FR3076461A1 - Cosmetic composition of active prevention signs of age. - Google Patents

Abstract

The present invention relates in particular to the cosmetic use of at least one extract of at least one Iridaceae of the genus Iris, as an agent for preventing and / or delaying the appearance of the first signs of cutaneous aging, in particular related to skin phenomena. oxidation and / or glycoxidation induced by oxidative stress,

Description

Description

Title of the invention: Cosmetic composition for active prevention of signs of aging.

Technical Field [0001] The present invention relates to the field of skin aging, and more precisely the prevention of the appearance of the first signs of age otherwise known as "pre-aging".

STATE OF THE ART

[0002] Skin aging has for many years mobilized research efforts to identify new active agents and / or new technologies aimed at reducing and / or correcting the signs of aging, in particular visible signs such as wrinkles, the loss of elasticity and sagging of the skin which appear and then increase with age and are in particular characteristic of mature skin.

In the context of the present invention, we are interested in the active prevention of the appearance of the first signs of aging, an area for which there still remains the need to develop new cosmetic compositions, in particular adapted to young skin (20-35 years). We speak of “pre-aging” or “pre-aging”, upstream of the phenomena of chronological aging, also called intrinsic aging and photo-induced aging, also called extrinsic aging.

The skin is continuously subjected to multiple attacks which can accelerate its natural aging process. It is particularly sensitive to oxidative stress generated both by the normal functioning of our organism and by external elements such as atmospheric pollution, solar radiation or tobacco. This oxidative stress is characterized by the production of Reactive Oxygen Species (ERO) which can react with all cellular components, causing their modification by oxidation and a deterioration of their function. This notably leads to a progressive decrease in cellular functions following the aggregation (bridging) of macromolecules. In order to counter the action of ERO, cells have developed defense mechanisms, enzymatic or not. We speak of "natural antioxidant defense system of the skin". But these protective mechanisms are also disrupted during aging.

It was recently highlighted by the team of Radjei S et al. (Experimental

Dermatology, 2016, 25, 475-494) the presence of a glyoxalase enzyme system in the epidermis, playing a protective role against oxidative damage induced by reactive oxygen species (ERO) such as glyoxal ( GO) and methylglyoxal (MG). Glyoxalase eliminates glyoxal (GO) and methylglyoxal (MG). Thus this enzyme prevents their accumulation and subsequent glycation phenomena, resulting from the reaction of carbonyl compounds such as GO and MG with the proteins of the skin leading to advanced glycation products (AGE). The elimination of carbonyl compounds (glyoxal and methylglyoxal) is therefore essential to protect the skin from the glycation phenomena involved in skin aging.

According to a particular mode, the "natural antioxidant defense system of the skin" according to the invention involves glyoxalase.

It is in this context that the Applicant has surprisingly demonstrated that an iris extract is capable of increasing the activity of glyoxalase, thus making it possible to act directly on the natural system. of antioxidant defense of the skin to strengthen it and thus delay the appearance of the signs of aging.

The use of an iris extract in cosmetics is already known, in particular from application JPS60-201249 from Shiseido published in 1987, to prevent advanced 'visible' signs of aging, in particular the roughness of the skin. and sagging of the skin, which are rather characteristic of mature skin. We also know of applications WO 97/003556 from the company L'OREAL and WO 02/234229 from the company SILAB, the effects of an iris extract on the reduction of wrinkles via a skin tissue relaxation effect or an inhibition collagenase activity in the dermis, again targeting advanced signs of aging.

But to the knowledge of the Applicant, this is the first time that we have demonstrated the effect of an iris extract on the activity of glyoxalase and its role in the active prevention of the appearance the first signs of aging ('pre-aging'). Summary of the invention A first subject of the invention therefore relates to the cosmetic use of at least one extract of at least one Iridaceae of the genus Iris, as an agent for preventing and / or delaying the appearance of the first signs of skin aging, otherwise known as 'pre-aging'.

Another object of the invention is a cosmetic care process, intended in particular for young skin (subjects between 20 and 35 years old), to prevent and / or delay the appearance of the first signs of skin aging, in particular related to the glycation and / or glycoxidation phenomena induced by oxidative stress, comprising the application to said skin of at least one cosmetic composition comprising at least one Iridaceae extract of the genus Iris.

