KR20160021802A - Anti-inflammatory Composition - Google Patents

Abstract

The present invention relates to an anti-inflammatory composition and, specifically, to an anti-inflammatory composition using an Isodon inflexus (Thunb.) Kudo extract, a Boehmeria pannosa Nakai & Satake extract, and a Gnaphalium affine D. Don extract, a Mosla punctulata (GMEL.) NAKAI extract, a Prunella vulgaris var. lilacina Nakai extract, or a Rubus trifidus Thunb. extract. The extracts have the inhibitory activities of NO generation, the inhibitory activities of PGE_2 generation, and the inhibitory activities of inflammatory cytokines (TNF-α, IL-1β, and IL-6) generation.

Description

[0001] Anti-inflammatory Composition [

The present invention relates to an antiinflammatory composition, and more particularly to a composition comprising an extract of Isodon inflexus , Boehmeria pannosa) extract, everlasting (Gnaphalium affine ) Extract, Perilla grass ( Mosla punctulata extract, Lamiaceae ( Prunella vulgaris ) extract or island strawberry ( Rubus trifidus extract of the present invention.

Inflammation is the defensive response of a living body to external infectious agents such as external physical and chemical stimuli, bacteria, fungi, viruses and allergens.

The inflammatory response is part of the innate immune response, and as in other animals, the innate immune response of humans begins by recognizing and attacking macrophages as non-self through a pattern of cell surfaces that are specific to the pathogen. During the inflammation reaction, plasma accumulates on the inflamed area, diluting the toxicities secreted by the bacteria, increasing the blood flow, and accompanied by symptoms such as erythema, pain, edema, and fever.

These inflammatory reactions involve a variety of biochemical events, in particular, cyclooxygenase (COX), which is associated with the nitric oxide synthase (NOS) and the biosynthesis of various prostaglandins, .

There are three isomers of NOS: endotoxin of bacteria such as calcium or camodanol-dependent eNOS (endothelial NOS), nNOS (neurotic NOS), and lipopolysaccharide (IL-1β, TNF-α, IL There are iNOS (inducible NOS) induced by various inflammatory cytokines such as IL-6, IL-8 and IL-12 and produce NO from L-arginine.

NO produced by eNOS or nNOS plays an important role in maintenance of homeostasis by performing various physiological responses related to blood pressure control, neurotransmission, learning, memory, etc. However, NO produced by iNOS is associated with arthritis, sepsis, (Moncade S. et al, Pharmacol. Rev., 1991, 43, 109, Nature Medicine, 2001, 7, 1138; Mu, S., et al., Immunoprecipitation, , MM, J. Endotoxic Res. 7, p341, 2001).

The COX enzyme synthesizes PGG ₂ and PGH ₂ from arachidonic acid with hydroperoxidase (HOX) activity together with the function of COX. These compounds include PGE ₂ , PGF ₂ , PGD ₂ , prostacyclin and create a duplex thromboxane _{a 2 (thromboxane A2, TxA2)} . Among the functions of COX, the function of PGH synthase is involved in the pain and inflammation reaction through synthesis of PGE ₂ .

There are two subtypes of COX and COX-1 is always expressed in most tissues, whereas COX-2 is rapidly induced by inflammatory cytokines and plays an important role in the inflammatory response.

Therefore, NO, PGE ₂ , Inhibitors such as inflammatory cytokines, iNOS inhibitors and COX-2 inhibitors may be used as therapeutic agents for inflammatory diseases.

The present invention relates to a method for producing NO, PGE ₂ , And acid mint extract having an activity of inhibiting the production of inflammatory cytokines and the like.

It is an object of the present invention to disclose an anti-inflammatory composition using an acid pepper extract or the like.

Other and further objects of the present invention will be described below.

The present invention is based on the finding that inhibition of NO production, inhibition of the production of PGE ₂ , and inhibition of inflammatory cytokines (TNF-α, IL-1β, and IL-1β) were observed in the extracts of mushroom extract, royal waxy extract, -6) production inhibitory activity. As described above, a substance having an NO production inhibitory activity, a PGE ₂ production inhibitory activity, and / or an inflammatory cytokine (TNF-α, IL-1β and IL-6) production inhibitory activity can be used as an anti-inflammatory agent.

