensitized control hair 5% - sensitized hair 16% 20 - cystine level in the hydrolyzate: _o 60 x 10 mole per 100 g of total protein material - cystine level in the initial keratin: _o 62 x 10 mole per 100 g of total protein material

Example 7: a) First step: Awareness

A procedure identical to that of Example 6 is used, but the sensitization is maintained for 24 hours.

b) Second step; Enzymatic digestion

A procedure identical to that of Example 1 is used.

The results obtained are as follows: 1) yield of enzymatic digestion: - control hair not sensitized 5% - sensitized hair 19% / »^ (f 11 2) 95ï§2iéïî: §§ti: 2? -4ê, 3rl ^ yëï2Î -Y§§t_de_kératine: - cystine level in the hydrolyzate: _o 58 x 10 mole per 100 g of normal protein material 5 - cystine level in the initial keratin: _q 62 x 10 mole per 100 g of total protein material

Example 8: a) First step: Sensitization 100 g of cut hair (2 cm long portions) 10 are immersed in two liters of formic acid preheated to 90 ° C.

The solution is brought to a boil and the reflux is maintained for thirty minutes.

The hair is filtered; they are washed thoroughly with demineralized water, then with alcohol and ether.

They are dried at room temperature.

b) Second step: Enzymatic digestion

A procedure identical to that of Example 1 is used.

20 The results obtained are as follows: 1) enzymatic_digestion_return: - non-sensitized control hair 5% - sensitized hair 14% 25, - level of cystine in 1 hydrolyzate: _q 59 x 10 mole per 100 g of total protein matter - level of cystine in the initial keratin: _q 3q 62 x 10 mole per 100 g of total protein material

Example 9: a) First step: Sensitization 100 g of cut hair (2 cm long portions) 35 are immersed in two liters of formic acid preheated to 90 ° C,

The solution is brought to a boil and the reflux / is maintained for thirty minutes. / Y

/ r / t 12

The hair is filtered. They are immersed again in two liters of formic acid and stirred for 16 hours at room temperature.

The hair is filtered; they are washed thoroughly with demineralized water, then with alcohol and ether. They are dried at room temperature.

b) Second step: Enzymatic digestion

A procedure identical to that of Example 1 is used.

10 The results obtained are as follows: 1) enzymatic_digestion_ yield: - non-sensitized control hair 5% - sensitized hair 23% j 2) ǧï§9t | çisation_de_l ^ hYdrolysate> _de> <ikératine: 15 - cystine level in the hydrolyzate: 57 x 10 ”3 mole per 100 g of total protein material - cystine level in the initial keratin: _q 62 x 10 mole per 100 g of total protein material

Example 10: a) First step: Awareness

A solution of lithium bromide is prepared by dissolving 1,737 g of L.jBr in demineralized water, adjusting the volume to two liters.

100 g of cut hair (2 cm long portions) are immersed in the two liters of sensitizing solution preheated to 90 ° C.

The solution is brought to the boil and the reflux is maintained for one hour.

The hair is filtered; they are washed abundantly with hot demineralized water, then with alcohol and ether. They are dried at room temperature.

b) Second step - Enzymatic digestion A procedure identical to that of Example 1 is used.

The results obtained are as follows: yield of the enzymatic digestion: / - non-sensitized control hair 5% A /

40 - sensitized hair 75 ° / J U

13 2) ǧïëÇ £ erisation_de_l ^ hYdrolysat_de_kératine: - rate of cystine in the hydrolyzate: 53 x 10 ~ J mole per 100 g of total protein material 5 - rate of cystine in the initial keratin: -3 62 x 10 mole for 100 g total protein material

Example 11: a) First step: Sensitization 10 A solution of lithium bromide is prepared by dissolving 1390 g of L ^ Br in demineralized water and adjusting the volume to two liters.

100 g of cut hair (2 cm long portions) are immersed in the two liters of sensitizing solution, preheated to 90 ° C.

The solution is brought to a boil and the reflux is maintained for four hours.

