KR101965482B1 - Cosmetic composition for recovering damaged skin barriers and improving aged skin comprising Lactobacillus rhamnosus as an active ingredient - Google Patents

Abstract

The present invention relates to a cosmetic composition for improving skin barrier or improving skin aging comprising a fermentation broth of Lactobacillus rhamnosus as an active ingredient, wherein the Lactobacillus lambosus fermentation liquid of the present invention contains water It has the effect of increasing the retention amount and oil content, decreasing the transepidermal water loss (TEWL) and skin temperature of the skin, decreasing the melanin index, erythema index and skin roughness of the skin and increasing the skin elasticity, And for preventing or ameliorating skin aging, or as an external preparation for skin.

Description

[0001] The present invention relates to a cosmetic composition for recovering skin barrier or improving aging of skin comprising Lactobacillus rhamnosus fermentation broth as an active ingredient,

The present invention relates to a method for improving skin dryness, skin irritation, skin inflammation, excessive tingling of the skin and skin burning caused by damage to the skin barrier comprising Lactobacillus rhamnosus fermentation broth as an active ingredient, And to a cosmetic composition for preventing or improving skin wrinkles, skin pigmentation, erythema, skin roughness, skin sagging, reduced elasticity and wrinkles of skin, and external preparation for skin.

Skin is a dynamic organ of the body that protects body fluids from external leakage and penetration of harmful substances such as bacteria (Madison, 2003), and epidermis plays a central role in skin barrier function (Seo Young-jun, 2009 ). In the basal layer of the epidermis with the squamous stratified epithelium structure, keratinocytes are produced endlessly through cell division and differentiation (Yuki et al., 2007), and corneocytes are found in the superficial layer It forms a cornified cell envelope through the granule layer and crosslinks between the keratinocytes in the inside and covalent bond with the keratinocyte lipid in the stratum corneum. And a complete skin barrier (Hwang, Sangmin, et al., 2001). The keratinocyte and intercellular lipid are not only able to supply water with natural moisturizing factor (NMF), but also to form a bricks and mortar with stratified corneodesmosome (Madison, 2003) And also functions as an antimicrobial barrier against external harmful substances through UV filtering and pH control of the stratum corneum (Lee, Seung-heon, 1999). In addition, the tight junction (TJ) distributed in the granular layer and the upper part of the polar layer has intercellular adhesion function and various regulatory functions (Schneeberger & Lynch, 2004). In case of barrier layer of stratum corneum, TJ protein expression is increased, resulting in a secondary barrier function that blocks moisture and mass transfer between cell spaces (Benedetto et al., 2010).

This perfectly visible skin barrier is always exposed to the external environment, so it can not be free from physical and chemical damage such as chronic ultraviolet rays, heat and irritating coating agents (Seo Young-joon, 2009). Barriers may be weakened or impaired by internal factors such as increased glucocorticoid due to stress, chronic manifestations of cytokines and aging, or even long-term consumption of foods deficient in essential fatty acids , 2006).

When aging of the skin occurs due to the overlapping of extrinsic aging such as intrinsic aging and chronic ultraviolet exposure due to aging (Lee, Jeong-duk, 2006; Glogau, 1997) Although functional, structural, and biochemical changes appear, morphologically, there are different patterns in the thickness of the epidermis, roughness, wrinkle depth, and pigmentation pattern. However, overall skin permeability and immune function are decreased, And dryness (Lee, Jeong-duk, 2006).

Specifically, the volume of the dermal-epidermal junction gradually becomes flattened (Fenske & Lober, 1986) and the macrofibril, which transmits the forces between the epidermis and the epidermis, decreases (Kadoya et al ., 2005 ). For this reason, not only the elasticity of the skin, but also the capillary blood vessels distributed in the skin and the skin are enlarged or weakened (Yeon-cheol, Lee, Moo-hyung, 2006). Furthermore, the concentrations of proteoglycan and hyaluronic acid (HA), which are extracellular matrix (ECM) in the dermis, are decreased, and the TEWL of the epidermis is also increased, resulting in a decrease in the hydration degree of the dermis and epidermis. In addition, the production and exchange rate of keratinocyte decreased, ultimately delaying the keratinization cycle of keratinocytes (Lee, Hee Kyung et al., 2006). Langerhans cells are reduced and melanocyte maturation and dispersion are uneven, leading to increased susceptibility to inflammation due to decreased immune function, and to a lack of skin tone (Weiss et al ., 2002;

In addition, photoaging increases the level of reactive oxygen species (ROS) in the cell and impairs skin's oxidative defense function (Glogau, 1997), increases the amount of matrix metalloproteinases (MMPs) that degrade extracellular matrix proteins And lipid peroxidation, resulting in abnormal cross-linking of collagen and elastin, chain cleavage, and HA chain cleavage (Kim, Ki-Young et al., 2004).

The milk is a report of a balanced nutrition and protein of milk and calcium mucosal cells promote absorption and sedation (Ca ^{2 +),} the fat-soluble vitamins, and vitamin B group contained in milk fat is keeping skin healthy (Kim, Lee et al., 2011). Fatty acids in milk fat contribute to improving skin's suppleness and skin's immune function by controlling antimicrobial and sebaceous secretions (Nakatsuji et al ., 2010). In addition, lecithin, which is a phospholipid, and ganglioside, which is a glycolipid, are also contained in the milk fat, thereby enhancing immunity and cell activity (Fox & McSweeney, 2007). In particular, in milk cream, which is a cream layer of the oil-in-water emulsion, fat-soluble nutrients such as lecithin and anti-dermatitis substances are significantly increased (Kim, Yoo Yoo, 2011; Jung Kwangyong, 2011).

Milk or oil cream lactic acid bacteria (lactic acid bacteria; LAB) geochimyeon the fermentation process antioxidant properties, as well as induce sebum control and moisture or are produced are materials that strengthen the vascular (Kang Tae Jin, 2009) increases and the absorption of Ca ^{2 +} concentrations (Kim, Young-Yoo, 2011; Jung, Kwang-yong, 2011). In addition, the constituents of the lactic acid bacteria culture fluid are similar to the natural moisturizing factor (NMF) components, thereby inducing moisturization and glazing on the skin (Moon, Hongseok, 2001, Kang Tae-jin, 2009).

In particular, Lactobacillus lan- nomus has an excellent acid-producing and antibiotic capacity, which helps the immune system (Silva et al., 1987) and is also very low in human toxicity (Princea et al ., 2012). In addition, it has antioxidative properties and has been shown to be effective in the treatment of anti-dermatitis when applied to the skin (Korpela et al ., 1997; Marschan et al ., 2008). In particular, Lactobacillus lan- nomase disruption has been reported to have a higher antioxidant potential than other LABs (Choi et al., 2013). Lactobacillus lamb- nosus in fermented milk also helps to improve cell viability by controlling intracellular pH The research on the efficacy of skin for milk and lactic acid bacteria has been carried out by applying various methods such as application to skin cells or animal skin. However, there is no known effect of the skin barrier recovery and the aging skin appearance improvement effect of the cosmetic composition containing the Lactobacillus laminosis fermentation liquid using the milk cream as a fermentation substrate.

Accordingly, the present inventors have made efforts to develop a cosmetic composition that is safe for human body and has no side effects and has an effect of improving skin barrier recovery and aging skin appearance. As a result, it has been found that lactose- The Bacillus lambsus fermentation broth is activated during the fermentation process to combine the fatty acids, organic acids, and fat-soluble nutrients in the milk, to stabilize the NMF and to maintain the homeostasis of the calcium gradient, resulting in skin dryness, skin irritation, Inflammation, excessive tingling of the skin, and burning of the skin, and shows significant effects on skin aging patterns such as skin roughness, skin pigmentation, erythema, skin roughness, skin sagging, elasticity reduction and skin wrinkles Thus, the milk cream Lactobacillus lanxosus fermentation solution of the present invention can be used for skin barrier protection, The skin by, for recovery of the barrier, and confirmed that this can be effectively used as an active ingredient for preventing or improving skin aging composition and completed the present invention.