The invention also relates to a cosmetic composition for topical application to the skin comprising, in a physiologically acceptable medium, at least: I) an Iridacea extract of the genus Iris, preferably of the species Iris florentina, of preferably a rhizome extract of the species Iris florentina II) an extract of red algae, preferably of the species Kappaphycus alvarezii and III) a tocopherol phosphate or one of its salts, preferably a sodium tocopheryl phosphate .

Description of the embodiments [0013] 'Skin aging' is a normal physiological process, involving intrinsic (genetic, hormonal, disease, etc.) and extrinsic (UV, stress, climatic stress, pollution, etc.) factors, and which increases in the course of an individual's life due to a decline in their defense system and their growing need for antioxidants.

Changes in the stratum corneum, epidermis, epidermal junction and dermis vary depending on the age of the individual and are manifested by 'visible signs' of aging, which progress with age, more or less quickly depending on the individual and his environment (intrinsic and extrinsic factors). These 'visible signs' of aging include loss of elasticity, tone and / or firmness of the skin, wrinkles around the forehead, around the eyes and lips, around the neck, loss facial volumes, and pigment spots.

By "pre-aging" within the meaning of the present invention is meant the "invisible signs" upstream of the appearance of visible signs of age. These 'invisible signs' or 'cellular signs' of age, as opposed to 'visible signs' otherwise known as 'clinical signs' of age, include the cellular damage induced by oxidative stress and notably involving oxidations, glycations or protein glycoxidation.

It has indeed been shown that on the skin of donors of different ages, the proportion of carbonylated and glycated proteins increases significantly as a function of age (Petropoulos, I. et al. (2000): Increase of oxidatively modified protein is associated with a decrease of proteasome activity and content in aging epidermal cells. The Journals of Gerontology Sériés a: Biological Sciences and Medical Sciences, 55 (5), B220-7.).

The object of the invention and therefore to act on these cellular phenomena of 'pre-aging', upstream of 'aging', in order to have a skin more resistant to the effects of oxidative stress, for a skin which looks younger longer.

The present invention thus aims to strengthen the natural antioxidant defense system of the skin and thus prevent and / or actively delay the appearance of the first signs of aging ("pre-aging").

By "first signs of age" is meant the very first signs of age, distinct from the advanced clinical signs of aging, described above and in the prior art. These first signs result from the first cellular damage induced by oxidative stress and in particular involving oxidations, glycations or glycoxidation of proteins.

The invention therefore relates in particular to the reuse of at least one extract of at least one Iridaceae of the genus Iris in a cosmetic composition, as an agent for preventing and / or delaying the appearance of the first signs of skin aging (' pre-aging ').

According to a particular embodiment of the invention, the Iridacea extract of the genus Iris is used in a content ranging from 0.0001% to 0.1% by weight of dry matter (active material), preferably from 0.001% to 0.01% by weight of dry matter (active material) relative to the total weight of the composition containing it.

According to a particular embodiment, the invention makes it possible to reduce the oxidation and / or glycoxidation phenomena induced by oxidative stress and thus prevent and / or delay the appearance of the first signs of aging.

Thus, in a particular mode, the iris extract prevents and / or delays the appearance of the first signs of skin aging linked to oxidation and / or glycoxidation phenomena induced by oxidative stress.

By "oxidative stress" according to the invention is meant in particular a stress resulting from the toxic effects of dicarbonylated compounds (ex: glyoxal and methylglyoxal) on proteins. We generally speak of 'oxidative stress' generated by the normal functioning of our organism and by external elements (pollution, UV radiation), which is characterized by the production of reactive oxygen species (ERO or ROS) which can react with all cellular components, in particular proteins and DNA, leading to their modification by oxidation.

By 'oxidation and / or glycoxidation phenomena' according to the invention (we also generally speak of 'glycation'), we mean in particular the reaction of a reducing sugar (glucose) or the aforementioned dicarbonylated compounds (glyoxal and methylglyoxal), along with proteins, leading to the formation of advanced glycation products (EFAs). The presence of these glycation adducts on proteins leads to their denaturation and the inactivation of enzymes.

According to a particular embodiment of the invention, the iris extract of the invention strengthens the natural antioxidant defense system of the skin.

According to a particular embodiment of the invention, the iris extract of the invention increases the activity of glyoxalase in skin cells, in particular epidermal stem cells.