The hair is filtered; they are washed thoroughly with hot demineralized water, then with alcohol and ether. They are dried at room temperature.

b) Second step: Enzymatic digestion

A procedure identical to that of Example 1 is used.

The results obtained are as follows: 25 1) enzymatic_digestion_stress: - non-sensitized control hair 5% - sensitized hair 15% 2) caracterization_of_ [hydrolys§t_de_kératine '· - cystine level in hydrolyzate: _o 30 54 x 10 mole per 100 g of total protein material - level of cystine in the initial keratin: _o 62 x 10 mole per 100 g of total protein material 35 Example 12: a) First step: Sensitization

A solution of lithium bromide is prepared by dissolving 1,737 g of L.Br in demineralized water, / adjusting the volume to two liters. a / 40 100 g of cut hair (2 cm long portions) / \ m 14 are immersed in the two liters of the sensitizing solution.

The solution is brought to 100 ° C., then maintained at this temperature for sixteen hours.

5 The hair is filtered; they are washed thoroughly with hot demineralized water, then with alcohol and ether. They are dried at room temperature, b) Second step: Enzymatic digestion

A procedure identical to that of Example 1 is used.

The results obtained are as follows: 1) yield_d§_la_digestion_enzymatique: - non-sensitized control hair 5% - sensitized hair 13% 15 2) karatinization_de_l2hydrqlysat_de_kératine - cystine in hydrolyzate: 60 x 10 mole per 100 g of total protein matter - cystine level in the initial keratin: 20 62 x 10 'mole per 100 g of total protein material

Example 13: a) First step: Awareness

A procedure identical to that of Example 10 is used.

After refluxing for one hour in the lithium bromide solution, the hair is filtered and then washed abundantly with hot demineralized water and alcohol.

They are then immersed in two liters of dimé-30 thyl-forraamide preheated to 140 ° C. The solution is brought to a boil and the reflux is maintained for thirty minutes.

The hair is filtered; they are rinsed several times with demineralized water, then with alcohol and ether. They are dried at room temperature.

35 b) Second step - Enzymatic digestion

A procedure identical to that of Example 1 is used.

The results obtained are as follows: / 1) yield_ of the enzymatic management: / 40 - non-sensitized control hair 5% / y / 15 - sensitized hair 91% 2) çaracterisation_de_! 2 hydrolyzate_de_keratine: - cystine level in the hydrolyzate: _q 50 x 10 mole per 100 g of total protein material - cystine level in the initial keratin: _o 62 x 10 mole per 100 g of total protein material

Example 14: 10 a) First step: Awareness

A urea solution is prepared by dissolving 1,440 g of urea at 80 ° C in demineralized water and adjusting the final volume to two liters.

100 g of cut cheveik (portions 2 cm long) are immersed in the two liters of sensitizing solution and kept for two hours at 80 ° C.

The hair is filtered; they are washed thoroughly with warm demineralized water, then with alcohol and ether. They are dried at room temperature.

B) Second step: Enzymatic digestion

A procedure identical to that of Example 1 is used.

The results obtained are as follows: 1) yield_of_the_ digestion_ enzymati gue: 25 - control hair not sensitized 5% - hair sensitized 12% 2) £ §ï§2 £ érisation_de_l2hydrolysat_de_keratine: - cystine level in the hydrolyzate: *, q 59 x lo ”mole per 100 g of total protein material ί - cystine level in the initial keratin: 62 x 10 mole, per 100 g of total protein material

Example 15:35 a) First step: Awareness

A procedure identical to that of Example 14 is used, but the sensitization is maintained for eight hours.

b) Second step: Enzymatic digestion ^ / 40 A procedure identical to that of ψ 16 Example 1 is used.

The results obtained are as follows: 1) yield_ of_1§_ diggstion_ enzymati gue: - control hair not sensitized 5% 5 - hair sensitized 17% 2) Ç ^ ïêÇtéHiSftign ^ of ^ hydrolyzate ^ of ^ keratin: - cystine level in the hydrolyzate: 56 x 10 "3 mole for 100 g of total protein material 10 - cystine level in the initial keratin: 62 x 10 ~ 3 mole for 100 g of total protein material

Example 16: a) First step: Sensitization 15 A solution of lithium bromide is prepared by dissolving 1,737 g of L 2 Br in demineralized water, adjusting the volume to two liters.