Korean Society of Food Science and Technology. Food Science and Technology. Seoul, Kwangil Publishing Co. However, (2011) Effect of natural cosmetics on skin condition. Korean Society of Cosmetic Arts, 5 (2), 57-64 Sung Hwang, Ahn Seong - gu, and Seung Heon Lee. (2001) Influence of epidermal calcium gradient on differentiation of keratinocytes. Korean Journal of Dermatology, 39 (4), 389-401 Fox PF and McSweeney PLH. Jeon Woo Min, Kang Shin Ho, Kim Se Heon, Moon Yong Il, Park Dong Joon, Lim Ji Young and Han Kyung Sik. (2007) Biochemistry of Milk and Dairy Products. Seoul, Life Science, pp. 62-361 Alam M, White LE, Martin N, Witherspoon J, Yoo S and West DP. (2010) Ultrasound tightening of facial and neck skin: A rater-blinded prospective cohort study. J. Am. Acad. Dermatol., 62 (2), 262-269 Andersen JL, Gniadecka M, Olivarius FF, Dahlstrom K and Wulf HC. (1998) Skin temperature of UV-induced erythema correlated to laser Doppler flowmetry and skin reflectance measured redness. Skin Res. Technol., 4 (1), 41-48 Barlow T and Wiechers J. (1999) Measuring skin hydration. Cosmetics & Toiletries, 114 (12), 47-53 Benedetto, Rafaels NM, McGirt LY, Ivanov AI, Georas SN, Cheadle C, Berger AE, Zhang K, Vidyasagar S and Yoshida T et al. (2011) Tight junction defects in patients with atopic dermatitis. J. Allergy Clin. Immunol., 127 (3), 773-786 (e7) Buraczewska I, Berne BM, Lindberg HT and Loden M. (2007) Changes in skin barrier function following a long-term treatment with moisturizers, a randomized controlled trial. Br. J. Dermatol., 156 (3), 492-498 JH, Seo JY, Kim YK, Lee SR, Kim KH, Cho KH, Eun HC and Chung JH. (2005) Heat Modulation of Tropoelastin, Fibrillin-1, and Matrix Metalloproteinase-12 in Human Skin In Vivo. J. Invest. Dermatol., 124 (1), 70-78 Elisa PM and Menon GK. (1991) Structural and lipid biochemical correlates of the epidermal permeability barrier. Adv. Lipid Res., 24, 1-26 Glogau RG. (1997) Phygologic and structural changes associated with aging skin. Dermatol Clin, 15 (4), 555-559 Kurban RS and Bhawan J. (1990) Histologic Changes in Skin Associated with Aging. J Dermatol Surg Oncol, 16 (10), 908-914 (2009) Isolation, identification, and characterization of small bioactive peptides from Lactobacillus GG, which exert both anti-Gram-negative and Gram-positive bactericidal activity . J. Pediatr. Gastroenterol. Nutr., 49 (1), 23-30 Madison KC. (2003) Barrier Function of the Skin: "La Raison d'Etre" of the Epidermis. J. Invest. Dermatol., 121 (2), 231-241 Marschi E, Kuitunen M, Kukkonen K, Poussa T, Sarnesto A, Haahtela T, Korpela R, Savilahti E and Vaarala O. (2008) Probiotics in infancy induce protective immunological profiles that characterize chronic low-grade inflammation. Clin. Exp. Allergy, 38 (4), 611-618 Marzio L, Centi C, Cinque B, Masci S, Giuliani M, Arcieria, Zicari L, De Simone C and Cifone MG. (2003) Effect of the lactic acid bacterium Streptococcus thermophilus on stratum corneum ceramide levels and symptoms of atopic dermatitis patients. Exp. Dermatol., 12 (5), 615-620 Nakatsuji T, Kao MC, Zhang L, Zouboulis CC, Gallo RL and Huang CM. (2010) Sebum Free Fatty Acids Enhance the Innate Immune Defense of Human Sebocytes by Upregulating β-Defensin-2 Expression. J. Invest. Dermatol., 130 (4), 985-994 Rabe JH, Mamelak AJ, McElgunn PJS, Morison WL and Sauder DN. 2006 Photoaging: mechanisms and repair. J. Am. Acad. Dermatol., 55 (1), 20-21 Schneeberger EE and Lynch RD. (2004) The tight junction: a multifunctional complex. Am. J. Physiol. Cell Physiol., 286 (6), 1213-1228 Sørensen LH, Pedersen KT and Maibach HI. (1993) Equation for conversion of transepidermal water loss (TEWL) to a common reference temperature: what is the slope ?. Contact Derm., 29 (5), 280-281 Spencer T.S. (1976) Water and the horny layer. J Soc Cosmet Chem, 27, 63-72 Thune P, Nilsen T, Hanstad IK, Gustavsen T and Lovig DH. (1988) The water barrier function of the skin in relation to the water content of stratum corneum, pH and skin lipids. The effect of alkaline soap and syndet on dry skin in elderly, non-atopic patients. Acta Derm. Venereol, 68 (4), 277-283 Yuki T, Haratake A, Koishikawa H, Morita K, Miyachi Y and Inoue S. (2007) Tight junction proteins in keratinocytes: localization and contribution to barrier function. Exp. Dermatol., 16 (4), 324-330 Zhang L, Seitz LC, Abramczyk AM and Chan C. (2010) Synergistic effects of cAMP and palmitate in promoting altered mitochondrial function and cell death in HepG2 cells. Exp. Cell Res., 316 (5), 716-727

It is an object of the present invention to provide a method for improving skin dryness, skin irritation, skin inflammation, excessive tingling of the skin and skin burning caused by damage to the skin barrier containing Lactobacillus lambosus fermentation broth as an active ingredient, And to provide a cosmetic composition for improving skin roughness, skin pigmentation, erythema, skin roughness, skin sagging, reduced elasticity and wrinkles of skin, and external preparation for skin.

In order to achieve the above object, the present invention provides a cosmetic composition for improving skin comprising an Lactobacillus laminocus fermentation broth as an active ingredient.

Further, the present invention provides a skin external preparation for improving skin comprising as an active ingredient a lactobacillus lanxos fermentation broth.

In addition, the present invention provides a cosmetic composition for skin improvement comprising a milk fermentation broth containing Lactobacillus Lymphosus strain as an active ingredient.

The present invention also provides a skin external preparation for skin improvement comprising a milk fermentation broth comprising Lactobacillus lambosus strain as an active ingredient.

The present invention also provides a cosmetic composition for improving skin comprising an oil-in-milk fermentation broth containing Lactobacillus lansosus strain as an active ingredient.

In addition, the present invention provides a skin external preparation for skin improvement comprising an oil-in-milk fermentation broth comprising Lactobacillus lambosus strain as an active ingredient.

The Lactobacillus lanxosus fermentation solution of the present invention increases the moisture retention and oil retention of the facial or neck skin, reduces the transepidermal water loss (TEWL) and skin temperature of the skin, and decreases the skin pigmentation, erythema, skin roughness and elasticity It can be effectively used as a cosmetic composition for restoring the skin barrier or for restoring the damaged skin barrier and for preventing or improving skin aging, or as an external preparation for skin.

Brief Description of the Drawings Fig. 1 is a graph showing the effect of the lactobacillus lanxos fermentation broth of the present invention on the moisture retention amount, oil retention amount, TEWL and skin surface temperature of the facial skin.
2 is a graph showing the effect of the Lactobacillus laminocus fermentation broth of the present invention on the melanin, erythema, roughness and elasticity of the facial skin.
FIG. 3 is a graph showing changes in the facial skin before and after the test of a clinical subject treated with the lactobacillus laminosse oil cream fermentation liquid of the present invention.
FIG. 4 is a graph showing the effects of the lactobacillus lanxus fermentation broth of the present invention on moisture retention, oil retention, TEWL, melanin, roughness and elasticity of the neck skin.
FIG. 5 is a graph showing changes in the neck and neck of a clinical subject treated with the lactobacillus rhamnosus oil cream fermentation liquid of the present invention before and after the test.

Hereinafter, the present invention will be described in detail.

The present invention provides a cosmetic composition for skin improvement comprising a fermentation broth of Lactobacillus rhamnosus as an active ingredient.

Preferably, the Lactobacillus lambosus strain is a strain that is phylogenetically classified as Lactobacillus laminocus, more preferably a lactobacillus lambus strain derived from a human face such as a human face or a human mouth and a milk such as milk or cheese, Most preferably, Lactobacillus lambusus KCTC 5033, KCTC 3237, KCTC 5046, KCTC 5510, KCCM 11320, KCCM 32823, KCCM 32826, KCCM 40069, ATCC 9595, ATCC 14957, ATCC 21052, KCTC 10965BP or RA-32 It does not.

The fermentation broth means a dried product obtained by culturing Lactobacillus laminocus in a culture medium, a culture concentrate, a dried product of the culture broth, a culture filtrate, a concentrated culture filtrate, or a culture filtrate. Or a culture filtrate obtained by removing the strain after culturing. The culture is not limited in its formulation, and may be, for example, a liquid, an emulsion, or a solid.