The anti-inflammatory composition of the present invention is provided on the basis of the results of these experiments. The anti-inflammatory composition of the present invention can be used as an effective ingredient for extracting acid mint extract, royal waxy extract, rice crumb extract, perilla grass extract, .

As used herein, the term "extract" refers to an extract of a plant, a plant, a stem, a root, a petal or a mixture thereof from a plant such as an alcohol having 1 to 4 carbon atoms such as methanol or ethanol, acetone, ethyl acetate, saturated normal butanol, chloroform, , Water, or a mixed solvent thereof, and fractions further purified with the above-listed solvents in the extracts. Here, the extraction method includes both a method of immersing the object to be extracted in an extraction solvent and a method of distilling the object to be extracted into an extraction solvent. In addition, any method such as cold-pressing, heating, ultrasonic wave, and reflux may be applied to the extraction method through immersion. However, the above-mentioned "extract" preferably means that the object to be extracted is extracted (immersed or distilled) with water, ethanol or a mixed solvent thereof, more preferably an ethanol aqueous solution having an ethanol content of 70% to 90% it means. Where% is the concentration (v / v) by volume percentage and refers to a volume of solute dissolved in a volume of solution as is known in the art. For example, 30% (v / v) means that 30 ml of the solute is dissolved in 100 ml of the solution. The term "extract" in the present specification includes a purified form of the extract through filtration, a liquid concentrated extract from which the extraction solvent has been removed, and a solid extract from which the extraction solvent has been removed.

In the present specification, the above-mentioned "active ingredient" means an ingredient that exhibits the desired activity alone or can exhibit activity together with a carrier that is itself inactive.

In the present specification, "anti-inflammatory" means an improving activity of an inflammatory disease as defined below.

In the present specification, the term "inflammatory disease" as used herein refers to any state including inflammatory reaction as a local or systemic bio-defense reaction against external physical or chemical stimuli or infections of external infectious agents such as bacteria, fungi, viruses, Can be defined. This reaction is enzyme secretion (e.g., iNOS, COX-2, etc.) activation, release of inflammatory mediators (e. G., NO, TNF-α, IL -6, IL-1β, PGE 2 related to various inflammatory mediators and the immune cells ), Bodily fluid infiltration, cell migration, and tissue destruction, and manifest externally by symptoms such as erythema, pain, edema, fever, deterioration or loss of specific function of the body. The inflammatory disease may be acute, chronic, ulcerative, allergic or necrotic, so long as it is included in the definition of inflammatory diseases as above, it may be acute, chronic, ulcerative, allergic, Whether it is necrotic or not. Specifically, the inflammatory diseases include asthma, allergic and non-allergic rhinitis, chronic and acute rhinitis, chronic and acute gastritis or enteritis, ulcerative gastritis, acute and chronic nephritis, acute and chronic hepatitis, chronic obstructive pulmonary disease, Inflammatory bowel syndrome, inflammatory pain, migraine headache, headache, back pain, fibromyalgia, fascia disease, viral infection (e.g., C type infection), bacterial infection, fungal infection, burn, wound due to surgical or dental surgery, These may include Prostaglandin E Overdose Syndrome, atherosclerosis, gout, arthritis, rheumatoid arthritis, ankylosing spondylitis, Hodgkin's disease, pancreatitis, conjunctivitis, iritis, scleritis, uveitis, dermatitis, eczema and multiple sclerosis.

The antiinflammatory composition of the present invention may contain any amount (effective amount) as long as it exhibits antiinflammatory activity depending on the purpose of formulation, compounding, etc., To 99.999% by weight based on the total weight of the composition. Herein, "effective amount" refers to the amount of active ingredient capable of exhibiting anti-inflammatory activity. Such effective amounts can be determined experimentally within the ordinary skill of those skilled in the art.

The composition of the present invention can be used as a pharmaceutical composition in a specific embodiment.

The pharmaceutical composition of the present invention can be formulated for oral administration or parenteral administration by mixing the active ingredient with pharmaceutically acceptable carriers, excipients, additives, and the like.

Examples of pharmaceutically acceptable carriers or excipients include lactose, magnesium stearate, starch, talc, gelatin, agar, pectin, gum arabic, olive oil, sesame oil, cacao butter, ethylene glycol and others commonly used.