100 g of horn powder are immersed in the two liters of sensitizing solution, preheated to 90 ° C.

The solution is brought to the boil and the reflux is maintained for one hour.

The horn powder is filtered; it is washed thoroughly with hot demineralized water, then with alcohol and ether. It is dried at room temperature.

B) Second step: Enzymatic digestion

An enzyme solution containing proteinase "PSF 2019" (Company ORXL - PARIS) is prepared just before use. Its formula is as follows: - Purified "PSF 2019" proteinase 30 (11,000 Anson units / mg) '2.5 g - Tris (hydroxymethyl) aminomethane 24.2 g - HCl (normal solution) 55 ml - MgCl2, 6H20 0 , 03 g - Demineralized water ... qs ... 2,000 ml 35 The horn powder presensitized with lithium bromide is immersed in the enzymatic solution brought to 40 ° C. An agitator ensures continuous agitation. .

Digestion lasts four days.

The insoluble residue is filtered and the solution is / / 40 neutralized. {/ 17

The results obtained are as follows: 1) rendexnent ^ de ^ 1§_ tion_enzymaticjue: - non-sensitized control horn powder 46% 5 - sensitized horn powder 62% 2) ǧï§Ç £ erisation_de_l ^ hydrolysat_de_îœr§tine: - level of cystine in the hydrolyzate: -3 25 x 10 mole, for 100 g of total protein material 10 - level of cystine in the initial keratin: -3 31 x 10 mole for 100 g of protein material. that total

Example 17: a) First step: Sensitization 15 100 g of horn powder are immersed in two liters of dimethylformamide, preheated to 120 ° C.

The solution is left for four hours at 120 ° C.

The horn powder is filtered; it is rinsed several times with demineralized water, then with alcohol and ether. It is dried at room temperature.

b) Second step: Enzymatic digestion

An enzyme solution containing chymotryp-sine is prepared just before use.

25 Its formula is as follows: - Alpha-chymotrypsin (47 u / mg) 1.5 g - Tris (hydroxymethyl) aminomethane 24.2 g - HCl (normal solution) 100 ml - Demineralized water ... qs ... 2000 ml 30 The horn powder presensitized with dimethylformamide is immersed in the enzymatic solution brought to 40 ° C. An agitator ensures continuous agitation.

Digestion lasts four days.

The insoluble residue is filtered and the solution is neutralized.

The results obtained are as follows: yield ^, of enzymatic_digestion: - control horn powder not * / sensitized 18 7, / DD 40 - sensitized horn powder 35 ♦ 18 2) This is the keratin hydrolysate: - cystine level in hydrolyzate: 24 x 10 mole per 100 g of total protein material 5 - cystine level in the initial keratin:

w O

31 x 10 “J mole per 100 g of total protein material

Example 18: a) First step: Sensitization 10 100 g of clean rabbit hair are immersed in two liters of dimethylformamide preheated to 120 ° C.

The solution is left for three hours at 120 ° C.

Rabbit hair is filtered; they are rinsed several times with demineralized water, then with alcohol and ether. They are dried at room temperature.

b) Second step: Enzymatic digestion

An enzyme solution containing Prônase (KOCH-LIGHT) is prepared just before use.

20 Its formula is as follows: - Pronase (ex ** streptomyces griseus) 2.4 g - Boric acid (H ^ BO ^) 22.5 g - Normal soda 130 ml - MgC ^, 6H20 0.03 g 25 - Demineralized water .., qsp ,,. 2000 ml

Rabbit hair presensitized with dimethylformamide is immersed in the enzymatic solution brought to 40 ° C. An agitator ensures continuous agitation.

Digestion lasts four days.

The insoluble residue is filtered and the solution is neutralized.