Preferably, the fermentation broth is preferably a fermentation broth in which Lactobacillus laminocus is cultured in an MRS medium, or a fermentation broth in which lactobacillus lambosus is inoculated into milk or a milk cream, and is produced as follows But is not limited thereto.

1) pre-culturing Lactobacillus laminocus to prepare a culture;

2) Inoculating the Lactobacillus laminocyte culture with MRS, milk or milk cream, and culturing the mixture at 35 to 40 ° C for 60 to 80 hours to prepare a milk fermentation broth or a milk cream fermentation broth.

The culture medium of step 1) above means a culture solution obtained by culturing Lactobacillus laminocus in a culture medium (MRS broth), a concentrate culture, a dried product of the culture solution, a culture filtrate, a concentrated culture filtrate, or a culture filtrate Which may include the above strain or a culture filtrate obtained by removing the strain after cultivation.

The milk of step 2) may be non-fat milk, low-fat milk added with not more than 3 parts by weight of milk fat, milk milk or skimmed milk, and the milk cream may contain not less than 3 parts by weight of milk fat separated from crude oil or milk It is preferably a milk cream.

The cultivation in step 2) is preferably carried out at 35 to 40 DEG C for 60 to 80 hours, more preferably at 36 to 38 DEG C for 65 to 75 hours, more preferably at 36 to 38 DEG C for 72 hours Most preferably, it is not limited thereto.

It is preferable that the skin is a skin having a barrier or an aging skin.

The fermentation broth of Lactobacillus laminosus, preferably Lactobacillus laminosus milk cream, increases the moisture retention and oil retention of the facial or neck skin, reduces transepidermal water loss (TEWL) and skin temperature of the skin, It shows the effect of improving deposition, erythema, skin roughness and elasticity.

The skin changes in accordance with the skin barrier damage according to the present invention include skin dryness, skin irritation, skin inflammation, excessive tingling of the skin, and skin burning, and the aging pattern of the skin includes skin rash, skin pigmentation, erythema, Skin roughness, skin sagging, reduced elasticity, and wrinkles of the skin.

In a specific embodiment of the present invention, the present inventors prepared formulations such as toners, lotions and the like, respectively, using a lactobacillus laminocyte culture medium and milk or milk cream fermentation broth (see Tables 1 to 4).

In addition, after collecting the clinical test group for the present inventors, it was found that there was no significant difference between the test groups in terms of the skin condition homogeneity before the test for the accuracy of the test before the test, (See Table 5, Table 6, and Table 7).

In order to confirm the skin barrier recovery effect of the Lactobacillus laminocus fermentation broth, the present inventors measured the moisture retention, oil retention, TEWL and skin temperature after applying the Lactobacillus laminosis fermentation broth to clinical subjects. As a result, It has been confirmed that the fermentation broth of laminocus increases the moisture retention and oil content of the facial skin, decreases the TEWL and skin temperature of the skin, and in particular, the fermentation broth of the Lactobacillus laminosus milk cream exhibits a remarkable skin barrier recovery effect (Tables 8-19 , And Fig. 1).

In order to confirm the effects of skin pigmentation, erythema, skin roughness and elasticity improvement which are typical examples of aged skin of Lactobacillus laminocus fermentation broth, the inventors of the present invention have found that the Lactobacillus laminosis fermentation broth can be applied to the face and neck skin of a clinical subject After the application, the melanin index, the erythema index, the roughness and the degree of elasticity change were examined. As a result, the Lactobacillus laminosis fermentation liquid showed the effect of improving the pigmentation, erythema and elasticity of the skin. Especially, the Lactobacillus lambsus milk cream fermentation broth had remarkable skin complexion And the elasticity improving effect (see Figs. 2 and 3).

In order to confirm the effect of improving the neck skin of Lactobacillus laminocus fermentation broth, the present inventors measured the moisture content, oil content, TEWL, melanin, roughness and elasticity of the neck skin after applying the Lactobacillus laminosis fermentation broth to the clinical subjects As a result, Lactobacillus lanxos fermentation broth has an effect of increasing moisture retention and oil retention, decreasing TEWL of skin, improving skin pigmentation, erythema and elasticity, and in particular, Lactobacillus lanomyos milk cream fermentation broth (Fig. 4 and Fig. 5).

Accordingly, the Lactobacillus lanxosus fermentation broth of the present invention has an effect of increasing the moisture retention amount and oil retention amount of the neck or face skin, decreasing the TEWL and skin temperature of the skin, improving the skin pigmentation, erythema and elasticity , For restoring skin barrier or for improving skin aging.

The cosmetic composition according to the present invention may be in the form of a solution, suspension, emulsion, paste, gel, cream, lotion, powder, soap, surfactant-containing cleansing, oil, powder foundation, emulsion foundation, wax foundation, ≪ / RTI >

The cosmetic composition according to the present invention may be prepared into any of the formulations conventionally produced in the art, for example, a solution, a suspension, an emulsion, a paste, a gel, a cream, a lotion, a powder, a soap, But are not limited to, cleansing, oil, powder foundation, emulsion foundation, wax foundation, and spray. More particularly, when the composition of the present invention is used as a cosmetic composition, a cosmetic preparation is selected from cosmetic lotion, emulsion, cream, essence, gel, pack and cleansing cream; Makeup cosmetics such as foundation, and the like.

When the formulation of the present invention is a paste, cream or gel, an animal oil, vegetable oil, wax, paraffin, starch, tracant, cellulose derivative, polyethylene glycol, silicone, bentonite, silica, talc or zinc oxide may be used as the carrier component .

When the formulation of the present invention is a powder or a spray, lactose, talc, silica, aluminum hydroxide, calcium silicate or polyamide powder may be used as a carrier component. In the case of a spray, in particular, / Propane or dimethyl ether.

When the formulation of the present invention is a solution or an emulsion, a solvent, a dissolving agent or an emulsifying agent is used as a carrier component, and examples thereof include water, ethanol, isopropanol, ethyl carbonate, ethyl acetate, benzyl alcohol, benzyl benzoate, , 3-butyl glycol oil, glycerol aliphatic ester, polyethylene glycol or sorbitan fatty acid esters.

In the case where the formulation of the present invention is a suspension, a carrier such as water, a liquid diluent such as ethanol or propylene glycol, a suspending agent such as ethoxylated isostearyl alcohol, polyoxyethylene sorbitol ester and polyoxyethylene sorbitan ester, Cellulose, aluminum metahydroxide, bentonite, agar or tracant, etc. may be used.

When the formulation of the present invention is a surfactant-containing cleansing, the carrier component may include aliphatic alcohol sulfate, aliphatic alcohol ether sulfate, sulfosuccinic acid monoester, isethionate, imidazolinium derivative, methyltaurate, sarcosinate, fatty acid amide ether Alkylamido betaine, aliphatic alcohol, fatty acid glyceride, fatty acid diethanolamide, vegetable oil, lanolin derivative, or ethoxylated glycerol fatty acid ester.

In addition, the cosmetic composition of the present invention may contain other ingredients such as oil, water, a surfactant, a moisturizer, a lower alcohol, a thickener, a chelating agent, a coloring agent, an antiseptic, May be appropriately used in combination.

For example, besides the fermentation broth according to the present invention, the number of softening times may be adjusted to 1 to 10 wt% of polyhydric alcohols (propylene glycol, glycerin, etc.) and 0.05 to 2 wt% of a surfactant (polyethylene oleyl ether, polyoxyethylene hardened castor oil, etc.) Can be manufactured. The nutritional lotion and nutritional cream may contain 5 to 20% by weight of oils (squalane, petrolatum, octyldodecanol, etc.) and 3 to 15% by weight of wax components (cetanol, stearyl alcohol, And the essence may be prepared by adding 5 to 30% by weight of polyhydric alcohols such as glycerin, propylene glycol and the like in addition to the fermentation liquid according to the present invention. In addition to the fermentation broth according to the present invention, the massage cream contains 30 to 70% by weight of oils such as liquid paraffin, petrolatum, isononylisononanoate, etc., and the pack contains 5 to 20% by weight of polyvinyl alcohol, A washout pack containing 5 to 30% by weight of a pigment such as kaolin, talc, zinc oxide, titanium dioxide or the like in addition to the culture medium of the present invention in a peel off pack or general emulsifiable cosmetic containing the above- .

Further, the present invention provides a skin external preparation for skin improvement comprising a lactobacillus Laminocus fermentation broth as an active ingredient.