By "epidermal stem cells" according to the invention, is meant in particular cells with high clonogenicity potential located preferentially at the level of the basal layer of the epidermis. Said cells, which make up a small population of skin cells, have the strongest ability to divide and form large colonies compared to other skin cells.

Iris extract According to a preferred embodiment of the invention, the extract of at least one Iridaceae of the genus Iris is chosen from an extract of a species chosen from the group consisting of iris florentina, Iris germanica, Iris pallida or Iris pallasii, preferably Iris florentina.

According to a particular embodiment, it will be a rhizome extract, preferably an rhizome extract of iris florentina.

The iris extract can be mixed in powder form with a composition for topical application to the skin, or can be in the form of a liquid extract obtained by extraction in the presence of an appropriate solvent, preferably at least one cosmetically acceptable polar solvent.

Prior to the extraction step itself, the plant material may have been dried and / or ground.

The extract can be prepared by different extraction methods known to those skilled in the art.

Advantageously, the extraction is preferably carried out by bringing the selected plant material into contact with a polar solvent or a mixture of polar solvents. According to the present invention, the expression “polar solvent” means that the solvent has a value of Polarity index which is equal to or greater than a value of 4. The polarity index is a quantity calculated on the basis of thermodynamic quantities (of solubility and change of state) which highlights the more or less polar character of a molecule. Reference will be made, for the polarity indices of the solvents, to the article by L.R. SNYDER: Classification of the solvent properties of common liquids; Journal of Chromatography, 92 (1974), 223-230.

The preferred polar solvents are those consisting of a compound comprising at least one polar covalent bond of O-H type.

As a particularly preferred polar solvent, a solvent or a mixture of solvents chosen is chosen from water, C1-C4 alcohols, such as ethanol, glycols, such as ethylene. glycol, glycerol, butylene glycol and propylene glycol, and mixtures thereof.

According to a preferred implementation, the plant material is extracted using water. The extraction can be carried out hot by reflux or else by maceration at room temperature.

Advantageously, ultrasound is used during extraction in order to improve the mass yield of said extraction.

The extraction process advantageously comprises a filtration step aimed at separating the liquid phase from the spent plant material.

We can reproduce the extraction cycle then filtration, several times to deplete the plant material of substances having an affinity for the extraction solvent.

The extraction process can also include at least one bleaching and / or purification step, for example in the form of treatment of the extract with a solution of at least one polar solvent in the presence of particles activated carbon. In particular, the chlorophyll extracted by the solvent is eliminated.

The extraction process can also be supplemented by a step of partial or total removal of the extraction solvents.

It is advantageous to concentrate the extract by eliminating part of the solvent or of the mixture of extraction solvent.

One can thus obtain an aqueous concentrate devoid of a significant amount of organic solvents or alternatively, by eliminating all the extraction solvent, obtain a dry residue.

Alternatively, the product of the extraction step can be freeze-dried or atomized to be in the form of a powder.

The polar plant extract as described above can be used in a cosmetic composition in the form of a powder or else be dissolved or suspended in at least one cosmetically acceptable solvent, which can be the same or different from the one used for the extraction.

According to a preferred variant, the concentrated extract of iris is redissolved in water. We will speak of iris extract solution or aqueous iris extract according to the invention. The aqueous extract also advantageously comprises at least one antioxidant, in particular phenoxyethanol.

According to a particular embodiment, the iris extract, in particular iris florentina is capable of being obtained by a process comprising the following steps: - grinding the rhizome of the plant, - extraction of the plant material by steam distillation ("steam distillation"), - filtration then optionally re-solution of the extract obtained in a solvent or a mixture of polar solvents.

Alternatively, powder, concentrated liquid or dilute liquid (extract solution or aqueous extract) forms of iris extract can be used in the preparation of cosmetic compositions. According to a particular and preferred embodiment of the invention, the iris extract according to the invention will be used in the form of an iris extract solution (aqueous extract) in the preparation of cosmetic compositions.

According to a particular preferred mode, the iris extract is in the form of an aqueous extract of 'Iris florentina, preferably an aqueous extract of rhizome A’Iris florentina.

In particular, the extract A ’Iris florentina obtained by hydrodistillation of the rhizome of Iris florentina is in solution in water and advantageously comprises an antioxidant, such as phenoxyethanol.

The iris extract with the name INCI ‘Water and Iris Florentina root extract and phenoxyethanol’ such as that sold under the name Vegebios® of Florence iris 1.5P by the company SOLABIA will advantageously be used. The amount of dry extract (dry matter = active ingredient) in this aqueous commercial solution is approximately 0.5% by weight of dry extract relative to the total weight of the commercial solution.

