JP2004075692A - Composition and drink containing the same - Google Patents

Abstract

<P>PROBLEM TO BE SOLVED: To provide a composition preventing rot and oxidation of a composition containing β-1, 3-1, 6-glucan in preserving, improving antioxidative property, antiallergic property and the like and suitable for drinks. <P>SOLUTION: The composition contains β-1, 3-1, 6-glucan and a polyphenol extracted from apple, especially, contains β-1, 3-1, 6-glucan obtained by cultivating a microbe belonging to genus Aureobasidium and polyphenol extracted from unripe fruits of the apple. The composition is useful as a drink, especially as a health drink, wherein vitamin C is preferably added to the drink to be pH4 to pH6. <P>COPYRIGHT: (C)2004,JPO

Description

The present invention relates to a composition containing β-1,3-1,6-glucan and a polyphenol extracted from apple, and a beverage comprising the same.

β-1,3-1,6-glucan is a polysaccharide in which a large number of glucoses are mutually linked by β-1,3 glucose bonds and β-1,6 glucose bonds. It is known to be a substance having various effects as described below, and is a substance useful for maintaining and promoting human health.
(1) Immunity-enhancing action: enhances the function of lymphocytes and improves immune function.
(2) Anti-tumor activity: After cancer cells have already developed and become ill, they attack the cancer cells.
(3) Cancer cell growth inhibitory action: After cancer cells are generated, their growth is suppressed.
(4) Antiallergic action: suppresses type I allergy such as atopic dermatitis.
(5) Anti-inflammatory action: enhances the protective function by improving the immune system.
(6) Cholesterol lowering action: lowers cholesterol in blood.
(7) Dietary fiber effect: adsorbs carcinogenic substances and discharges them out of the body.
(8) Antithrombotic action: Prevents the inside of blood vessels from narrowing or clogging.
(9) Blood pressure lowering action: When blood sent from the heart becomes abnormal due to the pressure applied to the artery wall, it returns to a normal state.
(10) Hypoglycemic action: lowers excessive glucose in blood.
(11) Liver hyperactivity: Improves the detoxification ability for liver function.

β-1,3-1,6-glucan is contained in mushrooms such as Kawatake mushroom, Shiitake mushroom, Suehirotake mushroom, and the like, and can be ingested by eating them. Ingestion is also possible. However, if eaten as it is, the absorption of β-1,3-1,6-glucan into the body is insufficient, and storage is not easy. Also, β-1,3-1,6-glucan can be extracted from these mushrooms, but it requires long-time cooking from a large amount of mushrooms, and is kept in a refrigerator or the like after the cooking. There is a need.

Japanese Patent Application Laid-Open No. 57-149301 (Patent Document 1) discloses that a microorganism belonging to the genus Aureobacidium, which is an incomplete fungus and a black bacterium belonging to the family Aureobacidium, has a non-reducing terminal from a main chain in which glucose is linked to β-1,3 glucose. Has a structure branched by a β-1,6 glucose bond, and produces a high-molecular polysaccharide in which a phosphate group is bonded to glucose. The microorganism used here is a microorganism of Deposit No. 4257 (FERM-P.4257).

Japanese Patent Application Laid-Open No. Hei 6-340701 (Patent Document 2) discloses that a β-1,3 linked glucose residue is used as a main chain by culturing Aureobacidium pullulans IFO4466 strain. It is described that a β-glucan having a branched chain of -1,6-linked glucose residues as a large number of side chains is produced.

In addition, the fact that a microorganism of the genus Aureobasidium produces β-1,3-1,6-glucan is described in Acta Chemical Scandinavia 17, 1351-1356 (1963) (Non-Patent Document 1), Agric. Biol. Chem. 47 (6), 1167-1172 (1983) (Non-Patent Document 2), @Chem. Pharm. Bull., 40, 2215 (1992) (Non-Patent Document 3) and the like.

As described above, a method of efficiently obtaining β-1,3-1,6-glucan by culturing a specific microorganism has been reported.

However, when a composition containing β-1,3-1,6-glucan is used for direct use by a general consumer, such as a health drink or a skin coating, it is liable to rot due to propagation of various bacteria during storage. There was a problem. In ordinary households, no special measures against falling bacteria are taken, so that even once sterilized compositions, bacteria often adhere during use. In particular, in the case of directly drinking or applying a composition containing the culture solution of aureobasidium, it is difficult to prevent decay over a long period of time because the composition is a liquid having a composition in which microorganisms can easily propagate in the first place. there were. However, the use of chemically synthesized bacteriostatic agents has a great resistance to natural-minded consumers for use as health drinks and skin application agents.

Β Further, β-1,3-1,6-glucan is susceptible to oxidation, and it is necessary to prevent oxidative deterioration for long-term storage. However, the use of chemically synthesized antioxidants also has a great resistance for natural-oriented consumers.