The Lactobacillus lanxosus fermentation broth of the present invention has an effect of increasing the moisture retention amount and oil content of the neck or face skin, decreasing the TEWL and skin temperature of the skin, improving the skin pigmentation, erythema and elasticity, It can also be useful as a skin external preparation for barrier restoration or aging skin improvement.

For skin barrier recovery or aging skin improvement, it is important to choose a suitable topical formulation. Thus, the lactobacillus lan- myus fermentation broth can be produced with an ointment so that it can be effectively applied to the affected part. The ointment preparation is prepared by combining the lactobacillus lanxosus fermentation broth of the present invention with an inorganic substance and coating it with a liposoluble base. The inorganic material is preferably a material having excellent antimicrobial activity, anti-inflammatory effect, epidermal regeneration effect, etc. Specific examples thereof include zinc oxide, zinc carbonate, iron oxide and the like. Further, it is preferable to further use a ceramic carrier capable of safely impregnating the composition of the present invention. As the ceramic carrier, zeolite, talc, gypsum, mortar and mixtures thereof are preferably used. Such a ceramic carrier is excellent in the impregnation property of the water-soluble component, so that the water-soluble component can be smoothly supplied to the skin.

In addition, the present invention provides a composition for improving skin barrier or improving skin aging comprising the fermentation broth of Lactobacillus rhamnosus milk cream as an active ingredient, or an external preparation for skin.

The fermentation broth prepared by inoculating the lactobacillus lambosus of the present invention with milk cream increases the moisture retention and oil retention of the neck or facial skin, decreases the TEWL and skin temperature of the skin, and improves skin pigmentation, erythema and elasticity , It can be effectively used as a cosmetic composition for restoring skin barrier and for improving skin aging, or as an external preparation for skin.

Hereinafter, the present invention will be described in detail with reference to Examples and Experimental Examples.

However, the following examples and experimental examples are merely illustrative of the present invention, and the content of the present invention is not limited to the following examples and experimental examples.

< Example  1> Lactobacillus Lambrosse  Preparation of strain, culture thereof and fermentation broth thereof

<1-1> Lactobacillus Lambrosse  Preparation of strain and its culture

1 × 10 ⁶ cfu / ml of Lactobacillus rhamnosus strain (Accession No. KCTC 5033) pre-cultured in 1 L of MRS medium was inoculated and cultured at 37 ° C. for 24 hours.

<1-2> Lactobacillus Lambrosse  Preparation of strain fermentation broth

When MRS broth was used as the main culture medium, the pre-cultured L. rhamnosus culture was inoculated at 1% and cultured at 37 ° C for 72 hours to obtain a MRS culture broth. When milk and milk cream were used as the main culture medium, they were sterilized at 120 ° C for 20 minutes, then inoculated 1% of the pre-cultured L. rhamnosus culture and incubated at 37 ° C for 72 hours in a fermentation broth &Lt; / RTI &gt;

&Lt; 1-3 > Various Lactobacilli Production of a milk cream fermentation broth using Laminoscase strain

KCTC 5033 (D1), KCTC 5046 (D2), KCTC 5510 (D3), KCCM 11320 (D4), KCCM (D5), KCCM 32826 (D6), KCCM 40069 (D7), ATCC 9595 (D8), ATCC 14957 (D9), or ATCC 21052 (D10), KCTC 10965BP (C-IND, Changshin science, Korea) for 72 hours at 37 ° C under a constant temperature condition to obtain a fermented milk cream lan- myosus solution.

< Example  2> Lactobacillus Lambrosse  Using the strain Foolish  Produce

In the test group of the present invention, L. rhamnosus was cultivated in distilled water (control group; C group), non-fermented milk group (M group), sterilized milk cream (MC group) and MRS broth (MRS group), milk fermentation broth fermented with sterilized milk (FM group), and milk cream fermentation broth fermented with sterilized milk cream (FMC group). Toner, lotion or the like, and then clinical studies were conducted.

<2-1> The test group  Manufacture of used toner

The toner to which the corresponding undiluted solution was added according to each test group was agitated while sequentially adding the A-phase of [Table 1] to the disinfected beaker according to the composition ratios shown in Table 1 below. The phases were heated to 60 &lt; 0 &gt; C. The A-phase was put into a W-phase, and emulsified with a homo mixer (2,000 rpm) for 3 minutes to prepare a toner. The completed toner was filled in an ethanol-sterilized spray container and then stabilized at room temperature for 24 hours. However, in the case of Group C, distilled water was used instead of the test solution.

<2-2> The test group  Manufacture of used lotion

The lotion added with the corresponding raw solution according to each test group was added to the W-phase corresponding to each disinfected beaker according to the composition of [Table 2], and the O phase was added at 60 ° C after 70 ° C (O / W type emulsion control) after the contents were completely melted. The mixture was stirred with a homomixer (3,000 g / L) until the formulation was cooled to 40 ° C, rpm), A phase was added, and the mixture was stirred with a homomixer (2,000 rpm) for 3 minutes to prepare a lotion. The completed lotion was filled into an ethanol disinfected dispenser container and then stabilized at room temperature (23 ± 2 ° C) for 24 hours.

<2-3> Production of sun lotion

In order to prevent the skin changes that may occur due to the external environment such as ultraviolet irradiation during the test group and to make the test group homogeneous during the test period, prepare a sunscreen according to the composition ratio of [Table 3] Physical blockers were added. W and O phases were added to each disinfected beaker and heated to 70 ° C to completely dissolve the contents. The W phase was added to the O phase and stirred with a W / O type emulsion control The emulsion was emulsified with a homomixer (3,000 rpm) until the formulation was cooled to 40 DEG C, and the A phase was added successively, followed by stirring with a homomixer (2,000 rpm) for 3 minutes to prepare a sun lotion. The completed sun lotion was charged to an ethanol-sterilized dispenser vessel and then stabilized at room temperature (23 ± 2 ° C) for 24 hours.

<2-4> Cleanser's  Produce

To prevent skin changes that may occur with different cleansers during the application of the test group, a cleanser was prepared according to the composition ratios in Table 4 for the homogeneity of the test groups during the test period, and a naturally occurring low-activity surfactant was used. The A phase was added in turn, and the mixture was stirred. Then, the S phase was added to the A phase one by one, and the mixture was stirred without bubbling to produce a cleanser. The completed cleanser was filled into an ethanol-sterilized foam-forming container and then stabilized at room temperature (23 ± 2 ° C) for 24 hours.

< Example  3> Selection of subjects for clinical trial

Among the women aged 40 to 59, who have not received any special medical treatment or taking medication within the last 6 months, the participants who did not give any physical stimulation to the skin, such as dermatology, were selected as the first test subjects . The subjects of the first test should be explained in detail with the purpose and contents of the clinical study and then taken together with the health supplement and other medicines such as blood circulation and antioxidants which may cause a significant change in skin during the test, Only one person who agreed to the study, including not using any other cosmetics other than one UV blocker, and not doing any procedures or skin care that directly affect skin change, was selected as the final test subject.

A total of 68 participants were randomly assigned to 5 control subjects, 12 non-fermented subjects in each group, and 13 subjects in 3 groups of fermentation liquids in the order of written consent. A total of 59 subjects were selected for the final selection, except for the 9 patients who were excluded due to inappropriate use of cosmetic products other than the test product or long-term use of the product due to travel, etc. Fifteen patients in the C group, 9 patients in the M group, 12 patients in the MC group, 9 patients in the MRS group, 11 patients in the FM group, and 13 patients in the FMC group were included. The duration of the study was 7 weeks (49 days).

< Example  4> How to measure skin change

<4-1> Image capture

Before and after the clinical study, the front and side of the facial region of the subject were photographed using a digital camera (VLUU PL150, SAMSUNG, Korea) for the visual observation of the skin changes of the clinical subjects participating in the present invention. In order to obtain the same results, the test group before skin entry into the skin test room was cleaned with the same cleanser supplied at the time of supply, and one person of the same person photographed the image at the designated location.

<4-2> Measurement using a skin meter

(C + K electronic GmbH, Koln, Germany), a multi-function integrated sensor system equipped with a sensor for room condition (SRC100) for measuring the temperature and humidity conditions of the laboratory environment, Were used. In addition, in the clinical test of the present invention, a corneometer (CM825) for measuring moisture content, a sebumeter (SM815) for measuring oil content, a tewameter (TM300) for measuring TEWL, a skin thermometer (ST500) Mexameter (MX18) for measuring erythema index, Frictiometer (FR700) for measuring skin roughness using skin friction coefficient, and Cutometer 580 for measuring skin elasticity. The above measurements were taken five times in total and the average was taken as the final value. In addition, it was set to 20 ~ 25 ℃, relative humidity of 40 ~ 60%, which is the optimal temperature and humidity condition for measuring the exact condition of skin. After entering the skin measuring room, Respectively.

