KR100374161B1 - Skin care composition containing Phytosphingosine and Morus alba Extract - Google Patents

Abstract

The present invention relates to a skin-improving cosmetic composition containing phytosphingosine and upper limb extract, and stabilizes phytosphingosine with superior upper limb extract and skin cell proliferation and blood circulation promoting effects. The present invention relates to a skin-improving cosmetic composition which contains an anti-shadowing effect on the eyes or under the eyes by containing).

Description

Skin care composition containing Phytosphingosine and Morus alba Extract}

The present invention relates to a skin improvement cosmetic composition containing phytosphingosine and upper limb extract.

Skin, the largest organ that makes up the human body with an area of 1.8m ^2, has a barrier function, temperature control function, respiratory function, and excretory function that protects other important organs of the human body from the outside and prevents useful components from getting out. It plays various roles.

However, the skin is in direct contact with the outside compared to other organs of the human body, so it is not only sensitive to changes in the environment, but also like other organs, it ages and ages, resulting in various forms such as wrinkle formation, skin elasticity, blemishes, and freckles. Indicates problems

Human skin color is largely determined by the amount of melanin, hemoglobin, carotene and the like, of which melanin plays the most important role. Melanin acts as a skin protective action (ultraviolet absorption, Free Radical Scavenger) in addition to human skin color determination, but excessive skin due to external environmental changes (excess exposure to ultraviolet rays, air pollution, stress, etc.) When it is generated inside, the pigmentation phenomenon occurs in the skin, which causes the skin color to blacken, blemishes, and freckles. The melanin synthesis process, which is the cause thereof, is as follows.

First, an enzyme called tyrosinase produces dopaquinone using tyrosine in a cell as a substrate, and a melanin copolymer is produced through autooxidation and enzymatic reaction from dopaquinone. The melanin produced in this way is transferred to the keratinocytes through the melanosomal sac, and the keratinocytes undergo 28 days of keratinization and come out to the skin surface. However, in this process, if the melanin is excessively produced by a factor that promotes melanin production and melanin is not completely eliminated by keratinization, pigmentation occurs. Therefore, in order to prevent the pigmentation phenomenon, it can be suppressed by controlling some processes in melanogenesis.

There are several mechanisms that inhibit melanin synthesis. A typical synthesis inhibition process is the most known to inhibit tyrosinase, an important enzyme of melanin synthesis, a chelator such as kojic acid, and a substrate-like substance such as arbutin. In addition, plant extracts include lettuce extract, licorice extract and the like. However, these whitening raw materials have a disadvantage that their effects do not last long due to their low stability, so the scope of application of the products is very narrow.

In addition to the problems mentioned above, in order to solve problems such as wrinkle formation and skin elasticity reduction, functional cosmetics are emerging under the concept of `` Cosmeceuticals '' that emphasize functions and effects. Although most of them are formed, they have problems of effectiveness and stability.

Therefore, researches on cosmetics using biological ingredients to enhance functionality and safety have been carried out. Among them, ceramide is emerging as a raw material of high functional cosmetics due to its variety and safety of physiological functions. Specifically, it is as follows.

Human skin is composed of epidermis, dermis, and subcutaneous fat layer. The epidermis can be divided into four layers. The keratinocytes, the main cells of the epidermis, rise from the basement layer to the stratum corneum, resulting in biochemical and morphological changes. At this time, the intercellular lipid component between keratinocytes and keratinocytes of the stratum corneum is mostly in the form of phospholipids in the basal layer, but is mostly in the form of ceramide in the stratum corneum through lipid metabolism. This ceramide is restored by the synthesis and supply of cholesterol, fatty acids and ceramides within the skin cells even if the skin's epidermal layer is normal. Among these, ceramide synthesis starts at the latest, which protects the skin and normal function of the skin. Supply of ceramide is required for maintenance. This ceramide helps the collagen synthesis by signaling the external environment of the epidermal layer cells, and the cell damage caused by UV rays, which is the main cause of skin aging and wrinkles, wrinkles and wrinkles. It is excellent in preventing elasticity loss due to water evaporation and collagen destruction, delaying and alleviating fine wrinkles. In addition, it provides a moisturizing effect that inhibits moisture control and moisture evaporation, and a lifting function that enhances elasticity by tightly connecting cells to cells. The ceramide is not chemically referring to a single substance but is a generic term for various kinds of substances, and six ceramides are known to exist in the human skin. In particular, ceramides are generally animal-derived similar to human ceramides than those derived from plants derived from soybeans, and recently, the same ceramides as human skin are separated from yeast. Sphingoid bases are one of the most abundant intercellular lipids in the stratum corneum.Sphingoid bases contain phytosphingosine, sphingosine, and sphinganine in a ratio of 5.6: 2.4: 1. Ceramide is formed by the enzymatic action of ceramidase from these free sphingoid bases and free fatty acids. The free sphingoid base inhibits the activity of protein kinase C and plays an important role in cell growth, promotes ceramide biosynthesis, anti-inflammatory effect, antioxidant effect and skin surface. Antibacterial effect that inhibits the growth of bacteria and microorganisms has various physiological activities such as effectively inhibit the growth of acne-forming strains.