JP-A-57-149301 JP-A-6-340701 Acta Chemical Scandinavia 17, 1351-1356 (1963) Agric. Biol. Chem. 47 (6), 1167-1172 (1983) Chem. Pharm. Bull., 40, 2215 (1992)

The present invention solves these problems, and further provides a composition capable of enhancing the antioxidant and antiallergic effects in the body, and particularly provides a composition useful as a beverage. It is.

The above object is achieved by providing a composition containing β-1,3-1,6-glucan and polyphenols extracted from apple. Polyphenols extracted from apples, which are natural products, prevent the decay and oxidation of the β-1,3-1,6-glucan-containing composition, and further enhance the antioxidant and antiallergic effects in the body. is there. At this time, when the β-1,3-1,6-glucan is obtained by culturing aureobasidium, the effect of blending the polyphenol extracted from apple is remarkable. As the polyphenols extracted from apples, those extracted from immature fruits of apples are preferable. The composition is suitably used for applications applied to the human body as a medical composition or a pharmaceutical composition.

組成 The composition of the present invention is useful as a drink, particularly as a health drink, and various effects such as antitumor activity can be obtained by drinking. At this time, a beverage obtained by further mixing vitamin C and adjusting the pH to 4 to 6 is preferable.

By blending polyphenols extracted from apples with a composition containing β-1,3-1,6-glucan, it is possible to prevent decay and oxidation during storage and to have antioxidant and antiallergic effects in the body. Can also be enhanced. A composition useful for a beverage or a skin application can be provided.

組成 The composition of the present invention contains β-1,3-1,6-glucan. Here, β-1,3-1,6-glucan is a polysaccharide in which a large number of glucoses are mutually linked by β-1,3 glucose bonds and β-1,6 glucose bonds. Those having a structure in which glucose is branched at β-1,6 bonds from a main chain having glucose β-1,3 bonds (β-1,6-branched-β-1,3-glucan) are preferred. Having such a branched structure increases the physiological activity.

The β-1,3-1,6-glucan of the present invention contains glucose as a main component, but may contain a small amount of other constituent sugars. Preferably, the proportion of glucose in all constituent sugars is usually 90% or more. Further, the β-1,3-1,6-glucan of the present invention may have another functional group. In particular, having an acid group as another functional group enhances physiological activity. The acid group to be contained is preferably a phosphoric acid group, and in this case, the content of the phosphoric acid group is preferably at least 1 mol% based on glucose units.

分子 The molecular weight of β-1,3-1,6-glucan of the present invention is not particularly limited, and usually has a repeating structure of 100 or more glucose. Preferably, the number average molecular weight in the molecular weight measurement by an osmotic pressure method (measured using a cellophane semipermeable membrane using a Zimm-Myerson type osmometer) is about 50,000 to 500,000.

Β The content of β-1,3-1,6-glucan in the composition of the present invention is appropriately adjusted depending on the purpose of use, and a content of usually 0.001 to 5% by weight is exemplified. However, in consideration of the balance between production cost and effectiveness, the content is preferably 0.01 to 0.5% by weight, and more preferably 0.02 to 0.3% by weight.

The β-1,3-1,6-glucan used in the present invention is preferably obtained by culturing a microorganism of the genus Aureobacidium.
The microorganisms of the genus Aureobasidium that can be used are not particularly limited, and include, for example, bacteria of Microengineering Research Deposit No. 4257 (FERM-P.4257) and IFO4466 bacteria. Among them, the bacterium No. 4257 (FERM-P.4257) is preferable from the viewpoint of bioactivity.

It is possible to use β-1,3-1,6-glucan extracted and purified from the culture broth, but it is better to use the culture broth as it is in the composition without using any unnecessary processing. Meets the needs of nature-oriented consumers. It is also preferable in that the cost required for purification can be saved. At this time, the content of the culture solution in the composition is preferably 10 to 99.999% by weight.

The composition of the present invention also contains an apple extract. Apples contain various polyphenols that have various effects such as antioxidant, bacteriostatic, and antiallergic effects. They prevent decay and oxidation of the composition, and also have antioxidant and antiallergic properties in the body. It enhances the action.

In the case of a composition containing only β-1,3-1,6-glucan and not containing polyphenols extracted from apples, it was difficult to prevent rot for a long time in a general household. . This is greatly improved by further containing polyphenols extracted from apples. This is supported by the fact that the addition suppresses the growth of staphylococci and Escherichia coli in the examples described below.

Tea is a well-known polyphenol-containing food, but apple extract is more than 10 times more soluble in water than tea extract. Is preferred. In addition, compared to a tea extract having a strong bitterness, an apple extract has a smaller effect on taste, and is suitable for use in eating and drinking. In addition, since the tea extract is dark brown and the color of the product becomes brown, there is a possibility that the consumer may avoid using the tea extract when it is used for eating, drinking, coating, or the like.