Examples of the solid composition for oral administration include tablets, pills, capsules, powders, granules and the like. In such a solid composition, the plant extract as an active ingredient is mixed with at least one inert diluent such as lactose, mannitol, glucose, hydroxypropylcellulose, microcrystalline cellulose, starch, polyvinylpyrrolidone, magnesium aluminometasilicate, Mixed. The solid composition may contain additives other than an inert diluent, for example, a lubricant such as magnesium stearate, a disintegrant such as calcium cellulose glycolate, a solubilizing agent such as glutamic acid or aspartic acid, according to a conventional method. The tablets or pills may be coated with a film made of a material such as sucrose, gelatin, hydroxypropylmethylcellulose phthalate or the like, if necessary, and may be coated with two or more layers as the case requires.

The liquid composition for oral administration may contain a generally used inert diluent such as purified water, ethanol, etc., including pharmaceutically acceptable emulsions, solutions, suspensions, syrups, elixirs and the like. The composition may contain, in addition to an inert diluent, a wetting agent, an adjuvant such as a suspending agent, a sweetening agent, a flavoring agent, a fragrance, an antiseptic, and the like.

Injections for parenteral administration include sterile aqueous or non-aqueous solutions, suspensions, and emulsifiers. Examples of aqueous solutions and suspensions include water for injection and physiological saline for injection. Examples of the non-aqueous solution / suspension include propylene glycol, polyethylene glycol, vegetable oils such as olive oil, alcohols such as ethanol, polysorbate 80® and the like. Such a composition may again contain adjuvants such as preservatives, wetting agents, emulsifying agents, dispersing agents, stabilizing agents (for example, lactose), and solubilizing agents (for example, glutamic acid, aspartic acid). These can be sterilized by a conventional sterilization method such as filtration sterilization with a microfiltration membrane, heat sterilization such as high pressure steam sterilization, or sterilizing agent combination. Injections can be solution formulations or freeze-dried preparations which can be used by dissolving in use. Examples of excipients for freeze-drying include sugar alcohols and sugars such as mannitol, glucose and the like.

The pharmaceutical composition of the present invention may be administered orally or parenterally.

Preferable examples include parenteral administration methods such as administration by injection (subcutaneous injection, intravenous injection, intramuscular injection, intraperitoneal injection, etc.), transdermal administration, transmucosal administration (transrectal administration, etc.) to be. Of course, oral administration methods may also be used.

The dosage of the active ingredient of the pharmaceutical composition of the present invention may be determined according to the severity of the disease and the age of the patient, but is generally in the range of 0.005 / / kg to 100 mg / kg, preferably 0.02 / / 5 mg / kg. However, since the dosage of the pharmaceutical composition of the present invention is determined in view of various related factors such as route of administration, age, sex, weight, and patient's severity of the patient, the dose is limited in any aspect to the scope of the present invention It should not be understood.

In another specific embodiment, the composition of the present invention can be identified as a food composition.

The food composition of the present invention may contain sweetening agents, flavoring agents, physiologically active ingredients, minerals and the like in addition to the active ingredients thereof.

Sweetening agents may be used in an amount that sweetens the food in a suitable manner, and may be natural or synthetic. Preferably, natural sweeteners are used. Examples of natural sweeteners include sugar sweeteners such as corn syrup solids, honey, sucrose, fructose, lactose and maltose.

Flavors may be used to enhance taste or flavor, both natural and synthetic. Preferably, a natural one is used. When using natural ones, the purpose of nutritional fortification can be performed in addition to the flavor. Examples of natural flavoring agents include those obtained from apples, lemons, citrus fruits, grapes, strawberries, peaches, and the like, or those obtained from green tea leaves, Asiatica, Daegu, Cinnamon, Chrysanthemum leaves and Jasmine. Also, those obtained from ginseng (red ginseng), bamboo shoots, aloe vera, banks and the like can be used. The natural flavoring agent may be a liquid concentrate or a solid form of extract. Synthetic flavoring agents may be used depending on the case. Synthetic flavoring agents such as esters, alcohols, aldehydes and terpenes may be used.

Examples of the physiologically active substance include catechins such as catechin, epicatechin, gallocatechin and epigallocatechin, and vitamins such as retinol, ascorbic acid, tocopherol, calciferol, thiamine and riboflavin.

As the mineral, calcium, magnesium, chromium, cobalt, copper, fluoride, germanium, iodine, iron, lithium, magnesium, manganese, molybdenum, phosphorus, potassium, selenium, silicon, sodium, sulfur, vanadium and zinc can be used.