The invention also relates to a cosmetic care process, in particular intended for young skin (subjects aged 20 to 35), to prevent and / or delay the appearance of the first signs of skin aging, in particular related to the phenomena glycation and / or glycoxidation induced by oxidative stress, comprising the application to said skin of at least one cosmetic composition comprising at least one Iridacea extract of the genus Iris.

According to a particular embodiment, the cosmetic composition comprising at least one Iridacea extract of the genus Iris is applied to young skin, in particular to the skin of a subject aged 20 to 40, preferably from 20 to 35 years, preferably still from 20 to 30 years.

According to a particular embodiment, the composition is applied to the skin of the body and / or of the face and / or of the neck, in particular the skin of the face and / or of the neck, in particular the skin of the face.

According to a particular mode, the composition is applied to the skin of the face of a subject from 20 to 25 years old.

According to a particular mode, the composition is applied to the skin of the face of a subject from 25 to 30 years old.

According to another particular mode, the composition is applied to the skin of the face of a subject aged 30 to 35 years.

According to a particular and preferred mode, the cosmetic care method according to the invention comprises the application to the skin of a composition comprising, in a physiologically acceptable medium, at least: I) an extract of Iridaceae of the genus Iris, preferably of the species Iris florentina, more preferably an extract of rhizome of iris florentina, II) an extract of red alga, preferably of the species Kappaphycus alvarezii and III) a tocopherol phosphate or the one of its salts, preferably a sodium tocopheryl phosphate.

According to a particular and preferred mode, such a composition is applied to the skin of a subject having from 20 to 40 years, preferably from 20 to 35 years, more preferably from 20 to 30 years.

Additional active ingredients According to a preferred embodiment of the invention, the cosmetic composition also comprises at least one agent which protects and / or stimulates the activity of epidermal cells, in particular epidermal stem cells.

The term “protective agent and / or stimulating the activity of epidermal cells” according to the invention means in particular an agent capable of maintaining the number and / or the activity of epidermal cells, for example under oxidative stress conditions . Such an agent can for example be selected for its effect on the protection of telomeres, which delays the entry into senescence of cells.

One can in particular use as an agent with a protective effect and / or stimulating the activity of epidermal cells, a red algae extract, a tocopherol phosphate or one of its salts, and preferably their mixture.

By "red algae extract" according to the invention means in particular an extract obtained from the species Kappaphycus alvarezii- [0066] According to a particular mode, we will use an extract of red alga (Kappaphycus alvarezii ) rich in galactans, such as that sold by the company SILAB under the name TELOSOMYL®. Such an extract, described in patent application LR 3047172 (SILAB), is obtained by hydrolysis of a red algae powder of the species Kappaphycus alvarezii, separation of the soluble and insoluble phases, and filtration so as to collect the fraction aqueous comprising in particular biopolymers. This extract limits damage to the telosome, the protective covering of telomeres. Indeed, TELOSOMYL® stimulates the expression of telosome proteins, thus limiting the shortening of telomeres. TELOSOMYL® preserves the replicative potential of fibroblasts. Longevity is maintained, and programmed aging of the skin is delayed.

The content of red algae extract in the composition of the invention will in particular range from 0.001% to 1% by weight, preferably from 0.0f to 0.1% by weight of dry extract (active material) relative to the total weight of the composition.

The term “protective agent and / or stimulating the activity of epidermal stem cells” according to the invention means in particular an agent capable of maintaining the number and / or the activity of epidermal stem cells, for example under the condition of oxidative stress. Such an agent can for example be selected by a clonogenicity test which is based on the ability of the stem cells to adhere to a support and divide to form large colonies (> 4mm2).

It is recognized that the homeostasis of the interfollicular epidermis, a cutaneous compartment which is constantly renewing, is maintained by a small population of so-called stem cells, located in the basal cellular layer of the epidermis.

To study this population of cells, the test carried out, known as clonogenicity test, is based on the ability of these stem cells to adhere to a support and to divide to form a large population of daughter cells grouped together in the form of colonies. (Barrandon et al., Proc. Nati. Acad. Sci. USA 84 (1987), 2302-2306). The analysis of the number and size of the colonies makes it possible to characterize the stem cells of the epidermis and to evaluate in particular the protective action of an active agent ('protective agent and / or stimulating the activity of epidermal stem cells') ) during stress.