The results obtained are as follows: 1) enzymatic_digestion-yield: - non-sensitized control rabbit hair 4% - sensitized rabbit hair 78% 2) _ri ^atign_de _! ^ Keratin hydrglysat: - cystine level in the hydrolyzate: d 23.5 x 10 "3 moles per 100 g of protein material IA / 40 than total. Dd» 19 - cystine level in the initial keratin: -3 31 x 10 mole per 100 g of total protein material

Example 19: 5 a) First step: Awareness

A lithium bromide solution is prepared by dissolving 1,737 g of L ^ Bj. in demineralized water, adjusting the volume to two liters.

100 g of clean rabbit hair are immersed in two liters of sensitizing solution, preheated to 90 ° C.

The solution is brought to a boil and the reflux is maintained for one hour.

Rabbit hair is filtered; they are washed thoroughly with hot demineralized water, then with alcohol and ether. They are dried at room temperature, b) Second step: Enzymatic digestion

An enzyme solution containing trypsin is prepared just before use.

20 Its formula is as follows: - Pure trypsin (317 u / mg) 15 g - Boric acid (H ^ BO ^) 50 g - Normal soda 290 ml - Demineralized water ... qs ... 5000 ml 25 The hairs of rabbits pre-sensitized to lithium bromide are immersed in the enzymatic solution brought to v 40 ° C. An agitator ensures continuous agitation.

Digestion lasts four days.

The insoluble residue is filtered and the solution is neutralized.

The results obtained are as follows: 1) de_1§-: - non-sensitized control rabbit hair 3% 35 - sensitized rabbit hair 33% 2) ç§ï§çterisation_de_l2hydrolysat-de_kératine: - cystine level in the hydrolyzate: / 25 x 10 ~ 3 mole for 100 g of protein material / l / that total / ί 4 20 - cystine level in the initial keratin: -3 v 31 x 10 mole for 100 g of total protein material

Example 20: 5 a) First step: Awareness

A urea solution is prepared by dissolving 1,440 g of urea at 80 ° C in demineralized water and adjusting the final volume to two liters.

100 g of poultry feathers (down) are immersed in the two liters of sensitizing solution and kept for five hours at 80 ° C.

The feathers are filtered; they are washed abundantly with hot demineralized water, then with alcohol and ether. They are dried at room temperature.

15 b) Second step: Enzymatic digestion

An enzymatic solution containing papain is prepared just before use.

Its formula is as follows: - Papai'ne 8 g 20 - Sodium acetate 32.8 g - Acetic acid 24 g - Demineralized water ... qs ... 4000 ml

The feathers sensitized to urea are immersed in the enzymatic solution brought to 40 ° C. An agitator 25 ensures continuous agitation.

Digestion lasts four days.

The insoluble residue is filtered and the solution is neutralized.

The results obtained are as follows: 30 1) yield of enzymatic digestion: - control poultry feathers not sensitized 7% - sensitized poultry feathers 12% 35 2) çaraçtérisatign_de_ljhydrglys§t_de_kératine: - cystine level in hydrolysate : 30 x 10'3 mole per 100 g of protein material - / ........_ / "21 - cystine level in the initial keratin: _3 34 x 10 mole per 100 g of total protein material

Example 21: 5 a) First step: Sensitization 100 g of poultry feathers (down) are immersed in two liters of dimethyl format, preheated to 120 ° C.

The solution is left for four hours at 120 ° C.

10 The feathers are filtered; they are rinsed several times with demineralized water, then with alcohol and ether. They are dried at room temperature, b) Second step; Enzymatic digestion

An enzyme solution containing Pronase 15 (KOCH-LIGHT) is prepared just before use.

Its formula is as follows: - Pronase (ex ^ -streptomyces griseus) 2.4 g - Tri s (hydroxymé thyl) aminomé thane 24,2 g - HOl (normal solution) 55 ml 20 - MgCl2, 6H20 0,03 g - Demineralized water ... qs ... 2000 ml

The feathers presensitized with dimethylformamide are immersed in the enzymatic solution brought to 40 ° C.

An agitator ensures continuous agitation.