In addition, the food composition of the present invention may contain preservatives, emulsifiers, acidifiers, thickeners and the like as needed in addition to the above sweeteners.

Such preservatives, emulsifiers and the like are preferably added in a very small amount as long as they can attain an application to which they are added. By "trace amount" is meant numerically the range of from 0.0005% to about 0.5% by weight based on the total weight of the food composition.

Examples of the preservative which can be used include calcium sodium sorbate, sodium sorbate, potassium sorbate, calcium benzoate, sodium benzoate, potassium benzoate and EDTA (ethylenediaminetetraacetic acid).

Examples of the emulsifier which can be used include acacia gum, carboxymethyl cellulose, xanthan gum, pectin and the like.

Examples of the acidulant that can be used include acid, malic acid, fumaric acid, adipic acid, phosphoric acid, gluconic acid, tartaric acid, ascorbic acid, acetic acid, and phosphoric acid. Such an acidulant may be added so that the food composition has a proper acidity for the purpose of inhibiting the growth of microorganisms other than the purpose of enhancing the taste.

Agents that may be used include suspending agents, sedimentation agents, gel formers, bulking agents and the like.

Further, the herbal composition of the present invention may be added to improve the flavor or palatability and to have other functionalities (for example, arthritis or osteoporosis prevention). Examples of herbal medicines that can be added include mulberry extract, There may be exemplified extracts such as extracts of Pseudomonas spp., Pseudomonas sp. Extract, Mushroom extract, Sambrook extract, Bulb extract, Corn oil extract, Gugija extract, Licorice extract, Angelica keiskei extract, .

The composition of the present invention can be identified as a cosmetic composition in another specific embodiment.

When the composition of the present invention is identified as a cosmetic composition, the cosmetic composition may be prepared in various forms, for example, emulsion, lotion, cream (oil-in-water type, water-in-water type, multiphase), solution, suspension (Water and water), anhydrous products (oil and glycol), gel, mask, pack, powder and the like.

The composition of the present invention may contain an acceptable carrier in cosmetic formulations other than those containing the active ingredient.

As used herein, the term " acceptable carrier for a cosmetic preparation "refers to a compound or composition that is already known and used in the cosmetic preparation, or a compound or composition to be developed in the future, and has no toxicity that the human body can adapt to when contacted with skin.

The carrier may be included in the composition of the present invention in an amount of from about 1% by weight to about 99.99% by weight, preferably from about 50% by weight to about 99% by weight of the composition, based on the total weight thereof.

However, since the ratio depends on the above-mentioned formulation of the cosmetic composition and its specific application site (face or hands) or its preferable application amount, the ratio is limited in any aspect to the scope of the present invention It should not be.

Examples of the carrier include alcohols, oils, surfactants, fatty acids, silicone oils, humectants, moisturizers, viscosifiers, emulsifiers, stabilizers, sunscreens, coloring agents and perfumes.

The compounds / compositions which can be used as the carrier and which can be used as alcohols, oils, surfactants, fatty acids, silicone oils, wetting agents, moisturizers, viscosifiers, emulsions, stabilizers, sunscreens, A person skilled in the art can select and use appropriate substances / compositions.

The cosmetic composition of the present invention may further comprise a functional substance such as a skin moisturizing active substance, an anti-atopic active substance, an anti-acne active substance, a whitening active substance, etc., which are known in the art.

The composition of the present invention can be identified as a soap composition in another specific embodiment.

When the composition of the present invention is identified as a soap composition, the soap composition of the present invention can be prepared by incorporating the active ingredient into a soap base.

Examples of the soap base material include vegetable oils such as palm oil, palm oil, soybean oil, perm free oil, olive oil and palm kernel oil or animal fats such as tallow, lard, sunshine and fish oil. Examples of the skin moisturizers include glycerin, erythritol, polyethylene glycol , Propylene glycol, butylene glycol, pentylene glycol, hexyl glycol, isopropyl myristate, silicone derivatives, aloe vera, sorbitol and the like. Examples of the emulsifier include natural oils, wax fatty alcohols, hydrocarbons, May be used. As the water softening agent, tetrasodium ethylenediate and the like may be used.

The soap composition of the present invention may further contain, as an additive, an antibacterial agent, a dispersant, a foam inhibitor, a solvent, a scouring inhibitor, a corrosion inhibitor, a fragrance, a dye, a sequestering agent, an antioxidant and an antiseptic.