The measurement site for the change of the facial skin is divided into three parts: the forehead, which is the mid point between the center of the bamboo and the vertical line of the hair line, the part from the pupil to the vertically downward part, The right part of the eye and the right part of the eye were selected. To measure the change of the neck skin, the measurement site was 2 parts, The neurogenic response was most pronounced, the softness and smoothness of the muscles and skin were reported to be restored, and the bone marrow was selected as the posterior segment and evaluated at each site after 7 weeks of use.

< Experimental Example  1> Lactobacillus Lambrosse  Protecting skin barrier and recovery effect of fermentation liquid

<1-1> Identification of facial skin condition of clinical subjects before test

In order to confirm whether or not the skin barrier of the facial skin is protected or restored to the test subjects selected in the above <Example 3>, in order to confirm the homogeneity of the facial skin condition of the subject before the test, Were used to measure the water retention, oil retention, TEWL, and skin surface temperature of the facial skin before each test.

As a result, as shown in Table 5, there was no significant difference between the test groups in moisture retention, oil retention, TEWL, and skin surface temperature, and thus homogeneity was verified (Table 5).

<1-2> Test group  apply

The toner, lotion, sun lotion and cleanser prepared in Example 2 were supplied to clinical subjects in the same manner and used twice a day in the morning and evening. However, in the morning, after applying the toner and lotion separately, make sure to apply the sun lotion with a sufficient amount.

<1-3> Confirmation of moisture content

The moisture in the stratum corneum resilience and softens the skin (Spencer, 1976). This moisture retention is determined internally by NMF, which is a component that includes water holding capacity (WHC) and hygroscopicity (HGS) (Pyeong Chan et al., 1988) (2006). In this paper, we propose a new methodology to solve this problem. Therefore, in the present invention, moisture content measurement before and after the test was also carried out to confirm whether the fermentation liquid of milk cream L. rhamnosus could act as such an external factor and protect the moisture barrier of the skin surface.

As a result, as shown in Fig. 1, the average moisture content of the control group C tended to decrease by 0.17% from 59.12 (M) before the test to 59.02 (M) after the test, while the group M of the non- The MRS group showed a tendency to increase by 0.55% to 61.62 (M) after the test and to 59.98 (M) before the test and to 60.93 (M) after the test in the MC group. ), And the FM group tended to increase by 4.38% from 62.84 (M) before the test to 65.60 (M) after the test. In particular, the FMC group showed 58.17 (M) , And 67.83 (M) after the test (16.59%) (Fig. 1).

<1-4> Oil reserves  Confirm

Skin lipid plays an important role in preventing skin irritation and micro-water evaporation, thus acting as a barrier to maintaining the moisturizing condition of the stratum corneum, neutralizing skin acidity, germicidal power, and delaying skin aging (Eun-Young Choi, 2006; &Amp; Menon, 1991). The lipid of the skin is formed by sebum component secreted from the sebaceous gland and lipid component secreted from the stratum corneum during the keratinization process, or by applying cosmetics, topical application, etc. to the skin (Kang Ho Jeong, 1996). In addition, an increase in oil retention in normal or dry skin not only protects the water barrier by lowering the TEWL with moisture retention, but also acts as an important factor in delaying skin aging (Thune et al., 1988) It is known that aged epidermis can be applied to restore the skin barrier by applying an appropriate mixture of epidermal lipid components (Kim, 2006) or by applying either one of them (Lee, Jeong-duk, 1999 ). Therefore, in order to evaluate whether the test group of the present invention is effectively protecting or restoring these lipid barriers, measurement of oil content was carried out before and after the test.

As a result, as shown in Fig. 1, the average amount of oil in the control group C tended to decrease by 3.76% from 70.80 (M) before the test to 68.13 (M) after the test. M group of the non- (M) and 68.59 (M), respectively, and the MC group showed a significant increase of 8.57% from 70.72 (M) before the test to 76.77 (M) after the test. The MRS group showed a decrease of 4.25% from 69.66 (M) before the test to 66.70 (M) after the test, while the FM group showed a decrease of 5.42% from 69.24 (M) before the test to 73.00 , And the FMC group showed a significant increase of 15.44% from 67.05 (M) to 77.41 (M) after death (Fig. 1).

<1-5> TEWL (trans epidermal water loss)

TEWL refers to the amount of water lost through passive diffusion of water in the body through the skin as the most commonly used measurement tool to address skin barrier damage and recovery (Byeonki, 1996) (Lee, Seong-heon, 1999). This water is known to be preserved by moisture permeability barrier and NMF (Barlow & Wiechers, 1999). Therefore, in the present invention, TEWL was measured before and after the test in order to examine whether the fermented milk cream L. rhamnosus similar to the epidermal lipid and the NMF component can effectively preserve the moisture by reducing the TEWL of aging skin.

As a result, as shown in FIG. 1, the TEWL of the control group C tended to increase by 6.22% from 17.86 (M) before the test to 18.98 (M) after the test. M group of the non- (M), and the MC group showed a slight decrease of 0.89% from 16.83 (M) before the test to 16.67 (M) after the test. The FM group showed a tendency to decrease by 9.09% from 16.73 (M) before the test to 15.20 (M) after the test, while the FMC group showed a decrease of 16.40 (M) before the test M) and a significant decrease of 23.41% (12.55 (M)) after the test (FIG. 1).

In addition, as shown in FIG. 3C, this result was also confirmed in the visual evaluation of the TEWL before and after the test of the clinical subjects belonging to the FMC group. The TEWL value before the test was very high (average 16.7) And the skin was rough and irritated. The wrinkles and mouths of the wrists were rough and dry, accompanied with erythema, and the skin of the jaws was flattened and sagged. However, after 7 weeks of testing, it was found that the rough, rough skin such as balls, wrinkles, and mouth area changed to smooth and shiny skin, and the erythema disappeared and the elasticity of skin increased to make the ball and jaw line smooth 3c).

<1-6> Confirmation of skin surface temperature change

In order to maintain the homeostasis of body temperature corresponding to the external temperature, not only the stratum corneum present in the outermost layer of the skin has a primary defense function from external physical and chemical stimuli (Lee, Seung-Heon, Change the temperature from time to time (Andersen et al., 1998). Increased surface temperature of the skin accelerates the reduction and collapse of collagen and elastin, accelerating skin aging (Chen et al. 2005) and increasing the TEWL of the elevated area (Kim, 2006; , Sørensen et al., 1993), leading to the collapse of the skin barrier. Thus, the present invention analyzed the changes in the surface temperature of the facial skin of a clinical subject treated with each test group.

As a result, as shown in FIG. 1, the control group, C, showed an increase of about 2.49% from 32.14 (M) before the test to 32.94 (M) after the test. In the case of the non-fermented solution group, the tendency was increased by about 1.05% from 32.16 (M) before the test to 32.51 (M) before the test, and from 32.06 (M) before the test to 33.07 3.12% It was confirmed that the skin surface temperature was significantly increased. On the other hand, in the case of the MRS group as the fermentation broth, the skin surface temperature tended to increase by about 0.56% from 32.15 (M) before the test to 32.34 (M) after the test. On the other hand, in the FM group of the fermented broth which showed a tendency to decrease in TEWL, the fermentation broth tended to decrease by about 0.09% from 32.06 (M) before the test to 32.02 (M) After the test, the skin surface temperature was significantly lowered to about 0.56% at 31.94 (M) (FIG. 1).

< Experimental Example  2> Lactobacillus Lambrosse  Confirmed the improvement effect of fermentation liquid on skin aging

<2-1> Identification of facial skin status of clinical subjects before test

In order to confirm the anti-aging effect of the facial skin on the test subjects selected in the above <Example 3>, in order to confirm the similarity of the facial skin condition of the clinical subjects before the test, The pre - test melanin index, erythema index, skin roughness and skin elasticity were measured for each clinical subject.

As a result, as shown in Table 6, there was no significant difference between the test groups in the melanin index, erythema index, skin roughness and skin elasticity, and it was verified that there is homogeneity (Table 6).