25 Digestion lasts four days.

The insoluble residue is filtered and the solution is neutralized.

, The results obtained are as follows: 1) r§nd§ment_de_l§_digestign_enzym§tigue: 30 - non-sensitized control feathers 10% - sensitized feathers 27 2) ǧ? §Ç £ iïi§§tion_de <iil ^ hydrolysate_de_kératine; - cystine level in the hydrolyzate: 31.5 x 10 mole per 100 g of total proteinaceous material - cystine level in the initial keratin: / -3 / 34 x 10 mole per 100 g of proteinic material - / than total / '/.

<22

Example 22: a) First step: Awareness

A urea solution is prepared by dissolving 1,440 g of urea at 80 ° C in deionized water and adjusting the final volume to two liters.

100 g of poultry feathers are immersed in the two liters of sensitizing solution and kept for five hours at 80 ° C.

The feathers are filtered; they are washed thoroughly with hot demineralized water, then with alcohol and ether. They are dried at room temperature.

b) Second step: Enzymatic digestion • An enzymatic solution containing Pepsin is prepared just before use; its formulation is as follows: - Pepsin (2,870 u / mg) ...................... 2.4 g - IN hydrochloric acid .... ................ 20 ml - Demineralized water .. .qsp ................ 2000 ml

The feathers sensitized to urea are immersed in the enzymatic solution brought to 40 ° C. An agitator ensures continuous agitation. Digestion lasts four days.

The insoluble residue is filtered and the solution is neutralized.

The results obtained are as follows: 1) yield_of_the_digestign_enzym§tique:

- non-sensitized control feathers 6 Z

- sensitized feathers 24 7 2) çaraçtérisatign_de_li [hydrglysat_de_kératine: - cystine level in the hydrolyzate: 30 28 x 10 ~ 3 mole per 100 g of total protein material - cystine rate in the initial keratin: 34 x 10 mole per 100 g of total protein material 35 Protein hydrolysates have a beneficial influence on the hair when they are used in the composition of care or treatment products. The positive physiological and cosmetic effects are explained by the formation of a more or less ordered deposit in the cuticle of the che-yi / 40 veu, which thus protects it from chemical or physical attacks / /, f / y 23 chemicals and which gives it appreciable styling properties. The keratin hydrolysates which have a formula rich in sulfur, are, by their chemical composition, very close to the hair and therefore constitute the ideal proteins for hair care.

Two examples of the use of keratin hydrolysates according to the invention will be given below.

EXAMPLE 23 Vitalizing Lotion

The lotion has the following formulation: 10 - Keratin hydrolyzate ....................... 1 g - Polyoxyethylenated oleic ether containing 20 moles of ethylene oxide (sold under the name of "BRIJ 98" by the company ATLAS) .............. 0.1 g - Acetic acid ___ q.sp ............ .......... pH 7 15 - Colorant ................................... .. 0.1 g - Perfume ....................................... 0.1 g - Alcohol (96th) ............................... 10 ml - Demineralized water ... qs ... ................ 100 ml

The lotion is applied to the hair. A light massage helps distribute the liquid well. Drying takes place at room temperature or under a helmet.

EXAMPLE 24 Rinse Lotion

The lotion has the following formulation: - Hydro lysate of keratin ....................... 1 g 25 - Polyoxyethylenated oleic ether with 20 moles of oxide ethylene (sold under the name "BRIJ 98" by the company ATIAS) .............. 0.1 g - Acetic acid .. .qsp ......... ............. pH 7 - Colorant ................................. .... 0.1 g 30 - Perfume ....................................... 0.1 g - Demineralized water ... qs ................... 100 ml

This lotion is applied to clean hair evenly. After a pose of approximately 5 mn, the hair is rinsed with water and dried under helmet.

The effect of the keratin hydrolysates according to the invention and the keratin hydrolysates of the state of the art was compared. To this end, the microstructures deposited on the surface were studied and, in the lotions / examples 23 and 24, three types of keratin hydrolysates were compared: / 40 * the hydrolyzate prepared according to Example number 2 of this patent application, a hydrochloric keratin hydrolyzate, and an enzymatic hydrolyzate prepared from a degraded keratin poor in cystine.