The first step in isolating these cells consists in preparing a suspension of epidermal cells which is then seeded on a nourishing layer of 3T3 fibroblasts whose mitotic activity is blocked by mitomycin.

This support makes it possible: (1) to select the basal cells of the epidermis containing the stem cells and (2) to ensure the growth of cells with high division capacity which then form colonies of daughter cells. The cells with the strongest capacity to divide and form large colonies (> 4mm2) come from the epidermal strain population. The smaller colonies are not from stem cells.

As a protective agent and / or stimulating the activity of epidermal stem cells, mention may in particular be made of tocopherol phosphate or one of its salts, the protective effect of which on the stem cells is illustrated below in the examples.

By “vitamin E phosphate” or “tocopherol phosphate” according to the invention, is meant in particular a tocopherol phosphate in the form of a base or a cosmetically acceptable salt. In the case of a tocopherol phosphate salt, an alkali metal salt, preferably a sodium salt, is preferred.

Advantageously, the tocopherol phosphate is alpha-tocopherol phosphate, beta-tocopherol phosphate, delta-tocopherol phosphate or gamma-tocopherol phosphate, and more particularly alpha tocopherol phosphate otherwise known as alpha tocopheryl phosphate.

A tocopherol phosphate or one of its salts can thus advantageously be used in the composition of the invention, in combination with the iris extract of the invention, to obtain a protective effect of epidermal stem cells .

We preferably combine an extract of Iris forentina and tocopherol phosphate or one of its salts, preferably a tocopheryl sodium phosphate with the name INCI: sodium tocopheryl phosphate.

The tocopherol phosphate content in the composition of the invention will range in particular from 0.001% to 0.1% by weight, preferably from 0.01% to 0.1% by weight relative to the total weight of the composition.

The composition may also comprise other derivatives of tocopherol, such as tocopherol esters other than tocopherol phosphate, to produce an antioxidant protective effect of the cosmetic composition but devoid of a biological effect. Mention will be made, for example, of tocopherol acetate as the antioxidant tocopherol ester of the composition.

Thus, according to a preferred embodiment of the invention, the cosmetic composition of the invention comprises an Iridacea extract of the genus Iris and at least one protective agent and / or stimulating the activity of epidermal cells chosen from the group consisting of a red algae extract, tocopherol phosphate or one of its salts and preferably their mixture.

The cosmetic composition of the invention will advantageously include: an Iridacea extract of the genus Iris for its effect at the molecular level by reducing the production of reactive oxygen species; - a red algae extract for its effect at the cellular level by an action on the protection of telomeres, which delays the entry into senescence of cells; - a tocopherol phosphate, in particular alpha-tocopherol phosphate, or one of its salts, for its effect on the tissue level by an action on the protection of stem cells.

The invention therefore also relates to a cosmetic composition for topical application to the skin comprising, in a physiologically acceptable medium, at least: i) an Iridacea extract of the genus Iris, preferably of the species Iris florentina, preferably still an extract of rhizome <¥ Iris florentina. ii) an extract of red algae, preferably of the species Kappaphycus alvarezii and iii) a tocopherol phosphate or one of its salts, preferably a sodium tocopheryl phosphate.

According to a particular and preferred mode, the Iridacea extract of the genus Iris, the red alga extract and the tocopherol phosphate are packaged in the same cosmetic composition.

The cosmetic composition of the invention may also include other active agents which can in particular be chosen from hydrating agents such as hyaluronic acid or glycerol, smoothing agents or even anti-wrinkle agents such as adenosine, complexes of natural or synthetic polymers producing tensor films on the skin at the time of application to the skin, or even anti-aging active agents, more particularly plant extracts obtained by processes known to man of the trade and which act on biological targets of the superficial or deep layers of the skin in particular, the epidermis, and the dermis, to maintain the elasticity of the skin, to produce a plumping effect, to ensure the renewal or repair of the tissues , maintaining the skin barrier or acting on the complexion of the skin. They can also be lightening or whitening active ingredients which act on tasks that may appear with age, especially on the hands.

Galenic The cosmetic composition of the invention will generally comprise at least one cosmetically acceptable excipient.