リ ン ゴ It is more preferable that the apple extract to be used is extracted from immature apple fruits. Here, the immature fruit is one that is cut at a time when the weight per one is about 5 to 20 g, and one that is cut at a time when the polyphenol is most contained. Apple immature fruits contain about 10 times as many polyphenols as mature fruits. The polyphenols contained are apple condensed tannin, (+)-catechin, (-)-epicatechin, chlorogenic acid, dihydrochalcone, quercetin glycoside, p-coumarate and the like. An extract of immature apple fruit is available, for example, from Nikka Whiskey Co., Ltd. as "Applephenon (registered trademark)".

(4) The amount of the apple extract is appropriately adjusted depending on the purpose of use, and the content is typically 0.001 to 5% by weight without water. However, in consideration of the balance between production cost and effectiveness, the amount is preferably 0.01 to 1% by weight, more preferably 0.02 to 0.5% by weight, based on the weight of the composition. If it exceeds 5% by weight, it becomes bitter when used as a beverage and tends to be colored when subjected to heat sterilization. On the other hand, if the amount is less than 0.001% by weight, the effect of the blending is often insufficient.

The composition of the present invention contains the above β-1,3-1,6-glucan and polyphenol extracted from apple as essential components, and is usually used as an aqueous solution or a water-containing paste. If necessary, other components may be further added.

成分 The components to be blended are not particularly limited. Cordyceps sinensis, bear bamboo extract, matcha or kelp, which are plant-derived nutrients for the purpose of complementing macronutrients such as vitamins, minerals, chlorophyll and protein in a well-balanced manner; vitamin B1 or vitamin B6 for complementing neurotransmitter proliferation; Glucose, chlorella, powdered turtle powder, vitamin B12 or folate for supplementing hematopoietic regulation; alginic acid, catechin, licorice extract, glycyrrhizin, chlorella, tannin, vitamin C or propolis for supplementing antiviral function; Ginkgo biloba extract, γ-oryzanol, catechin, sesaminol, soybean saponin, tannin, vitamin E, vitamin B2 or vitamin C for the purpose of complementing the lipid-suppressing function; isomaltoligosaccharide, galactooligosaccharide, Kisil sucrose, ki Looligosaccharide, chitosan, glycomacropeptide, wheat fiber, corn fiber, soy oligosaccharide, hemicellulose or soy peptide, etc .; inositol, casein phos peptide or vitamin D, etc. for complementing calcium absorption; Suppon powder, vitamin C or heme iron; opioid peptide, gymnema, wheat fiber, corn fiber, tannin, maltooligosaccharide or hemicellulose may be added for the purpose of supplementing digestive absorption.

In addition, aloe extract, aloe vera extract, rose extract, seaweed extract, Emmeso, Erythrium, seaweed, sorghum, wormwood, licorice, kikyo, kumasasa, brown sugar, gennoshoko, burdock, chlorella, Shiitake, Shikon, Shiso, Peony, Juyaku, Iris, Senkyo, Senburi, Souhakuhi, Chimpi, Carrot, Touki, Loquat, Bukuryu, Peach, Yukinoshita, Yuzu, Reishi, Royal Jelly, Orange, Chamomile, Birch, Parsley, Butterfly, Tanpa Mulberry, fennel, garlic, lemon, Tochu tea and other extracts, vitamins, ginkgo biloba extract, chitosan, heme iron, vitamin D, blueberry extract, mucopolysaccharide protein, nucleic acid extract, collagen, konjac etc. may be added. .

方法 The method of using the composition of the present invention is not particularly limited, but suitable uses include food and beverage use and external use preparations.

First, a description will be given of a case where the composition is used as a food or drink, particularly a beverage. By drinking the composition of the present invention, a tumor-suppressing effect and an I-type allergic reaction-suppressing effect are obtained, and the storage stability is also improved, so that the composition is suitable as a health drink.

The beverage of the present invention contains β-1,3-1,6-glucan and polyphenols extracted from apple. At this time, if the polyphenol extracted from apples does not contain only β-1,3-1,6-glucan but does not contain polyphenols, the preservability is not sufficient, and various bacteria grow and rot or discolor. Easy to do. Moreover, when taken, there is a high incidence of side effects such as allergic rash and vomiting. Furthermore, the period until the effect of drinking tends to be long tends to be long.

When the composition containing β-1,3-1,6-glucan and polyphenol extracted from apple of the present invention is used as a beverage, vitamin C may be further added to the composition of the present invention. It is suitable.

Vitamin C is a water-soluble vitamin also called L-ascorbic acid, but cannot be synthesized in the body, and must be taken from food or the like every day. It is said that it has antioxidant, antiviral, detoxifying, and anticancer effects. However, in the present invention, β-1,3-1,6-glucan can enhance the tumor-suppressing effect and can be extracted from apple. It is particularly preferable to mix the polyphenols because they can enhance the antioxidant action of the obtained polyphenols. Vitamin C is easily oxidized during storage, but the combined effect of vitamin C can be maintained by using applephenone in combination. The amount of vitamin C is preferably 0.01 to 5% by weight, more preferably 0.02 to 2% by weight.