<2-2> City Foolish  apply

The toner, lotion, sun lotion and cleanser prepared in Example 2 were supplied to clinical subjects in the same manner and used twice a day in the morning and evening. However, in the morning, after applying the toner and lotion separately, make sure to apply the sun lotion with a sufficient amount.

<2-3> Confirmation of change of melanin index

Melanin is a very important and aggressive means of protecting the skin from aging and ultraviolet radiation, and is expressed in several layers of the horny layer (Quevedo et al., 1985). However, when overproduced, the accumulation of spots and freckles may be increased, promote skin aging, and cause skin cancer (Seo, Won, 2006). In particular, 40-50 menopausal women may have increased pigmentation, including senile spots, or darker complexions due to pigmentation under the eyes (Kwon, Jeong-Soon, et al., 2012; Skovgaard et al., 2006). Therefore, in the present invention, the change of the melanin index before and after the clinical test was observed, and it was confirmed whether the fermented milk cream L. rhamnosus could be a new substance which has a whitening action.

As a result, as shown in FIG. 2, the mean melanin index of the control group C tended to increase by 1.33% from 159.60 (M) before the test to 161.73 (M) after the test, and M of the non-fermentation broth was 159.44 ) And 160.39 (M), respectively, while the MC group showed a tendency to increase by 2.43% from 159.38 (M) before the test to 163.27 (M) after the test. On the other hand, the MRS group showed a tendency to decrease by 0.69% from 161.48 (M) before the test to 160.37 (M) before the test and from 3.91% (M) to 151.93 (M) The FMC group showed a significant decrease of 7.20% from 158.74 (M) before the test to 147.30 (M) after the test (FIG. 2).

In addition, as shown in FIG. 3A, visual observation was possible even before and after the test of the clinical subjects who belonged to the FMC group, and the pigmentation sites of the ball and jaw before the test were observed in the pigmentation distribution range (Fig. 3A).

<2-4> Confirmation of change of erythema index

It is a typical example of sensitive skin such as facial flushing symptom (Kim Kye-hyun, 2011), minimal erythema dose (MED) due to strong ultraviolet rays and high temperature, , And erythema (erythema), which can be attributed to various factors, are often indicators of skin type (Kwang, 2004). Therefore, the present invention evaluated whether or not the milk cream L. rhamnosus fermentation solution stabilizes the skin by observing the erythema index of the skin before and after the clinical test.

As a result, as shown in Fig. 2, the mean erythema index of the control group C tended to increase by 3.61% from 260.13 (M) before the test to 269.53 (M) after the test. M group of the non- (M) in the MC group increased from 276.63 (M) before the test to 288.41 (M) after the test and increased to 4.25% in the MC group, (1981), and melanin index and erythema index were found to be highly correlated (Kim et al., 1981). In addition, , 2009), and so on.

On the other hand, the MRS group showed a decrease of 4.51% from 274.55 (M) before the test to 262.18 (M) after the test and 3.28% from the 270.57 (M) before the test to 261.69 (M) The FMC group showed a tendency to decrease by 6.96% from 276.61 (M) before the test to 257.35 (M) after the test. The MRS group and the FM group showed a tendency to decrease by 8.12% and 6.89% 10.57%. As in the case of the change of the melanin index, it was confirmed that the contribution to the skin stability varies depending on the fermentation substrate of the L. rhamnosus fermentation broth (FIG. 2).

In addition, as shown in FIG. 3B, in the case of the clinical subjects who had skin that was sensitive to the stimuli belonging to the FMC group and had redness even after cleansing, the skin that was scarred after 7 weeks of testing was stable and the erythema almost disappeared (Fig. 3B). In addition, the degree of elasticity of the ball was increased to a certain degree.

<2-5> Confirmation of changes in skin surface roughness

The keratinization of the epidermis causes the skin to be elastic and smooth and glossy on the surface of the skin, but if the keratinization cycle is delayed or not smooth, the skin layer becomes thicker, resulting in fine lines and roughness of the skin surface (Aberer et al. , 1981). On the other hand, improvement of roughness of skin can be seen that old horny layer of stratum corneum is removed. When old horny layer of skin is peeled, it can promote the metabolism of skin and absorption of nutrients to help regenerate skin , Hwang Inchul, 2010).

On the other hand, there is a significant correlation between skin thickness and roughness as the density of dermis increases. (Hee Kyung et al., 2006), the degree of skin aging, such as wrinkle depth and skin elasticity, The skin roughness was measured before and after the test in order to examine the extent to which the test group of the present invention changed the roughness of the skin.

As a result, as shown in Fig. 2, the average facial skin roughness of the control group C was significantly increased by 16.11% from 183.78 (M) before the test to 213.38 (M) after the test (p <.05) The M group showed a tendency to increase by 6.54% from 174.48 (M) before the test to 185.89 (M) after the test, and increased by 4.30% from 174.91 (M) before the test to 182.43 (M) When the index and erythema index increased, the roughness of the skin also increased, confirming that the melanin index, erythema index and skin roughness were positively correlated.

On the other hand, the MRS group showed a decrease of 0.55% from 179.25 (M) before the test to 178.27 (M) before the test and 1.41% after the test from 183.45 (M) before the test to the 180.85 (M) , And the FMC group showed a decrease of 8.04% from 181.41 (M) before the test to 166.82 (M) after the test. Especially, the decrease was significant (p <.01) in the eyes. Therefore, the skin roughness of MRS group compared to control group was 16.66%, FM group deda showed 17.52 percent reduction in the tendency, in particular, FMC group is hence further reduced to 24.15% MRS group fermented with L. rhamnosus, FM group, FMC The group was found to have a positive effect on improving the roughness of the facial skin (Fig. 2).

In addition, as shown in FIG. 3C, in the change of the skin before and after the test of the clinical subjects belonging to the FMC group, the old horn was not dropped before the test, and the skin was rough and rough. Especially, the wrinkles and mouths of the wrists were rough and dry, After 7 weeks of testing, the severely rough skin, such as balls, wrinkles, and mouth area, was changed to a smooth, shiny skin. In addition, the erythema disappeared and the elasticity of the skin increased. It was confirmed that the jaw line became smooth (FIG. 3C).

In addition, as shown in FIG. 3D, in the change of the skin before and after the test of the clinical subjects belonging to the FMC group, the skin around the ball before the test was deeply caustic enough to catch caustic wrinkles, (Fig. 3d). In addition, as shown in FIG. 3E, the skin before the test was rough, the skin tone was not clear and the wrinkles were deeply dense. However, after 7 weeks of testing, the rough skin changed into a smooth and shiny skin, (Fig. 3 (e)).

<2-6> Skin Of skin elasticity  Confirm change

Skin elasticity refers to the degree to which skin elasticity is restored to its original state after being deformed by external forces, and is often used as a measure of skin aging, as a measure of skin aging (Seodae Heon et al., 1999 ). In addition, since the skin aging phenomenon can be improved by long-term continuous use of cosmetics containing anti-aging raw materials (Lee Ji Hyeok et al., 2001), in the present invention, , And it was confirmed whether the fermented milk of L. rhamnosus cream could be an anti - aging material.

As a result, as shown in Fig. 2, the average skin elasticity of the control group C tended to decrease by 9.52% from 0.42 (M) before the test to 0.37 (M) after the test. In the group M of the non- M) to 0.40 (M) after the test. However, MC group did not change from 0.43 (M) to 0.43 (M).

On the other hand, the elasticity of the FM group tended to decrease from 0.33 (M) before the test to 0.26 (M) before the test, while the FM group tended to decrease by 21.21% from 0.36 (M) (M) in the FMC group, and a significant increase of 28.21% in the FMC group (0.39 (M)) to 0.51 (M) after the test (FIG. 2).

In addition, as shown in FIG. 3, in the visual evaluation, it was confirmed that the subjects of the FMC group had higher skin elasticity after the test (FIG. 3), and the skin texture was rough and pore- After the 7 week test, the skin texture was smooth and smooth, and the elasticity at the pore and the corners was significantly increased (FIG. 3f).

< Experimental Example  3> Lactobacillus Lambrosse  Confirming the improvement of neck skin of fermentation broth

<3-1> Identification of neck skin status before clinical trial subjects

In order to confirm whether or not the skin barrier of the neck skin of the test subjects selected in the above <Example 3> is protected or restored, in order to confirm the homogeneity of the neck skin condition before the test, The skin moisture content, oil retention, melanin index, erythema index, TEWL, skin roughness and skin elasticity were measured before and after each test.

As a result, as shown in Table 7, there was no significant difference in the moisture content of the neck skin, the oil retention amount, the melanin index, the erythema index, the TEWL, the skin roughness and the skin elasticity, (Table 7).