Therefore, in order to solve this problem in relation to skin aging such as skin elasticity reduction, wrinkle formation, skin moisturizing, research on ceramides having excellent functionality and safety as a raw material of high functional cosmetics has been actively conducted.

An object of the present invention is a dull phenomenon appearing around the eyes or under the eyes by simultaneously containing the upper limb extract extracted from the upper limbs of Morus alba Linne and the skin cell proliferation and blood circulation promoting effect Phytosphingosine In addition, the present invention provides an anti-shadow cosmetic composition that improves the appearance of unhealthy skin.

In order to achieve this object, the cosmetic composition of the present invention is iosome stabilized by containing phytosphingosine and upper limb extract (0.05 to 20.0% by weight, preferably 0.1 to 10.0% by weight relative to the total weight of the cosmetic) It is characterized by containing in%.

Hereinafter, the configuration of the present invention in more detail as follows.

The present invention relates to a skin improvement cosmetic composition containing the upper limb extract and phytosphingosine at the same time, looking at this in detail.

The upper extremity extract is extracted from the upper limbs of the mulberry ( Morus alba Linne) of the mulberry family, excellent tyrosinase inhibitory effect and long-lasting, melanin synthesis inhibitory effect of the present inventors have already patented the whitening effect of the upper limb extract Application (97-47258) has been filed.

In addition, the phytosphingosine is an intermediate of the ceramide biosynthetic pathway, which is applied to the skin to supplement the deficient ceramide component or allow the skin cells to directly synthesize ceramide (USP5578641), from yeast. It is used separately and is the same as Phytosphingosine whose structure and properties are present in human skin.

The phytosphingosine (Phytosphingosine) is an intermediate of ceramide (ceramide) 1, 3, 6 of the six ceramides present in the skin to inhibit the growth of unnecessary microorganisms on the skin, protein kinase C (protein kinase C) It inhibits the secretion of interleukin 1α (IL-1α), an inflammatory precursor, by inhibiting inflammation and irritation to maintain healthy skin and promote blood circulation and cell activity.

The skin improvement cosmetic composition of the present invention contains niobium stabilized by containing the upper limb extract and phytosphingosine in an amount of 0.05 to 20.0 wt% based on the total weight of the cosmetic, preferably 0.1 to 10.0 wt% do. At this time, the upper limb extract is blended with 0.01-5.00% by weight, preferably 0.1-2.0% by weight relative to the total weight of niosomes, and phytosphingosine is 0.01-5.00% by weight, preferably 0.1- with respect to the total weight of niosomes. It is compounded at 2.0 weight%.

The cosmetic composition containing the upper limb extract and phytosphingosine is a softening longevity, astringent longevity, nourishing longevity, eye cream, nourishing cream, massage cream, cleansing cream, cleansing foam, cleansing water, powder, pack, essence, pack, etc. The formulation is not particularly limited and may be appropriately selected and blended with other components other than the phytosphingosine and the upper limb extract according to the formulation or purpose of use of the cosmetic.

The following is described in more detail with reference to the following embodiments of the present invention configured as described above. However, these examples are intended to illustrate the present invention, it is obvious to those skilled in the art that the scope of the present invention is not limited to these examples. Compounding amount is shown by weight%.