Further, when the composition of the present invention is used as a beverage, it is preferable to adjust the pH to 3 to 5. More preferably, the pH is 3.5 to 4.8. Usually, the pH of the aureobasidium culture solution is about 5.2, but if it is kept as it is, the preservability may be poor. By adjusting the pH to a slightly acidic side, the storage stability is improved. In addition, by doing so, a suitable acidity can be exhibited, and it becomes suitable for drinking also in terms of palatability. At this time, it is particularly preferable to adjust the pH by adding the above-mentioned vitamin C, since the effect of adding vitamin C is also obtained. In addition, the beverage of the present invention can also contain other sweeteners, flavors and the like.

The intake amount when the beverage of the present invention is used as a health drink should be appropriately adjusted depending on the health condition, disease symptoms, etc., and contains 0.18% by weight of β-1,3-1,6-glucan. It is standard to drink a beverage having a weight of 3 / 10,000 to 8/10000 of the body weight. That is, it is standard for a person weighing 60 kg to drink about 18 to 42 ml per day.

Since the beverage of the present invention has an effect of restoring and adjusting the immunity inherent in humans, it is expected to have an effect of improving various symptoms. Such effects are listed below, and various effects can be expected.
(1) The effect of reducing various allergic symptoms such as atopic dermatitis, hay fever, and asthma.
(2) Improvement effect on immunological disorders such as collagen disease, rheumatism and HIV.
(3) Suppressive effect on various cancers such as stomach cancer, lung cancer, colon cancer, uterine cancer, breast cancer.
(4) Improvement effect on vascular disorders such as myocardial infarction and cerebral infarction.
(5) Improvement effect on viral diseases such as hepatitis B and hepatitis C.
(6) Improvement effect on urinary system diseases such as diabetes and dysuria.
(7) The effect of improving digestive diseases such as constipation, diarrhea, stomatitis, hemorrhoids, anorexia, and hangover.

Next, the case where the composition is used as an external preparation, particularly as a skin coating agent, will be described. The composition containing the polyphenols extracted from β-1,3-1,6-glucan and apples of the present invention can be used to prevent itch against atopic dermatitis, dialysis pruritus, senile pruritus, xerosis, etc. It has an effect and is useful as a skin coating for those who have these symptoms.

Atopic dermatitis has recently become widely affected from infants to adults, and has become a major problem. In particular, many patients are suffering from severe itching, and there is a need for a method to stop itching. Atopic dermatitis has a wide variety of causes, such as diet, housing, chemicals, clothing, and stress, so it is not easy for specialists to find the cause and provide definitive solutions. There is often no choice but to provide symptomatic treatment.

From the viewpoint of dermatology, the present inventors have intensively studied to obtain a skin coating agent that can be easily applied to the skin and does not cause itching due to rash. As a result, they have found that the composition containing β-1,3-1,6-glucan and polyphenol extracted from apple of the present invention can achieve the above object. That is, by applying a skin coating composition comprising the composition of the present invention, a kind of protective film is formed on the skin of the affected area, and by maintaining the protection state for a long time, invasion and propagation of various bacteria into the affected area are prevented. It promotes the original regenerative power, and as a result, itching is reduced.

By containing polyphenols extracted from apple in addition to β-1,3-1,6-glucan, spoilage during storage can be prevented as described above, and long-term storage is easy. In addition, when it did not contain polyphenols extracted from apples and contained only β-1,3-1,6-glucan, itching was insufficient.

皮膚 The skin coating composition comprising the composition of the present invention preferably further contains horse oil. Horse oil has long been known to be effective in treating dermatitis, burns, cuts, abrasions and the like. Horse oil is a component extracted and refined from the subcutaneous fat of horses, has a moisturizing effect, an oil content adjusting effect, and can enhance the antipruritic effect. In addition, the absorption of the active ingredient can be improved. A preferred amount is 2 to 20% by weight, more preferably 3 to 15% by weight. If it exceeds 20% by weight, stickiness may occur after use, and if it is less than 2% by weight, the effect of blending is insufficient.

馬 The horse oil blended in the skin coating composition comprising the composition of the present invention is usually deproteinized, blood removed, deodorized and decolorized. Above all, those having a melting point of room temperature or lower, particularly 10 ° C. or lower, and being liquid at room temperature are preferable because they can improve the permeability of horse oil to the skin. When the melting point exceeds 10 ° C., it may take time for the protective agent to dissolve on the skin, or the usability such as elongation to the skin may be reduced. Examples of the method for adjusting the melting point include a method of adding hydrogen and a method of blending a high melting point wax such as beeswax.

皮膚 When the skin coating composition comprising the composition of the present invention contains horse oil and is used as an emulsion, it is preferable that the composition further contains a surfactant. This is because the water and the oil derived from horse oil can maintain a stable emulsified state. The preferred content of surfactant is 0.2 to 15% by weight.

ノ As the above-mentioned surfactant, a nonionic surfactant is suitable, and it is particularly preferable to mix and use both a nonionic surfactant having an HLB of 8 or more and a nonionic surfactant having an HLB of less than 8. The preferred content ratio of the former is 0.1 to 10% by weight and the latter is 0.1 to 10% by weight.