<3-2> Checking moisture content

Changes in water retention before and after the clinical trial were measured according to the type of test group applied to the neck skin.

As a result, as shown in FIG. 4, the average moisture retention of the control group C was 2.61% lower than that of the test group 54.45 (M) before the test and 53.03 (M) after the test, and L. rhamnosus The MRS group showed a tendency to increase by 0.71% from 55.22 (M) before the test to 55.61 (M) before the test, and increased by 6.67% after the test from 55.60 (M) to 59.31 (M) Respectively. On the other hand, it was confirmed that the FMC group of milk cream fermentation showed a significant increase of 24.81% from 52.89 (M) before the test to 66.01 (M) after the test (FIG.

<3-3> Oil reserves  Confirm

Changes in oil retention were measured before and after the clinical trial according to the type of test group applied to the neck skin.

As a result, as shown in FIG. 4, the average amount of oil in the control group C tended to decrease by 2.20% from 41.00 (M) before the test to 40.10 (M) after the test, and the MRS group was tested at 35.16 And 29.56 (M), respectively. On the other hand, the FM group showed a significant increase of 3.68% from 34.54 (M) before the test to 35.81 (M) before the test, and 11.81% after the test from 33.88 (M) before the test to 37.88 (M) (Fig. 4).

<3-4> TEWL Confirmation of Change

TEWL changes were measured before and after the clinical test according to the type of test group applied to the neck skin.

As a result, as shown in FIG. 4, the average TEWL of the control group C increased by 1.79% from 15.62 (M) before the test to 15.90 (M) after the test, from 13.97 (M) before the MRS group test to 15.83 (M), indicating an increase of 13.31%.

On the other hand, in the FM group using the self-contained milk fat, the decrease tendency was 2.65% from 14.34 (M) before the test to 13.95 (M) after the test. Especially, in the FMC group, (M), indicating a significant decrease of 29.17% (FIG. 4).

In addition, as shown in FIG. 5C, it is possible to visually observe the changed appearance of the neck skin before and after the test of the clinical subjects belonging to the FMC group, and the skin becomes dry due to drying of the neck skin before the test, But the skin was itchy and scratched, but after 7 weeks the oil and water balance were controlled and the TEWL level was lowered, causing the rough skin to be smooth, shiny and elastic, (Fig. 5C).

<3-5> Confirmation of Change of Melanin Index

Changes in melanin index were measured before and after the clinical trial according to the type of test group applied to the neck skin.

As a result, as shown in FIG. 4, the average melanin index of the control group C tended to increase by 0.87% from 172.50 (M) before the test to 174.00 (M) after the test, whereas the MRS group of the fermentation broth showed 174.88 ), And the FM group tended to decrease by 2.22% from 179.86 (M) before the test to 175.86 (M) after the test, while the FMC group showed a tendency to decrease from 173.38 (M) before the test to 174.44 166.34 (M), showing a tendency to decrease by 4.05% (FIG. 4).

Also, as shown in FIG. 5, not only the pigmentation and erythema on the skin before the test of the clinical subjects belonging to the FMC group were significantly reduced or eliminated after the 7-week test as shown in FIG. 5, (Figs. 5A, 5B, 5C and 5D).

<3-6> Confirmation of changes in skin roughness

The roughness of the skin surface was measured before and after the clinical test according to the type of test group applied to the neck skin.

As a result, as shown in Fig. 4, the average neck skin roughness of the control group C tended to increase by 7.99% from 276.78 (M) before the test to 298.90 (M) after the test. In the MRS group, (M), and the FM group showed a tendency to decrease by 0.65% from 256.63 (M) before the test to 254.95 (M) after the test. In particular, in the FMC group, 288.87 ) To 261.19 (M) after the test (FIG. 4).

In addition, as shown in FIG. 5, it is possible to visually observe the change of the skin before and after the test of the study subjects belonging to the FMC group, so that the skin which was rough and had rough skin after the test was not only smooth and soft after the test, (Figs. 5B, 5C and 5D).

<3-7> Skin Elasticity  Confirm change

Skin elasticity changes were measured before and after the clinical trial according to the type of test group applied to the neck skin.

As a result, as shown in FIG. 4, the average skin elasticity of the control group, C, showed a tendency to decrease by about 1.51% from 0.66 (M) before the test to 0.64 (M) after the test, and the MRS group ) Showed a tendency to decrease by about 6.90% from 0.53 (M) after the test to 0.70 (M) after the test at 0.66 (M) before the test. In particular, the FM group showed a tendency to increase by about 4.55% M) to about 0.75 (M) after the test (FIG. 4).

In addition, as shown in FIG. 5, the skin elasticity was visually observed before and after the test of all the clinical subjects belonging to the FMC group. In particular, in FIG. 5E, the skin elasticity was improved, (Fig. 5E).

< Experimental Example  4> Various Lactobacillus Lambrosse  Strain Milk cream  Check the effect of fermentation broth

<4-1> Test group  apply

In the same manner as in EXPERIMENTAL EXAMPLES 1 to 4 using the milk cream fermentation broth using the various Lactobacillus lambosus strains prepared in Example 1 and Example 2, .

<4-2> Confirmation of skin moisture content

After applying the toner and lotion containing the milk cream fermentation broth using the various Lactobacillus lambosus strains prepared in Example 2 to the clinical subjects, changes in skin moisture content were measured.

As a result, KCTC 5033 (B2) showed a significant increase of about 17%, KCTC 3237 (D1) showed about 28% increase, and KCTC 5046 (D2) KCCM 32823 (D5) tended to increase by about 11%, KCCM 32826 (D6) tended to increase by about 20%, while KCCM 32826 (D6) ATCC 14957 (D9) tended to increase by about 10%, ATCC 21052 (D10) tended to increase by about 13%, KCCM 40069 (D7) tended to increase by about 5% (D11) showed a tendency to increase by about 13%, while RA-32 (D12) showed a tendency to increase by about 9%, and the cosmetic containing a milk cream fermented liquid fermented with Lactobacillus lambosus strains exhibited a skin moisture content (Table 8).

As shown in Table 9, KCTC 5033 (B2) showed a significant increase in KCTC 5033 (B2), KCTC 3237 (D1) showed an increase of about 32%, KCTC 5046 (D2) KCCM 32823 (D5) increased by about 22%, KCCM 32826 (D6) increased by about 19%, while KCCM 32203 (D5) increased by about 22% ATCC 14957 (D9) tended to increase by about 17%, ATCC 21052 (D10) tended to increase by about 33%, and ATCC 9595 (D8) KCTC 10965BP (D11) showed a tendency to increase by about 20% and RA-32 (D12) showed a tendency to increase by about 15%, indicating that cosmetics containing a milk cream fermentation broth fermented with Lactobacillus lambosus strain increased neck moisture retention (Table 9).

<4-3> Skin Oil reserves  Confirm

After applying the toner and lotion containing the milk cream fermentation broth using various Lactobacillus lambosus strains prepared in Example 2 to the clinical subjects, changes in the skin oil retention amount were measured.

As a result, as shown in Table 10, KCTC 5033 (B2) showed a significant increase by about 15%, KCTC 3237 (D1) increased by about 21%, and KCTC 5046 (D2) KCCM 32823 (D5) tends to increase by about 6%, KCCM 32826 (D6) tends to increase by about 5%. ATCC 14957 (D9) tended to increase by about 29%, ATCC 21052 (D10) tended to increase by about 22%, while ATCC 14957 (D9) KCTC 10965BP (D11) showed a tendency to increase by about 12% and RA-32 (D12) showed an increase of about 11%, indicating that cosmetic products containing a milk cream fermented product fermented with Lactobacillus lambosus strain increased facial skin oil retention (Table 10).

As shown in Table 11, KCTC 5033 (B2) showed a significant increase of about 12%, KCTC 3237 (D1) showed about 13% increase, and KCTC 5046 (D2) KCCM 32823 (D5) tends to increase by about 8%, while KCCM 32826 (D6) tends to increase by about 14%. , ATCC 14957 (D9) tended to increase by about 7%, ATCC 21052 (D10) tended to increase by about 9%, KCCM 40069 (D7) tended to increase by about 5%, ATCC 9595 10965BP (D11) showed a tendency to increase by about 8%, and RA-32 (D12) showed an increase of about 8%, indicating that the cosmetic containing a milk cream fermentation broth fermented with Lactobacillus lambosus strain (Table 11).