Preparation Example 1 Niosome Manufacturing Method

Niosome used in the present invention is composed of a stable nonionic surfactant, cholesterol and similar derivatives, polyoxyethylene alkylether (Polyoxyethylene alkylether), alkyl ester (Alkylester), Saccharose diester (Saccharose diester) A nonionic surfactant, such as), is used. Such nonionic surfactants use PEG-5-Soy sterol and cholesteryl oleate as bases, and supplement the role of lipids in the skin. In order to combine the ceramide 3 (Ceramide 3) in the glycerin skeleton to have amphiphilic properties, it was similar to the natural lipid component. In each composition, 60-70% of the cholesterol extracted from sheep's hair and beta-sitosterol derived from Finnish pine were used.The nonionic surfactant was Fiji-5-Soysterol (PEG) extracted from soybean. -Soy sterol) and cholesteryl oleate (Cholesteryl oleate) using 30-40% and ceramide 3 (Ceramide 3) using 0.1-10% Vesicle was made. Therefore, the niosomes used in the present invention are also referred to as nonionic surfactant vesicles (NSV). Phytosphingosine and upper extremity extracts of the present invention are combined with 0.01-5.00% by weight, preferably 0.1-2.0% by weight, based on the total weight of niosomes, respectively, and stabilized in the Vesicle to facilitate skin penetration. Maximize the effect of niosome (Niosome) is to manufacture.

Preparation Example 2 Preparation of Upper Limb Extract

The manufacturing method of the upper limb extract contained in the cosmetics of this invention is as follows. First, wash the upper limb with purified water, put 1kg of dry upper liquor in 5L of 70% ethanol, extract for 5 days at 4-40 ℃, filter with 300 mesh filter cloth, and leave it at 5-10 ℃ for 7-10 days to ripen, and then filter the Whatman filter paper. Filter with. The extract is dried on a rotary vacuum evaporator at 65 ° C. to obtain upper extremity powder.

Examples and Comparative Examples: Cream Preparation

Phytosphingosine (Phytosphingosine) of the present invention and the composition containing the niobium stabilized upper extremity extract as an example, to prepare a composition containing no niosomes as a comparative example as shown in Table 1 below.

Unit (part by weight) Ingredient Example Comparative example Niosome 10.0 - vaseline 7.0 7.0 Liquid paraffin 10.0 10.0 Beeswax 2.0 2.0 Polysorbate 60 2.0 2.0 Sorbitan sesquioleate 2.5 2.5 Squalane 3.0 3.0 Propylene glycol 6.0 6.0 glycerin 4.0 4.0 Triethanolamine 0.5 0.5 Carboxy Vinyl Polymer 0.5 0.5 Tocopheryl Acetate 0.1 0.1 Incense, preservative a very small amount a very small amount Purified water to 100 to 100

Experimental Example 1 Test for Anti-shadow Effect

1) Experiment Method

In order to measure the anti-shadow effect of the cosmetic composition containing phytosphingosine and the upper limb extract of the present invention and the cosmetic composition not containing the same as Examples and Comparative Examples, 30 women over 30 years old After dividing the group into two groups (A and B) of 15 people, group A contained a cream containing phytosphingosine and niobium stabilized upper extremity extract (example), and a cream not containing group B (comparative example) The anti-shadow effect was measured by applying 0.2mg twice a day for 12 weeks around the eyes and under the eyes. The degree of change in skin tone brightness (ΔL) was measured using chromata (Minolta CR300), and objective visual observation by a plurality of experts and subjective visual observation by a subject were performed. Visual observation was measured according to the following seven classifications and the results are shown in Table 2 below.

·Evaluation standard :

-3: very worse -2: worse -1: slightly worse 0: no change

1: slightly improved 2: improved 3: highly improved

2) Experiment result

Clinical Results for Anti-shadow Subject Change in brightness of skin color (ΔL) Objective evaluation of the skilled person Subjective Evaluation of Subject A B A B A B One 5.1 1.9 One One One 0 2 5.6 1.0 3 0 3 0 3 3.2 1.8 One -One 2 0 4 7.1 0.3 2 0 3 0 5 7.4 2.1 3 One 2 2 6 5.2 -0.5 One 0 2 0 7 5.5 1.6 3 One 3 One 8 8.8 2.2 3 One 3 2 9 2.9 0.7 2 One One 0 10 5.2 -1.0 2 0 One One medium 5.6 1.01 2.1 0.4 2.1 0.6