The reason why both nonionic surfactants having an HLB of 8 or more and nonionic surfactants having an HLB of less than 8 are used is to balance O / W emulsification and W / O emulsification. Examples of the nonionic surfactant include a polyhydric alcohol ester and an ethylene (propylene) oxide block copolymer. Examples of the nonionic surfactant having an HLB of 8 or more include polyethylene glycol monostearate, while examples of the nonionic surfactant having an HLB of less than 8 include glyceryl monostearate. It is preferable that at least one of the agents is of a self-emulsifying type. This is because if both nonionic surfactants are other than the self-emulsifying type, the temperature stability is reduced and it becomes difficult to prepare a uniform skin protective agent, and separation often occurs.

皮膚 Further, the skin coating composition comprising the composition of the present invention preferably contains a water-soluble polymer. The water-soluble polymer is blended to form a gel, and includes polysaccharides (guar gum, xanthan gum, hyaluronic acid, pectin, carrageenan, etc.), celluloses (methyl cellulose, ethyl cellulose, hydroxyethyl cellulose, etc.), starches (soluble Examples thereof include those based on starch, etc., those based on algin (eg, sodium alginate) and those based on synthetic polymers (eg, polyvinyl alcohol, sodium polyacrylate, carboxyvinyl polymer). The water-soluble polymer is usually blended in the form of a solution. The amount of the polymer itself in the skin protective agent is, for example, 0.1 to 5% by weight, and preferably 0.2 to 2% by weight.

皮膚 The skin coating composition comprising the composition of the present invention preferably contains a tea extract. By blending the tea extract, effects such as an antiallergic effect, an antibacterial effect, and an active oxygen suppressing effect can be enhanced. Main components in the tea extract include green tea catechins. Examples of green tea catechins include (+)-catechin, (−)-epicatechin, (+)-gallocatechin, (−)-epigallocatechin, (−)-epicatechin gallate, and (−)-epigallocatechin gallate. Is done. The content of the tea extract is preferably from 0.01 to 1% by weight, more preferably from 0.02 to 0.5% by weight.

皮膚 Further, the skin coating composition comprising the composition of the present invention preferably contains a licorice extract. An anti-inflammatory effect can be obtained by blending the licorice extract. The main component of the licorice extract includes glycyrrhizin, and glycyrrhizic acid or a salt thereof obtained by hydrolyzing glycyrrhizin can also be used. For example, dipotassium glycyrrhizinate and the like can be used. The content of the licorice extract is preferably from 0.01 to 1% by weight, more preferably from 0.02 to 0.5% by weight.

Further, it is preferable that the skin coating composition comprising the composition of the present invention contains allantoin. By containing allantoin, it is possible to reduce skin irritation and allergic reactions, and also has an effect of healing rough skin and wounds. The content of allantoin is preferably 0.01 to 1% by weight, more preferably 0.02 to 0.5% by weight.

皮膚 The skin coating composition comprising the composition of the present invention may contain a vegetable extract having skin astringency. Examples of the plant extract include a rose extract, an aloe extract, an arnica extract, a radish extract, a horsetail extract, a hypericum extract, a sage extract, an achillea millefolium extract, an altea extract, a chamomile extract, and a calendula extract. It is particularly preferable to incorporate a rose extract, and an aqueous solution extracted from rose petals can be incorporated.

皮膚 It is preferable that the pH of the skin coating composition comprising the composition of the present invention is 5 to 8, since skin irritation to sensitive skin is small. A more preferred pH is between 5.5 and 7.5. The pH is adjusted by adding an acid or an alkali.However, since the pH of the aureobasidium culture solution is usually about 5.2, the pH is adjusted to an alkaline side with an alkali such as potassium hydroxide or sodium hydroxide. Often do.

Hereinafter, the composition of the present invention will be specifically described with reference to examples.
First, an example in which the composition of the present invention is used for a health drink will be described.

[Example 1]
Cultivation of a microorganism belonging to the genus Aureobacidium of the incomplete fungus black bacterium Aureobacidium [Deposit No. 4257 (FERM-P.4257)] according to the method described in JP-A-57-149301. did. 0.18% by weight of a polymer polysaccharide having a structure in which a non-reducing end is branched by a β-1,6 glucose bond from a main chain in which glucose is β-1,3 glucose bonded and a phosphate group is bonded to glucose. The resulting culture broth was obtained. The pH of the main culture was 5.2.

に 対 し て To 500 kg of the main culture, 500 g of “Applephenone (registered trademark)” manufactured by Nikka Whiskey Co., Ltd., which is an extract of apple immature fruits, and 750 g of vitamin C were mixed, and the mixture was stirred in a kneading pot for 30 minutes. After transferring the obtained liquid to a filling tank, it was poured into a glass bottle having a capacity of 500 ml, stoppered, and then sterilized with steam at 85 ° C. for 30 minutes to obtain a health drink. The contents of β-1,3-1,6-glucan, apple extract and vitamin C in the health drink were 0.18% by weight, 0.1% by weight and 0.15% by weight, respectively, and the pH of the liquid was 4.2. .