By "cosmetically acceptable excipient" is meant a substance devoid of cosmetic or biological effect as such, but useful for Γincorporation of the active agent in the cosmetic composition, in the shaping of said composition, or still at its stability over time.

The excipient is advantageously chosen from solvents, co-solvents (ethanol, glycerol, benzyl alcohol), thickeners, diluents, antioxidants, dyes, chemical or physical filters against solar radiation of UVA and UVB type such as synthetic filters associated or not with filters made up of particles capable of attenuating the effects of this radiation on the skin, self-tanning agents, pigments, fillers, preservatives, perfumes , odor absorbers, cosmetic or pharmaceutical active ingredients, essential oils, vitamins, essential fatty acids, surfactants, film-forming polymers, trace elements, film-forming polymers, chemical or mineral filters, hydrating agents or thermal waters, natural polymers such as polysaccharides or polypeptides, cellulose derivatives, or even synthetic polymers, and in an op tional at least one other active cosmetic agent.

The cosmetic composition according to the invention advantageously comprises an aqueous phase and can advantageously be in all the forms normally used for topical application, in the form of an aqueous, hydroalcoholic or oily solution, of an oil-in emulsion -water or water-in-oil, an aqueous gel, or in any other form for topical application.

This composition may be more or less fluid and have the appearance of a white or colored cream, an ointment, a milk, a lotion, a serum, a paste, d 'a foam or gel. It can optionally be applied to the skin in the form of an aerosol or by means of a patch or a mask or an applicator.

Advantageously, the cosmetic composition according to the invention is an emulsion in the form of a day cream, a night cream, a sunscreen or an after-sun cream.

According to a particular embodiment, the composition according to the invention is a cream present in a cosmetic kit further comprising at least one serum comprising at least one antioxidant.

The invention will now be illustrated by the following nonlimiting examples.

Unless otherwise indicated, the percentages are expressed by weight relative to the total weight of said composition.

EXAMPLES Example 1 Effect of an Iris Extract on the Activity of Glyoxalase 1.1 Materials and Methods Cell Culture [0096] 250,000 KHN967 P6 cells are sown in wells of plate 6 (Costar) in the full Epilife environment (Life Technologies). For 4 days at 37 ° C in a humid atmosphere with 5%. Each point is made in triplicate.

Treatment of VEGEBIOS® IRIS LLORENCE 1.5P solution, comprises 0.5% by weight of dry matter of rhizome Iris florentina, is added to 0.31% by weight in the complete Epilife medium and then filtered through 0 , 22μΜ.

The medium is replaced by this treatment medium for 6 hours.

Protein extraction [0101] After treatment, the cell mats are washed with PBS IX (Invitrogen) in order to remove the dead cells, the various cell debris and the serum from the medium, a trypsin inhibitor.

500 μΐ of TrypLE ™ Express Enzyme (Invitrogen) are added and left for 10 minutes at 37 ° C to dissociate the cells.

The cells are collected in a Protein LoBind Eppendorf tube. The wells are rinsed with 500 μΐ of DMEM supplemented and added to each tube. After centrifugation at 1500 x g for 5 minutes, the cell pellet is rinsed 2 times with 1 ml of PBS IX buffer. The cell pellets are taken up in 70 μl of Cellytic lysis buffer (Sigma) and are stored at -80 ° C.

The cell extracts are thawed and the lysis of the cells is completed mechanically by sonication with Bioruptor (Diagenode); in 5 cycles of 8 seconds ΌΝ ’and 30 seconds OLE’ at 4 ° C. The supernatants are collected and stored at 4 ° C after centrifugation for 15 minutes, 4 ° C, 14,000 x g.

Protein determination (PC protein assay: Biorad} -Reagent B (500-0114) -Reagent A (500-0113) -Reagent S (500-0115)

Reagents B, A and S are the reagents of said DC protein assay kit from Biorad. • Preparation of the standard and reagent range

Stock solution of BSA: 5 mg / ml (Sigma; A2153; 4 ° C), aliquoted and frozen at -20 ° C.

The range is prepared in Eppendorf tubes stored at 4 ° C maximum 2 months.

[Tables 1]

Reagent A is prepared extemporaneously (stable for one week); 20 μL of reagent S are added to 1 ml of reagent A (reagent S is added if the samples contain detergents).