As can be seen in Table 2, the average ΔL value of the A group to which the Example containing the phytosphingosine of the present invention and the niobium stabilized upper limb extract was applied was 5.6 (P <0.01), The average ΔL value of the B group coated with the comparative example containing no was 1.01 (P> 0.05), and the nitosomes stabilized phytosphingosine and upper extremity extracts effectively improved skin tone. In the objective visual evaluation by skilled workers, group A was 2.1 (P <0.01), group B was 0.4 (P> 0.05), and subject A was 2.1 (P <0.01), B in subjective visual evaluation. As the group is represented by 0.6 (P> 0.05), it can be seen that the embodiment containing phytosphingosine and niobium stabilized upper extremity extract showed a definite anti-shadowing effect.

Experimental Example 2: Test of inhibitory activity of tyrosinase activity of the upper limb extract

1) Experiment Method

To determine the degree of inhibition of tyrosinase activity of the upper limb extract, the upper limb extract is prepared by dissolving the upper limb powder in high concentration in 1,3-butylene glycol and diluting it again in a buffer solution to prepare an extract sample solution as shown in Table 3 below. . Tyrosinase was isolated and purified from mushrooms (SIGMA), and the substrate tyrosine was dissolved in 0.05M sodium phosphate buffer (pH 6.8) to make 0.1 mg / ml solution.

0.5 ml of the tyrosine solution was added to a test tube, and 0.5 ml of the upper limb extract sample solution prepared at the concentration shown in Table 3 was added thereto, and the mixture was left to stand at 37 ° C. for 10 minutes, and 0.5 ml of 200 U / ml tyrosinase was added thereto for 10 minutes at 37 ° C. React. In this case, 0.5 ml of kojic acid, which is known to have strong tyrosinase activity inhibitory activity, was added instead of the upper extremity extract. The test tube containing the reaction solution was placed on ice to stop the reaction, and the absorbance at wavelength 475 nm was measured by using a spectrophotometer. The effect of increasing the tyrosinase activity of each extract was determined by the following formula. 3 is shown.

2) Experiment result

Inhibitory Effect of Upper Limb Extracts on Tyrosinase Activity Concentration (µg / ml) Tyrosinase activity inhibition rate (%) Upper limb extract Kojic acid One 6.5 5.4 2 14.1 16.9 5 37.0 42.5 10 55.8 64.4 20 67.5 77.2 50 76.8 84.6 100 84.4 88.8 200 93.2 92.3

As shown in Table 3, the upper limb extract has a strong tyrosinase activity inhibitory ability, but it can be seen that it shows a high tyrosinase activity inhibitory effect similar to kojic acid known to have problems of skin irritation and stability.

Experimental Example 3: Test of the inhibitory effect on melanin production in the melanocytes (Melanocyte) of the upper limb extract

1) Experiment Method

To investigate the inhibitory effect of the upper limb extract on melanin synthesis in melanocytes, melanocytes were used by purchasing a mouse-derived B-16 melanoma (ATCC CRL 6323) cell line. Melanoma cell lines were inoculated in DMEM medium containing 4.5 g / L glucose, 10% serum and 1% antibiotics and incubated at 37 ° C. in a 50 ml T-flask. After 24 hours of incubation under 5% CO ₂ , the cells were isolated by treatment with 0.05% Trypsin containing 0.02% EDTA, and then incubated in a 50 ml T-flask for 48 hours. At this time the cell number is 5.76 × 10 ⁶ cells / flask. The upper limb extract is diluted in DMEM medium at an appropriate concentration, treated with cultured melanoma cells, and incubated at 37 ° C. for 5 days. After incubation, all of the medium was removed, cells were treated with 1 ml of saline-phosphate buffer (PBS) containing 0.02% EDTA and 0.05% trypsin, and then cells were collected by centrifugation for 5 minutes. 5% trichloroacetate (TCA) is treated, stirred and centrifuged to wash the precipitated melanin with saline-phosphate buffer. 1N NaOH was dissolved in the melanin precipitated, and then the absorbance was measured at 475 nm. Melanin concentrations were determined from standard concentration curves of synthetic melanin (Sigma) and the results are shown in Table 4 below.