<4-4> TEWL  Confirm

The toner and lotion containing the milk cream fermentation broth prepared using the various Lactobacillus lambosus strains prepared in Example 2 were applied to the clinical subjects, and the changes of TEWL were measured.

As a result, as shown in Table 12 below, KCTC 5033 (B2) showed a significant decrease by about 23% in facial skin, KCTC 3237 (D1) decreased by about 10%, KCTC 5046 (D2) KCCM 32823 (D5) tends to decrease by about 20%, KCCM 32826 (D6) tends to decrease by about 15%, KCCM 32223 (D6) ATCC 14957 (D9) tended to decrease by about 22% while ATCC 21052 (D10) tended to decrease by about 21%. , KCTC 10965BP (D11) showed a tendency to decrease by about 15%, RA-32 (D12) showed a tendency to decrease by about 25%, and cosmetics containing a milk cream fermentation broth fermented with Lactobacillus lambosus strain reduced facial skin TEWL (Table 12).

As shown in Table 13, KCTC 5033 (B2) showed a significant decrease by about 29%, KCTC 3237 (D1) decreased by about 12%, KCTC 5046 (D2) KCCM 32823 (D5) tends to decrease by about 19% while KCCM 32826 (D6) tends to decrease by about 21%. ATCC 14957 (D9) tended to decrease by about 23%, ATCC 21052 (D10) tended to decrease by about 19%, and KCCM 40069 (D7) tended to decrease by about 17% D11) showed a tendency to decrease by about 19%, and RA-32 (D12) showed a tendency to decrease by about 19%, confirming that cosmetic products containing a milk cream fermentation broth fermented with Lactobacillus lambosus strain decreased neck skin TEWL Table 13).

<4-5> Confirm skin melanin index

After applying the toner and lotion containing the milk cream fermentation broth using various Lactobacillus lambosus strains prepared in Example 2 to the clinical subjects, the change of the skin melanin index was measured.

As shown in Table 14, KCTC 5033 (B2) showed a significant decrease by about 7%, KCTC 3237 (D1) decreased by about 5%, and KCTC 5046 (D2) %, Respectively. However, KCTC 5510 (D3) and KCCM 11320 (D4) showed about 3% increase respectively. However, KCCM 32823 (D5) tended to decrease by about 4%, KCCM 32826 (D6) tended to decrease by about 7%, KCCM 40069 (D7), ATCC 9595 (D8), ATCC 14957 (D11) and RA-32 (D12) showed a tendency to decrease by about 5%, respectively. The cosmetics containing the milk cream fermented by Lactobacillus lambosus strains decreased the skin melanin index (Table 14).

As shown in Table 15 below, KCTC 5033 (B2) group showed a decrease of about 4%, KCTC 3237 (D1) showed a decrease of about 3% and KCTC 5046 (D2) The trend of KCCM 11320 (D4) tended to decrease by about 4%, while that of KCCM 40082 (D7) tended to decrease by about 4%, while that of KCCM 32826 (D6) Respectively, while ATCC 14957 (D9) showed a slight increase tendency. In addition, KCTC 10965BP (D11) and RA-32 (D12) showed a decreasing tendency by about 4%, indicating that cosmetics containing a milk cream fermentation broth fermented with Lactobacillus lambosus strain reduced neck skin melanin index (Table 15).

<4-6> Confirm skin roughness

The toner and lotion containing the milk cream fermentation broth using the various Lactobacillus lambosus strains prepared in Example 2 were applied to the clinical subjects, and then the changes in skin roughness were measured.

As shown in Table 16, KCTC 5033 (B2) tended to decrease by 8.04%, whereas KCTC 3237 (D1) tended to increase by about 7% while KCTC 5046 (D2) tended to increase slightly , And ATCC 21052 (D10) showed about 7% increase respectively. KCCM 32823 (D5) tends to decrease by about 14%, KCCM 32826 (D6) tends to decrease by about 10%, while KCCM 32823 (D5) tends to decrease by about 14% ATCC 14957 (D9) tends to decrease by about 2%, KCTC 10965BP (D11) tends to decrease by about 3%, RA-32 (D7) tends to decrease by about 3%, ATCC 9595 (D12) showed a tendency to decrease by about 5%, and it was confirmed that the cosmetic containing the milk cream fermentation broth fermented with Lactobacillus lambosus strain substantially reduced the roughness of the facial skin (Table 16).

KCTC 5033 (B2) showed a significant decrease by about 10%, KCTC 3237 (D1) decreased by about 10% and KCTC 5046 (D2) was about 9% as shown in Table 17 below. KCCM 32823 (D5) tends to decrease by about 2% while KCCM 32826 (D6) tends to decrease by about 11%. , ATCC 14957 (D9) tended to decrease by about 8%, ATCC 21052 (D10) tended to decrease by about 10%, KCTC 10965BP (D11) showed a tendency to decrease by about 5%, while RA-32 (D12) showed a tendency to decrease by about 6%, indicating that cosmetic products containing a milk cream fermentation broth fermented with Lactobacillus lambosus strain reduced neck skin roughness (Table 17).

<4-7> Confirm skin elasticity

After applying the toner and lotion containing the milk cream fermentation broth using various Lactobacillus Lymphosus strains prepared in Example 2 to the clinical subjects, the changes in skin elasticity were measured.

As a result, as shown in Table 18 below, the KCTC 5033 (B2) and KCTC 3237 (D1) were significantly increased by about 28% and 42%, respectively, while the ATCC 21052 (D10) (D2) is about 26%, KCTC 5510 (D3) is about 6%, KCCM 11320 (D4) is about 4% and KCCM 32823 (D5) is about 6% ATCC 14957 (D9) showed about 39% increase, while KCCM 40069 (D7) showed about 8% increase, ATCC 9595 (D8) showed about 39% (D12) showed a tendency to increase by about 16%, while RA-32 (D12) showed an increase of about 18%. KCTC 10965BP (D11) (Table 18).

As shown in Table 19, KCTC 5033 (B2) showed a significant increase of about 12%, KCTC 3237 (D1) showed about 5% increase, and KCTC 5046 (D2) KCCM 32823 (D5) tends to increase by about 6%, while KCCM 32826 (D6) tends to increase by about 8%. , ATCC 14957 (D9) tended to increase by about 8%, ATCC 21052 (D10) tended to increase by about 3%, KCCM 40069 (D7) tended to increase by about 14%, ATCC 9595 10965BP (D11) showed a tendency to increase by about 9%, and RA-32 (D12) showed a tendency to increase by about 14%, indicating that cosmetics containing a milk cream fermented product fermented with Lactobacillus lambosus strain increased the elasticity of the neck skin (Table 19).

Claims (14)

Lactobacillus rhamnosus Lactobacillus rhamnosus A cosmetic composition for skin improvement comprising a milk fermentation broth as an active ingredient.
The composition of claim 1, wherein the Lactobacillus lambusaceus is selected from the group consisting of KCTC 5033, KCTC 3237, KCTC 5046, KCTC 5510, KCCM 11320, KCCM 32823, KCCM 32826, KCCM 40069, ATCC 9595, ATCC 14957, ATCC 21052 and KCTC 10965BP Wherein the composition is Lactobacillus lambusosus deposited with a deposit number selected from the group consisting of Lactobacillus laminosus and Lactobacillus laminosus.
delete [Claim 3] The cosmetic composition for skin improvement according to claim 1, wherein the oil cream is a milk cream containing at least 3 parts by weight of a milk fat separated from raw milk or milk.
The cosmetic composition for improving skin according to claim 1, wherein the skin is a skin having a damaged skin barrier or aging skin.
[Claim 7] The cosmetic composition for improving skin according to claim 5, wherein the skin is a face or neck skin.
6. The method of claim 5, wherein the skin damaged by the skin barrier is skin having at least one selected from the group consisting of dry skin, skin irritation, skin pruritus, excessive tingling of skin and skin burning, Wherein the skin has at least one skin selected from the group consisting of skin irritation, irritation, erythema, erythema, skin roughness, skin sagging, elasticity degradation and skin wrinkles. The cosmetic composition of claim 1, wherein the cosmetic composition is a solution, suspension, emulsion, paste, gel, cream, lotion, powder, soap, surfactant-containing cleansing, oil, powder foundation, emulsion foundation, wax foundation, And a mixture of at least one compound selected from the group consisting of:
A skin external preparation for improving a disease mediated by at least one skin barrier damage selected from the group consisting of dry skin of the skin, skin irritation and skin pruritus containing the fermented liquid of Lactobacillus lansosus milk cream as an active ingredient.










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