Reagents A, B and S of the kit are stored at room temperature. • Protocol

In a 96-well plate (Costar) are introduced in quadruplicate: - 5 μΐ of H2O for zero - 5 μΐ of lysis buffer for the blank sample - 5 μΐ of stock solution for the range - 5 μΐ of sample to be assayed (diluted to 1 / 2.5) 25 μΐ of reagent A 'are introduced into each well and shaken vigorously.

After 5 minutes, 200 μΐ of reagent B are added to each well.

After shaking the plate; the absorbance is read at 750 nm after 15 min.

Determination of the glyoxalase I activity (GLO1) • Reagents - 100 mM sodium phosphate buffer pH 6.6: 200 ml of monophasic phosphate solution (Sigma) at 100 mM are adjusted to pH 6.6

with a solution of dibasic phosphate (Sigma) about 6.6ml. - Methylglyoxal (MG) solution at 10 mM: 15.8 μΐ from the methylglyoxal solution at approximately 40% in water (Sigma) are added to 10 ml of 100 mM sodium phosphate buffer pH 6.6. - Solution of L-Glutathione reduced (GSH) with 10 mM: 30.7 mg of Glutathione reduced (Sigma) are dissolved in 10 ml of phosphate buffer. • Protocol

The protein lysates are thawed and then centrifuged at 4 ° C at 50,000 x g for 15 minutes.

In a 96-well UV-Star plate (Dutscher), 15 μg of protein are deposited per well.

The reaction mixture is prepared extemporaneously and incubated for 5 min at 37 ° C. [Tables2]

Then 200 μΐ of reaction mixture are mixed with the 15 μg of protein.

The formation of the lactoylglutathione absorbed at 240 nm is measured every minute for 10 min with the Lluostar Omega spectrophotometer (BMG) in an atmosphere at 37 ° C. 1.2 Results [0109] Using the Mars software, the slope corresponding to the reaction speed is calculated in the exponential phase (at the initial time T and at the final time T) from the fluorescence emitted in Lluorescence Units (LU ) every 2 minutes after subtracting the fluorescence emitted in the blank.

Speed AAbs / AT = [ABS test white ass final- [ABS test white ass initial T final-T initial

Activity = Speed / mg protein

Active effect in% = (Activity treated - control activity 1 X. 100 Control activity [0110] The results are presented in Table 3 below.

[Tables3]

Significant when p <0.01 [0112] Methylglyoxal (MG) in the presence of reduced gluthation (GSH) as a cofactor at 2 μΜ each are incubated for 5 min at 37 ° C. in a sodium phosphate buffer at 50 mM at pH 6.6 to produce hemithioacetate, the substrate for Glyoxalase 1 (GLO1). After addition of 15 g of epidermal lysate proteins, the activity of the enzyme is evaluated by measuring the increase in absorbance measured at 240 nm linked to the S-Dlactoylglutathion formed every 10 minutes for 10 minutes.

According to the dosage conditions, the extract &amp; Iris florentina significantly increases glyoxalase activity by 17%.

Example 2: Effect of alpha tocopheryl phosphate on the protection of epidermal stem cells [0115] To study the effect of alpha tocopheryl phosphate on a population of epidermal stem cells, the test carried out, known as clonogenicity test, is based on the ability of these stem cells to adhere to a support and to divide to form a large population of daughter cells grouped together in the form of colonies (Barrandon et al., Proc. Nati. Acad. Sci. USA 84 (1987) ), 2302-2306). Analysis of the number and size of colonies makes it possible to characterize the stem cells of the epidermis and to evaluate in particular the protective action of an active ingredient during stress.

The first step in isolating these cells consists in preparing a suspension of epidermal cells which is then seeded on a nourishing layer of 3T3 fibroblasts whose mitotic activity is blocked by mitomycin.

This support makes it possible: (1) to select the basal cells of the epidermis containing the stem cells and (2) to ensure the growth of cells with high division capacity which then form colonies of daughter cells. The cells with the strongest

ability to divide and form large colonies (> 4mm2) come from the epidermal strain population. The colonies of smaller sizes are not derived from stem cells. The protective effect of alpha tocopheryl phosphate is demonstrated by this culture method. In a first step, the keratinocytes are treated with lpg / ml of alpha tocopheryl phosphate for 24 hours and then subjected to oxidative stress with hydrogen peroxide for 15 min. They are reseeded at very low density which allows their individual growth. After 7 days of culture, the cell colonies formed from each keratinocyte are stained, counted by image analysis as a function of their size to assess the quantity of stem cells from the initial cell culture [0119] It is found that the treatment with alpha tocopheryl phosphate under these conditions makes it possible to maintain the large number of large colonies (greater than 4 mm 2) during oxidative stress of + 104% compared to the number of large colonies in the absence of treatment. The large colonies being derived from stem cells, alpha tocopheryl phosphate therefore protects this particular population of cells.