In the soap composition of the present invention, the soap base or additive may be included in a content commonly used in the art, wherein the soap base generally comprises from 99.999% to 50% by weight, based on the total weight of the soap composition And the additive may be added in an amount of 1 wt% to 20 wt%.

As described above, according to the present invention, there is provided an anti-inflammatory composition using an acid mint extract or the like.

The composition of the present invention can be commercialized as a cosmetic, a soap or a medicine.

Hereinafter, the present invention will be described with reference to Examples, Production Examples and Experimental Examples. However, the scope of the present invention is not limited to these examples, preparation examples and experimental examples.

< Example > Manufacture of extracts of royal waxy

&Lt; Example 1 & gt ; Preparation of Wang Moxiblo extract

Seventy percent by weight of 70% ethanol was added to the three outposts of Wang Mousypollus, and the extract was extracted for 24 hours and then filtered with Watman paper filter paper (Whatman No. 2). Then, the filtrate was concentrated under reduced pressure to remove the solvent to obtain a solid form of the extract.

Example 2: Preparation of perilla grass extract

The same method as above was used to extract the perilla seedlings.

Example 3 Preparation of Lamiaceae Extract

Extraction was carried out in the same manner as above, except that a mulberry outpost was used as an extraction target.

Example 4: Preparation of acid mint extract

Extraction was carried out in the same manner as above, except that the extract was used as the extraction target.

Example 5: Preparation of an island strawberry extract

Extraction was carried out in the same manner as above, except that strawberry leaves were used.

Example 6 Preparation of Rice Mugwort Extract

Extraction was carried out in the same manner as described above, except that the extract was used for the extraction.

< Experimental Example > Evaluation test of anti-inflammatory activity

&Lt; Experimental Example 1 > Cells and reagents

Mouse macrophage RAW264.7 cells were cultured in DMEM (Dulbecco's modified Eagle's medium) medium containing 100 units / ml penicillin, 100 μg / ml streptomycin and 10% fetal bovine serum (FBS) And cultured at 37 ° C, 5% CO ₂ and 95% humidity while maintaining subconfluence.

DMEM medium and FBS were purchased from Invitrogen-Gibco (Grand Island, NY), and ELISA kit for quantification of TNF-α IL-1β, IL-6 and PGE ₂ was purchased from R & D systems, Were purchased from BD biosciences (San Diego, Calif.).

<Experimental Example 2> Inhibitory activity evaluation NO

RAW 264.7 cells were pre-cultured at 1.5 × 10 ⁵ cells / ml and treated with test substance (100 μg / ml) and LPS (1 μg / ml) for 24 hours. The amount of NO produced was measured in the form of NO ₂ ^- present in cell culture medium using Griess reagent. Specifically, 100 μl of the cell culture supernatant was mixed with 100 μl of Griess reagent [1% (w / v) sulfanilamide, 0.1% (w / v) naphylethylenediamine in 2.5% (v / v) phosphoric acid] After the reaction, the absorbance was measured at 540 nm, which was measured in the form of NO ₂ ^- present in the cell culture. The amount of NO produced was compared with sodium nitrite (NaNO ₂ ) as standard. The results are shown in the following Table 1 as a percentage of the control group (LPS alone treatment group).

NO production inhibitory activity division NO production inhibitory activity (%) Control group (LPS alone treatment group) 100 The extract of Example 1 27.16 + - 3.21 ** The extract of Example 2 32.55 + - 5.33 ** The extract of Example 3 40.20 ± 2.50 ** The extract of Example 4 15.47 ± 4.22 ** The extract of Example 5 45.59 ± 1.43 ** The extract of Example 6 27.16 + - 2.62 **

The results of the above Table 1 show that the inhibitory activity of NO production is higher in the order of acid mint extract, royal waxy extract, waxy wort extract, perilla grass extract, lupine extract and strawberry extract (* P <0.05 ; ** P <0.01 ).

<Experimental Example 3> Inhibitory activity of inflammatory cytokine and PGE ₂

RAW 264.7 cells (1.0 × 10 ⁶ cells / ml) were cultured for 18 hours and cultured for 24 hours in the same manner as the test substances (treated at the same concentration as in <Experiment 2>) and LPS (1 μg / ml) . After 24 hours, the culture medium was centrifuged and PGE ₂ , TNF-α, IL-1β and IL-6 of the supernatant were quantitated using an ELISA kit. The results are shown in [Table 2] to [Table 5] below as a percentage of the control group (LPS alone treatment group).