[Tumor suppression test 1 (administration to mice)]
-Sample preparation method The supernatant of the health drink of Example 1 above was subjected to sonication treatment (200 W / 20 min.) Using an ultrasonic crusher (Ultrasonic Disruptor UR-200P), followed by ultracentrifugation (35000 rpm / 30 min.). Obtained and diluted 10-fold with HEPES Good buffer (ph7.4, μ0.15) were used as test materials.
As a comparative sample, a powder obtained by drying the fruit body of Agaricus mushroom was suspended in a HEPES Good buffer (ph7.4, μ0.15) to a concentration of 10% (w / v), and further, an ultrasonic crusher (Ultrasonic Disruptor). Using UR-200P), hot water extraction was performed for 2 hours after sonication treatment (200 W / 10 min.). Thereafter, a supernatant was obtained by ultracentrifugation (35000 rpm / 30 min.), And the supernatant was converted to a 1% (w / v) concentration based on the weight of the starting material to obtain a HEPES Good buffer (ph7.4, μ0.15). And diluted to obtain test materials.

·Test method
(1) Experimental animals:
BALB / c mice (female, 6 weeks old) were used in a group of 5 mice.
(2) Transplantation of Sarcoma180 solid tumor into mice:
Sarcoma (sarcoma) 180 cell line was subcultured in a 10% FCS / RPMI-1640 medium in a 37C / 5% CO ₂ incubator. The cells in the logarithmic growth phase (Full seat) were detached from the culture flask by Trypsin-EDTA, washed with RPMI-1640 culture solution, and used after adjusting the cell number to 5,000,000 cells / mL. This 0.1 ml was implanted subcutaneously on the back of each test mouse. All operations were performed aseptically.
(3) Method of administration of extract components From 24 hours after transplantation of Sarcoma180 solid cancer cells into mice, the test material was sterile-filtered with a 0.22 μm filter once a day (0.1 ml) for 14 days each. Administered intraperitoneally (ip).

-Test results The mice were sacrificed 3 weeks after tumor cell transplantation, the engrafted tumor weight (g) was measured after transplantation, and the tumor suppression rate (%) was calculated as compared with the control group (control). Table 1 shows the results. .
The control group here was one to which Na-Phosphate Buffered Saline (PBS) was administered instead of the test material.

よ う As is clear from the results, when the health food according to the present invention was administered, the tumor suppression rate was clearly higher than in the control group. In addition, when the health drink according to the present invention is used, compared with Agaricus mushrooms, which has been conventionally recognized as having an antitumor effect, a small amount (about 1/30 of the amount based on the amount) has the same tumor suppression effect Was found to be obtained.

[Tumor suppression test 2 (blood tumor cell growth suppression)]
Preparation following (1) to the cells of each cell line (6) at 37C / 5% CO ₂ incubator, under RPMI1640 culture environment containing 10% FCS, were suspended growth medium in a 25 cm ² culture Flask . When each cell was in the logarithmic growth phase, it was washed and replaced in an RPMI1640 culture medium environment to adjust the cell number to 400,000-800,000 cells / mL.

(1) CCRF-CEM cells:
Acute lymphoblastic leukemia-T lymphocyte (Human-lympoblast)
(Acute lymphocytic leukemia)
(2) K562 cells:
Chronic myelogenous leukemia-bone marrow (Human-lymphoblast)
(Chronic osteomyelitis)
(3) MOLT-4CL # 8 cells:
Acute lymphoblastic leukemia-T lymphoblast (Human-lymphoblast)
(Acute lymphocytic leukemia)
(4) U937 cells:
Histiocytic lymphoma-macrophage, histiocyte (Human-monocyte)
(Tissue lymphoma)
(5) Raji cells:
Burkitt lymphoma-EBV infected B lymphocyte (Human-lymphoblast)
(Burkitt lymphoma)
(6) YAC-1 cells:
Natural killer cell-sensitive lymphoma (Mouse-lymphoblast)
(NK cells)

-Reaction between tumor cells and test material Starting from the test material obtained from the health drink of Example 1 of the present application used in the above-described mouse anti-tumor experiment, a 10-fold diluted solution (1% stock solution), 20-fold A solution diluted with Na-Phosphate Buffered Saline (PBS) was prepared so as to be a 100-fold diluted solution, and this was sterile-filtered with a 0.22 μm filter to obtain a test material.
Further, 100 μl of each of the prepared cell suspensions prepared in the above (1) to (6) was dispensed into a 96-well cell culture plate, an equal amount of the test material was added thereto, and the mixture was mixed well. Reaction culture was performed in a 5% CO ₂ incubator for 36 hours.
Next, each of these cultured cells was stained with 0.5% Trypan blue, the number of viable cells after the reaction was counted, and compared with Control (PBS) as an antitumor (growth inhibitory) activity against each tumor cell. Calculated.