Example 3: Formulations [0120] Day cream [oil-in-water emulsion) [0121] The following composition is prepared [0122] Iris florentina rhizome extract (1) 0.005% (% DM *) [0123] Extract of Kappaphycus Alvarezii (2) 0.03% (% DM *) [0124] Tocopheryl sodium phosphate 0.02% [0125] Glyceryl stearate + PEG-100 stearate 5.0% [0126] Hydrogenated polyisobutene 4.0% [0127 ] Magnesium ascorbyl phosphate 3.0% [0128] Tricaprylate / glycerol caprate 3.0% [0129] Squalane 3.0% [0130] Glycerin 3.0% [0131] Shea butter 1.5% [0132] Cetearyl octanoate 1.5% [0133] Cetyl alcohol 1.0% [0134] Stearyl alcohol 1.0% [0135] Dimethicone 1.0% [0136] Xanthan gum 0.3% [0137] Citric acid 0.1% [ 0138] Sodium citrate 0.1% [0139] Adenosine 0.05% [0140] Neutralizer, Perfume, Preservatives qs.

Water qs. 100% [0142]% M.S *:% of dry matter in the total composition. 1.; VEGEBIOS IRIS FLORENCE 1.5P at 0.5% by weight of dry matter of extract 2. TEEOSOMYE®, 0.6% of dry matter of extract [0143] The aqueous phase and the oily phase are prepared separately and then mixed according to the classic mode of formulation of an emulsion.

The use of this cream, by its action its antioxidant action and the protection of the extracellular matrix also makes it possible to attenuate or delay the very first signs of aging of the skin in young subjects under 35 years.

Brightening Face Serum [0146] A serum is prepared according to the composition below: [0147] Iris florentina rhizome extract (1) 0.01% (MS *) [0148] Kappaphycus Alvarezii extract (2 ) 0.05% (MS *) [0149] Tocopheryl sodium phosphate 0.02% [0150] Glycerin 2% [0151] Xanthan gum 0.25% [0152] Polymethylsilsesquioxane 2% [0153] Ethyl alcohol 2% [0154] Lactic acid 1% [0155] Polyacrylate 0.50% [0156] Dimethicone copolyol 0.25% [0157] Neutralizer, Perfume, Preservative qs [0158] Water qs 100% [0159]% DM *:% of dry matter in the total composition. 1.; VEGEBIOS IRIS FLORENCE 1.5P at 0.5% by weight of dry matter of extract 2. TEEOSOMYE®, 0.6% of dry matter of extract [0160] A drop of serum, applies to the face generally before application of a face cream. This serum is usually used for one to two week courses.

Claims (1)

Claims [Claim 1] Cosmetic use of at least one extract of Iris florentina, as an agent for preventing and / or delaying the appearance of the first signs of skin aging linked to oxidation and / or gly-coxydation phenomena induced by oxidative stress. [Claim 2] Cosmetic use according to claim 1, in which the extract of iris florentina strengthens the natural antioxidant defense system of the skin. [Claim 3] Use according to claim 1 or claim 2, wherein the extract of 'Iris florentina increases the activity of glyoxalase in skin cells, in particular epidermal stem cells. [Claim 4] Use according to any one of claims 1 to 3, wherein the extract &amp; Iris florentina is used in a content ranging from 0.001% to 0.1% by weight of dry matter, preferably from 0.001% to 0.01% by weight of dry matter relative to the total weight of the composition. [Claim 5] Cosmetic care method for preventing and / or delaying the appearance of the first signs of skin aging linked to glycation and / or glycoxidation phenomena induced by oxidative stress, comprising applying the skin of a subject having 20 to 35 years, preferably 20 to 30 years, of at least one cosmetic composition comprising at least one extract &amp; Iris florentina. [Claim 6] Cosmetic care method according to claim 5, characterized in that the cosmetic composition also comprises at least one protective agent and / or stimulating the activity of epidermal cells, in particular chosen from the group consisting of an extract of red alga, a tocopherol phosphate one of its salts, and preferably their mixture.