5 In the arbitrary scale used, the cosmetic field is between 0 and 50. The closer the number is to 0, the better the quality of the deposit.

Vitalizing Lotion Rinse-off rinse 10 Hvdrnivsat used applied on applied on

Hydrolysate uses discolored hair discolored hair (ex. 23) (ex. 24)

Keratin hydrolyzate prepared according to example 2 - rich in cystine 19 11 15 (1000 <molecular weight <5000)

Hydrochloric acid 48 31 (Average molecular weight 20 cd 130)

Enzymatic hydrolyzate, of degraded keratin - poor 65 49 in λ, cystine. (1000 <Molecular weight <5000)

It appears that the keratin hydrolyzate prepared according to Example 2 of the present patent application is the one whose deposit is the most cosmetic. The hair thus treated.

30 is not weighed down by the deposit and acquires appreciable * - / qualities. /] /

Claims (14)

1. Process for the preparation of an oligopeptide composition by hydrolysis of a keratinous material, this process comprising a treatment with proteolytic and / or keratinolitic enzymes, characterized in that before the enzymatic treatment, the · keratinous material is subjected to an sensitization treatment allowing the subsequent enzymatic action and practically not destroying the cystine bonds initially existing in the keratin material treated. 10 2 - Process according to claim 1, characterized in that the sensitization treatment is carried out by means of at least one sensitization agent taken from the 1 group formed by the hydrogen bond breaking agents and the polar solvents. 15 3 - Process according to claim 2, characterized in that the hydrogen bond breaking agents are taken from the group formed by the electrolytes and urea or its derivatives, these agents acting in an aqueous medium at a concentration greater than or equal to 8 moles per liter. 20 4 - Method according to claim 3, characterized in that the electrolyte used is lithium bromide. 5. Method according to claim 2, characterized in that the polar solvents constitute during the sensitization treatment at least 75% by weight of the medium, where the treatment is carried out. 6 · <· Process according to claim 5, characterized in that the polar solvent is taken from the group formed * by dimethyl "" forraamide and methanol. 7. Method according to one of claims 2 to 6, ca-30 characterized by the fact that the sensitization treatment is carried out for a time greater than 30 min and at a temperature between room temperature and the reflux temperature of the medium at atmospheric pressure. 8. Method according to claim 1, characterized in that the keratin material consists of cuticle keratins and that the sensitization treatment is carried out by means of at least one decuticulating agent taken from the group formed by ultrasound and formic acid at a concentration greater than 90% by weight in the treatment medium. J 40 9 - The method of claim 8, wherein 1 * 26 decuticulating gent is formic acid, characterized in that the sensitization treatment is carried out for a time greater than 30 minutes and at a temperature between room temperature and reflux temperature at atmospheric pressure. 10. The method of claim 8, wherein the decuticulating agent is an emission of ultrasound, characterized in that the ultrasound has a frequency between 20 KHz and 70 KHz and an action time greater than 30 10 tnn, the dissipated power being between 50 and 150 watts O per dm treated. 11. Method according to one of claims 1 to 10, "characterized in that the enzymatic treatment after the sensitization treatment is carried out at a pH in-15 lower or equal to 9, at a temperature below 50 ° C and with an active concentration of enzymes. 12. Method according to claim 11, characterized in that the enzymatic treatment has a duration of between 20 --- h and 90 ---- h. 20 13 - oligopeptide composition * obtained by the process according to one of claims 1 to 12, characterized in that at least 75% by weight of the oligopeptides which it contains have a molecular weight of between 1,000 and 5,000, the composition containing, in addition, at least 30% by weight of the cystine groups contained in the keratinous material having served as raw material. 14. Use of the composition according to claim 13 for the treatment of hair or skin or in the food industry. ^; ..... Z ........ r- ... IA ......... ...... ^ ....... · ^ ^ ΛΜ. ...... ......% ....... -n: ...... To ......... · * - ·· '- · -' ψ · * · ^