Test Results Table 2 shows the results of comparing the number of living cells and the ratio of living cells for each test material at each concentration with respect to each tumor cell, as compared to the control (Control). As is clear from the results, the health food according to the present invention has an antitumor effect on blood tumor cells.

[Type I allergic reaction suppression test]
-Test feed The amount of the health drink obtained in Example 1 corresponding to the daily intake of humans (40 ml for a body weight of 60 kg) was calculated from the weight ratio between humans and mice (about 20 g). About 25 to 30 times the calculated amount is the ingestion concentration (oral administration experiment setting concentration), evenly mixed in normal mouse breeding powder, solid stamping and radiation sterilization And used as a test feed. The substantial concentration in the mouse diet is about 5%. The control group received only normal mouse sterilized solid feed.

・ Experimental animals Using atopic dermatitis spontaneous mice (NC / Nga mouse, clean, CV; obtained from Japan SLC Co., Ltd. at 4 weeks of age) in groups of 10 males and 10 females The test was performed in a total of four groups: a test feed administration group and a control group.
All the above experimental animals were pre-bred for one week after arrival, and the observation period was from the 5th week to the 16th age.

・ Test method The breeding conditions are 24 ± 1 ° C, relative humidity 55 ± 5%, light and dark for 12 hours (lighting time: 7:00 am to 7:00 pm). The animals were bred in a barrier system animal breeding room (mouse and rat room) set to 12 times or more. For breeding, 4 to 6 animals were bred in a sterilized plastic cage having a sterile bedding. The cage was replaced once a week, and the feed was a solid feed (manufactured by Oriental Yeast Co., Ltd., CFR-1) placed in a feeder, and drinking water was fed freely in a sterilized water bottle with tap water and raised.

Regarding the measurement of the blood IgE level, four times, one week (6 weeks old), 4 weeks (9 weeks old), 7 weeks (12 weeks old) and 11 weeks (16 weeks old) after the feed intake Blood was collected from the vein layer of the fundus of the mouse over time, and the change over time in the total amount of IgE in the obtained serum was calculated by a sandwich ELISA (enzyme antibody method) using a specific antibody against mouse IgE.
In addition, gross skin findings were compared and observed 11 weeks after administration (16 weeks of age).

-Test results Table 3 shows the variation of blood IgE concentration with age in male and female mice. Although the total amount of blood IgE concentration tended to increase with the growth of the solid, the results showed that in the test feed intake group, suppression of blood IgE production was significantly observed as compared to the control group. Was. In particular, the blood IgE value 11 weeks after administration (16 weeks of age) was statistically subjected to a t-test in both male and female groups. As a result, a significant difference was found at a risk factor p <0.05.

In addition, in the gross skin findings at 16 weeks of age (usually allergic spontaneous age), the skin symptoms appeared in the control group in appearance, whereas the test feed administration group was normal in appearance, Compared with the control group, the test feed intake group clearly showed a tendency to suppress skin allergic symptoms.

From these results, it was clarified that the health drink of the present invention was effective in suppressing the onset of type I allergic reaction in mice, and was also suggested to be useful for suppressing the onset of allergic reaction in humans when equivalent components were taken. Although this result is a result of drinking, it is also suggested that it may be useful for suppressing the onset of allergic reaction even in the use of a skin application as described below.

[Antibacterial test]
・ Specimen Sample 1;
Aureobasidium culture solution cultured in the same manner as in Example 1 and 0.1% by weight of "Applephenone (registered trademark)" manufactured by Nikka Whiskey Co., Ltd. Sample 2;
Only Aureobasidium culture solution cultured as in Example 1

-Test bacteria Test bacteria 1;
Staphylococcus aureus IFO 12732
Test bacterium 2;
Klebsiella pneumoniae IFO 13277

・ Test method To 10 ml each of specimens 1 and 2, add the bacterial solution of the above-mentioned test bacteria 1 and 2 to each about 100,000 cells / ml, and store at 35 ° C. After a time, the number of viable bacteria in the test solution was measured. In addition, as a control, only the bacterial solution was similarly stored, and the number of viable bacteria was measured.

-Test results Table 4 summarizes the test results.
As is clear from the table, both the specimens 1 and 2 containing β-1,3-1 and 6-glucan exhibit antibacterial activity, indicating that they have an antibacterial effect against any test bacteria. Furthermore, it is clear from the viable cell count at the stage after 6 hours that the specimen 1 containing the apple extract further has a stronger antibacterial activity.

As described above, it has been proved that the combination of the apple extract is effective in preventing the decay of the β-1,3-1,6-glucan-containing composition due to propagation of various bacteria. From these results, it can be inferred that the combination of the apple extract has a putrefaction-preventing effect in both the beverage use and the skin application.