PGE ₂ production inhibitory activity division PGE ₂ production inhibitory activity (%) Control group (LPS alone treatment group) 100 The extract of Example 1 58.42 + - 6.29 ** The extract of Example 2 67.27 ± 5.93 ** The extract of Example 3 62.43 + - 4.38 ** The extract of Example 4 57.27 ± 5.92 ** The extract of Example 5 63.68 + - 3.64 ** The extract of Example 6 61.35 ± 6.82 **

TNF-α production inhibitory activity division TNF-α production inhibitory activity (%) Control group (LPS alone treatment group) 100 The extract of Example 1 48.25 + - 5.27 ** The extract of Example 2 64.94 + - 7.38 ** The extract of Example 3 58.16 + - 4.82 ** The extract of Example 4 61.28 + - 4.51 ** The extract of Example 5 65.84 ± 7.63 ** The extract of Example 6 67.37 + - 5.28 **

IL-1? Production inhibitory activity division IL-1? Production inhibitory activity (%) Control group (LPS alone treatment group) 100 The extract of Example 1 43.84 + - 5.38 ** The extract of Example 2 56.92 + 4.56 ** The extract of Example 3 52.36 + - 6.94 ** The extract of Example 4 64.84 + - 5.83 ** The extract of Example 5 68.38 + - 6.48 ** The extract of Example 6 61.63 + - 4.95 **

IL-6 production inhibitory activity division IL-6 production inhibitory activity (%) Control group (LPS alone treatment group) 100 The extract of Example 1 56.62 + - 6.94 ** The extract of Example 2 62.34 + - 7.26 ** The extract of Example 3 58.73 ± 5.84 ** The extract of Example 4 66.48 ± 6.26 ** The extract of Example 5 62.28 + - 6.92 ** The extract of Example 6 56.25 + - 5.60 **

All of the plant extracts of the above Examples significantly inhibited PGE ₂ , TNF-α, IL-1β and IL-6 by referring to the results of the above Tables 2 to 5 (* P <0.05; ** P &lt; 0.01 ).

<Experimental Example 4> Cytotoxicity test

RAW 264.7 cells (1.5 × 10 ⁵ cells / ml) were pre-cultured for 18 hours and co-treated with the test substance (treated at the same concentration as in <Experiment 2> above) and LPS (1 μg / Time. LDH (lactate dehydrogenase) released from RAW 264.7 cells was measured to evaluate cytotoxicity. The efflux of LDH is used as an indicator of cytotoxicity. LDH activity can be determined by quantitating NADH produced in the process of producing acetic acid in lactic acid. LDH activity was quantitated using the LDH cytotoxicity detection kit (Promega, Madison, WI, USA) and the cytotoxicity was shown in the following Table 6 as a percentage of the control (untreated group).

Cell viability (%) division Cell viability (%) Control group (LPS alone treatment group) 100 The extract of Example 1 100.78 The extract of Example 2 101.99 The extract of Example 3 100.01 The extract of Example 4 100.80 The extract of Example 5 100.80 The extract of Example 6 100.40

The results of the above Table 6 show that all of the plant extracts of the above examples do not show any cytotoxicity, and the NO production inhibitory activity of the above <Experimental Example 2> and the PGE ₂ and inflammatory cytokines of the <Experimental Example 3> Indicating that the activity of inhibiting the formation of cytokines is not a result of cytotoxicity.

Statistical processing

Statistical significance was evaluated by one-way ANOVA test and student's t-test. Data from three or more independent experiments were expressed as mean ± standard deviation (SD).

Claims (6)

Which comprises as an active ingredient an acid mint extract, a royal waxy extract, a perilla grass extract, a Lamiaceae extract or an island strawberry extract.
The method according to claim 1,
Wherein the extract is obtained by extracting an object to be extracted with water, ethanol or a mixed solvent thereof.
The method according to claim 1,
Wherein the composition is a pharmaceutical composition.
The method according to claim 1,
Wherein the composition is a food composition.
The method according to claim 1,
Wherein the composition is a cosmetic composition.
The method according to claim 1,
Wherein the composition is a soap composition.