2) Experiment result

Inhibitory Effect of Upper Limb Extracts on Melanin Synthesis in Melanosite Upper limb extract concentration (㎍ / ㎖) Melanin production inhibition rate (%) No treatment - One 1.17 2 10.0 5 17.2 10 27.4 20 31.4 50 43.7 100 54.2

As shown in Table 4, as the concentration of the upper limb extract increases, the inhibition of melanogenesis in the melanocytes increases, indicating that the upper limb extract has a melanin synthesis inhibitory effect.

Experimental Example 4: Test for the cell proliferation effect of Phytosphingosine

1) Experiment Method

Human normal Keratinocytes are inoculated to ¹ × 10 ⁴ cells in each well of a 96-well microplate and incubated in DMEM medium for 24 hours. After incubation, phytosphingosine was dissolved in dimethyl sulfoxide (DMSO) and diluted again in an appropriate concentration in a buffer solution to adjust the final concentration to 250 μg / ml. Incubate for another 24 hours after replacement. Add 10 µl of MTT solution [3- (4,5-Dimethyl-thiazole-2-yl) 2,5-diphenyl tetrazolium bromide: 5 mg / ml], and leave for 4 hours, and then discard the media. 100 μl of dimethyl sulfoxide (DMSO) solution was added to each well, followed by stirring for 20 minutes, and the absorbance at 570 nm was measured using a microplate reader. The cell proliferation effect was calculated by the following formula. It is shown in Table 5 below.

2) Experiment result

Cell proliferation effect in keratinocytes Phytoshpingosine Concentration (㎍ / ㎖) Cell proliferation effect (%) No treatment - 10 8.3 50 17.5 100 31.8 200 66.3 500 78.5

* The above value is the average of 3 runs

Experimental Example 5: Skin safety test for cosmetics containing niosomes

1) Experiment Method

To test the skin stability of cosmetics containing phytosphingosine and niobium stabilized upper extremity extracts, 30 subjects (mean age 27.5 years, age distribution 19-35 years) were divided into two groups of Haye's Test Chamber Skin patch test (Patch Test) was performed on the upper arm by using. Psoriasis, eczema, and other skin lesion holders, or those who are pregnant, nursing or contraceptives, and antihistamines, were excluded from this study.

Wipe the test site with 70% ethanol and dry it. Then, add the Example and Comparative Example products to the A group and the B group by dropping 15 µg into the chamber, and fix the test site on the upper arm. The patch is applied for 24 hours, and after removing the patch, the test site is marked with a marking pen, and the test site is observed after 24 hours and 48 hours, respectively, and the results of the International Contact Dermatitis Research Group (ICDRG) shown in Table 6 below. Judging according to the regulations. The experimental results are shown in Table 7 below.

Criteria for international contact dermatitis sign Criteria evaluation Mean score ± ++++++- Doubtful or slight reaction and erythemaErythema + IndurationErythema + Induration + VesicleErythema + Induration + Bullae Stimulus stimulus non stimulus 0 to 0.91.0 to 2.93.0 to 4.95.0 or more

2) Experiment result

Skin safety Elapsed time Example Comparative example 24 hours 0 0.5 48 hours 0 0

As shown in Table 7, the cream containing the nitosomes stabilized phytosphingosine and the upper extremity extract of the embodiment of the present invention as a result of the skin safety test results do not show a stimulus from all the subjects as a safe base for skin Able to know.

Experimental Example 6: Formulation stability test of cosmetics containing niosomes

1) Experiment Method

In order to test the formulation stability of cosmetics, the examples containing phytosphingosine and niobium stabilized upper extremity extract and the comparative example were not maintained at 45 ° C. and 4 ° C., respectively. After storing for 12 weeks in an opaque glass jar in a shaded refrigerator, the degree of separation and discoloration were measured. The degree of separation and discoloration of the product was classified into six grades and evaluated. The results are shown in Table 8.

Product discoloration evaluation criteria:

0: no change 1: very little separation (discoloration)

2: Separate slightly (discolored) 3: Separate slightly (discolored)

4: severely separated (discolored) 5: extremely severely separated (discolored)

2) Experiment result

Separation and discoloration Temperature Discoloration degree of test substance Example Comparative example 45 ℃ 0 0 4 ℃ 0 0

As can be seen in Table 8, the embodiment containing the phytosphingosine (Phytosphingosine) of the present invention and the niobium stabilized upper extremity extract can be seen that there is no discoloration and separation phenomenon is a stable base.