[Example 2]
Next, an example in which the composition of the present invention is used for a skin coating agent will be described.
The ratio of the blended raw materials is as follows.
・ Same culture solution as in Example 1 60% by weight
・ Immature apple extract 0.1% by weight
"Applephenon (registered trademark)" manufactured by Nikka Whiskey Co., Ltd.
・ Horse oil (melting point 8 ℃) 5% by weight
"Liquid horse oil W" manufactured by Ikko Chemical Co., Ltd.
・ Green tea extract (main component: green tea catechin) 0.05% by weight
“Sanphenon (registered trademark) 100S” manufactured by Taiyo Chemical Co., Ltd.
・ Dipotassium glycyrrhizinate 0.1% by weight
・ Allantoin 0.1% by weight
・ Rose extract 20% by weight
・ Methyl paraoxybenzoate 0.2% by weight
・ Ethyl paraoxybenzoate 0.05% by weight
・ Carboxyvinyl polymer 0.8% by weight
B. F. "Carbopol ULTRES-10" manufactured by Goodrich Chemical
・ 0.2% by weight of potassium hydroxide
・ Glycerin 5 parts by weight ・ Purified water 8.4% by weight

同 じ To the purified water, the same culture solution as in Example 1, dipotassium glycyrrhizinate, allantoin, methyl parahydroxybenzoate, ethyl paraoxybenzoate and glycerin were added and dissolved by heating to 80 ° C. This was once cooled, and a carboxyvinyl polymer was added. Further, potassium hydroxide was added, and the mixture was stirred and gelled. Next, the apple immature extract and green tea extract dissolved in a rose extract were added and mixed. Finally, horse oil was added and mixed well, and then filled into a container. The pH of the obtained skin application agent was 7.

[Coating test]
With the cooperation of 10 patients with atopic dermatitis, an application test of the skin application preparation of Example 2 was performed. The patient is a patient with mild and moderate atopic dermatitis and a pruritus score described later of 2 (mild) or more.

日 An appropriate amount of the skin application agent of Example 2 was applied directly to the affected area once to several times a day. At this time, rubbing after bathing or before going to bed was essential. The administration period was set to 4 weeks, and evaluation was performed every two weeks by confirming the presence of clinical symptoms and adverse events. However, three out of ten persons were not evaluated after four weeks. Regarding clinical symptoms, scores were evaluated for each item on a 5-point scale based on the following criteria.

・ Itching It was judged based on the following criteria based on the patient's self-report.
0; no itching during the day No itching at night.
1: It is not necessary to be patient during the day. Sleeps well at night but is slightly itchy.
2: During the day, sometimes scratching does not matter. At night, itching can be a bit irritated and subsides.
3: Irritated and constantly scratching during the day. At night, she wakes up and scratches while sleeping.
4: Can't stand even during the day. At night, itchy and unable to sleep.

・ Flush 0: None 1: Minor (only slight redness)
2; Mild (slightly reddish with mild edema)
3: Moderate (clear reddish, mild edema)
4: High (bright red or purple-red, with edema conspicuous)

・ Papules 0; None 1: Minor (slight papules)
2; Mild (a few papules are seen)
3: moderate (between mild and altitude)
4: Altitude (a large number of papules exist or aggregate)

・ Dry roughening (keratin keratinization)
0; none 1; minor (between none and mild)
2; Mild (slightly roughened skin with slight pore conformational keratinization)
3: moderate (between mild and altitude)
4: High (skin is very rough and pore conformation keratinization is conspicuous)

・ Exfoliation (scratch, scratch marks)
0; None 1; Minor 2; Mild 3; Moderate 4;

・ Scale 0; none 1: slight (slight scale is observed)
2: Mild (skin is slightly dry and pathological keratin is slightly flat on skin surface)
3: Moderate (the whole skin is very dry)
4; altitude (state where the whole skin is dry, pathological keratin is raised from the skin surface, and peels off)

Table 5 shows the test results. As is clear from the test results, the score of the evaluation score was lowered in the items of pruritus, flushing, papules, dry roughening, and scales, and was flat in the exfoliation. As an adverse event, only one (C) complained of dry skin. Thus, it was confirmed that the skin application preparation of the present invention was effective in improving various symptoms of atopic dermatitis.

[Storage test]
The skin coating preparation obtained in Example 2 was stored in a sealed thermostat at 40 ° C. (dark place) in a sealed state, and the appearance of the contents was observed every month. As a result, there was no significant change in appearance and no separation was observed after 1 month, 2 months, and 3 months. In the storage test at 40 ° C., one month corresponds to about three months at room temperature. It was found that the skin application obtained in Example 2 had sufficient storage stability.

Claims (5)

A composition containing polyphenols extracted from β-1,3-1,6-glucan and apple. The composition according to claim 1, wherein the β-1,3-1,6-glucan is obtained by culturing a microorganism of the genus Aureobasidium. The composition according to claim 1 or 2, wherein the polyphenols extracted from apples are extracted from immature fruits of apples. A beverage comprising the composition according to claim 1. The beverage according to claim 4, wherein the pH is adjusted to 4 to 6 by further mixing vitamin C.