Formulation Example:

A composition containing phytospingosine of the present invention and a niobium stabilized upper extremity extract was introduced into a product, and the conventional cosmetics were formulated at 0.05-20.0% by weight, preferably 0.1-10.0% by weight, based on the total weight of the cosmetic. According to the manufacturing method in the field. However, the composition of the present invention is not limited to the following formulation examples.

Formulation Example 1: Softener (Skin Lotion)

Ingredient Parts by weight Niosome 1.0 1,3-butylene glycol 6.0 glycerin 4.0 Oleyl alcohol 0.1 Polysorbate 20 0.5 ethanol 15.0 Benzophenone-9 0.05 Incense, preservative a very small amount Purified water to 100

Formulation Example 2: Nutrients (Milk Lotion)

Ingredient Parts by weight Niosome 3.0 Propylene glycol 6.0 glycerin 4.0 Triethanolamine 1.2 Tocopheryl Acetate 3.0 Floating paraffin 5.0 Squalane 3.0 Macadamia Nut Oil 2.0 Polysorbate 60 1.5 Sorbitan sesquioleate 1.0 Carboxyvinyl Polymer 1.0 Bietchiti 0.01 IDT-2N 0.01 Incense, preservative a very small amount Purified water to 100

Formulation Example 3: Nutrition Cream

Ingredient Parts by weight Niosome 10.0 Cetostearyl alcohol 2.0 Glyceryl Stearate 1.5 Trioctanoine 5.0 Polysorbate 60 1.2 Sorbitan stearate 0.5 Squalane 5.0 Liquid paraffin 3.0 Cyclomethicone 3.0 Bietchiti 0.05 Delta-tocopherol 0.2 Concentrated glycerin 4.0 1,3-butylene glycol 2.0 Xanthan Gum 0.1 IDT-2N 0.05 Incense, preservative a very small amount Purified water to 100

Formulation Example 4: Massage Cream

Ingredient Parts by weight Niosome 1.0 Propylene glycol 6.0 glycerin 4.0 Triethanolamine 0.5 Beeswax 2.0 Tocopheryl Acetate 0.1 Polysorbate 60 3.0 Sorbitan sesquioleate 2.5 Cetearyl Alcohol 2.0 Liquid paraffin 30.0 Carboxy Vinyl Polymer 0.5 Incense, preservative a very small amount Purified water to 100

Formulation Example 5: Pack

Ingredient Parts by weight Niosome 2.0 Propylene glycol 2.0 glycerin 4.0 Carboxyvinyl Polymer 0.3 ethanol 7.0 Fiji-40 Hydrogenated Castor Oil 0.8 Triethanolamine 0.3 Bietchiti 0.01 IDT-2N 0.01 Incense, preservative a very small amount Purified water to 100

As described above, the skin improvement cosmetic composition containing the present invention phytosphingosine (Phytosphingosine) and the stabilized upper limb extract inhibits the production of melanin, which is the main cause of pigmentation phenomenon, appearing around the eyes or under the eyes It improves wrinkles, decreases skin elasticity, etc. by improving phytosphingosine, which is excellent in anti-shadowing of symptoms and symptoms that do not seem healthy (Anti-shadow), and has excellent skin cell proliferation and blood circulation promoting effects. And it will be effective to improve the reliability.

Claims (5)

Contain niosome prepared by stabilizing the active ingredient using PIG-5-Soy sterol, Cholesteryl oleate and Ceramide 3 as a nonionic surfactant In the skin improvement cosmetic composition, The active ingredient is phytosphingosine (Phytosphingosine) and skin improvement cosmetic composition, characterized in that the upper limb extract. The method of claim 1, Skin improvement cosmetic composition, characterized in that the niosom is formulated in 0.05-20.0% by weight based on the total weight of the cosmetic. The method of claim 1, Skin improvement cosmetic composition, characterized in that blending niosomes in 0.1-10.0% by weight relative to the total weight of the cosmetic. The method of claim 1, Phytosphingosine (Phytosphingosine) and the upper extremity extract is a skin-improving cosmetic composition, characterized in that the formulation in each 0.01-5.00% by weight relative to the total weight of niosomes. The method of claim 1, Phytosphingosine (Phytosphingosine) and the upper extremity extract is a skin-improving cosmetic composition, characterized in that the formulation in each 0.1-2.0% by weight relative to the total weight of niosomes.