JP6453534B2 - Lipid metabolism promoter - Google Patents

Description

  The present invention relates to a lipid metabolism promoter, and more particularly, to a lipid metabolism promoter comprising lactic acid and / or a salt thereof as an active ingredient.

  Obesity is one of the most serious diseases in modern society, but its main factor is fat overdose. It is known that excessive intake of fat causes not only obesity but also lifestyle-related diseases such as metabolic syndrome, diabetes, hyperlipidemia, hypertension and arteriosclerosis due to obesity.

  As a therapeutic agent for obesity, mazindol, an appetite suppressant, orlistat, a lipase inhibitor, and the like are used. However, these medications include dry mouth, constipation, nausea, insomnia, headache and palpitations, as well as oil spots, flatulence, sudden constipation, increased defecation, stool incontinence, rectal leakage, upper respiratory infections and fatty stools Such side effects have been reported, and safety is not necessarily sufficient.

  In order to prevent obesity, reducing calorie intake by dietary restriction is an effective means. However, sufficient nutritional guidance is required for this purpose, and it is often difficult to implement in daily life. Therefore, there is a strong demand for a substance that has sufficient safety and can effectively eliminate obesity.

  On the other hand, lactic acid is a substance synthesized as a result of lactic acid metabolism in order to obtain ATP from glucose transiently in the body when a rapid exercise (anoxic exercise) is performed. The blood concentration of lactic acid at rest is about 0.5 to 2.0 mM, but the blood concentration of lactic acid generated as a result of exercise is about 4 to 5 mM. In addition, it is known that the blood concentration of lactic acid rises to about 20 mM when exercise is performed so as to cause nausea.

  Lactic acid synthesized in the body is transported to the liver by blood circulation, converted into pyruvate by lactate dehydrogenase, and then glucose is regenerated by gluconeogenesis. This series of circuits is called a lactic acid circuit or a coli circuit. There is a limit point where lactic acid accumulation exceeds the metabolic removal of lactic acid during exercise accompanied by insufficient oxygen supply, and the point at which blood lactic acid concentration starts to increase rapidly is called the lactic acid accumulation threshold. In aerobic exercise training, the lactic acid accumulation threshold is sometimes used as an oxygen supply index to be used for setting exercise intensity.

  Thus, it is lactic acid synthesized and metabolized in the body, but it is also contained in foods, and it is known that it is contained in fermented foods in particular. Examples of such fermented foods include yogurt and pickles. Moreover, it is contained in a drink and it is disclosed that it is used as a sourness imparting substance to a drink (patent documents 1-3). However, it is not known that such lactic acid is used for relieving obesity, and use as a lipid metabolism promoter has not been reported so far.

JP 2011-254731 A Special table 2010-521163 Special table 2011-521167 gazette

  The objective of this invention is providing the agent and composition which can accelerate | stimulate a lipid metabolism safely and efficiently as a substance useful for elimination of obesity.

Means to solve the problem

  As a result of intensive studies to solve the above problems, the present inventors have surprisingly found that lactic acid and / or a salt thereof has an action of promoting lipid metabolism. Based on this finding, the present inventors have completed the present invention through further research.

That is, the present invention relates to the following.
[1] A lipid metabolism promoter comprising lactic acid and / or a salt thereof as an active ingredient.
[2] The agent according to [1], further containing caffeine.
[3] The content ratio of lactic acid and / or a salt thereof and caffeine is 0.9: 1 as a weight ratio (however, in the weight of lactate, a value converted to the weight as lactic acid is used) The agent according to [2], which is ˜1000: 1.
[4] The agent according to any one of [1] to [3], wherein the lipid metabolism promotion is a reduction in body fat.
[5] A composition having a lipid metabolism promoting action, comprising lactic acid and / or a salt thereof as an active ingredient.
[6] The composition according to [5], further comprising caffeine.
[7] The content ratio of lactic acid and / or a salt thereof and caffeine is 0.9: 1 as a weight ratio (however, in the weight of lactate, a value converted to the weight as lactic acid is used) The composition according to [6], which is ˜1000: 1.
[8] The composition according to any one of [5] to [7], wherein the lipid metabolism promoting action is a body fat reducing action.
[9] The composition according to any one of [5] to [8], which is a medicine.
[10] The composition according to any one of [5] to [8], which is a food or drink.

  ADVANTAGE OF THE INVENTION According to this invention, the agent and composition which can accelerate | stimulate lipid metabolism efficiently can be provided. In addition, lactic acid and / or a salt thereof used in the present invention is not only a substance synthesized in the body but also designated as a food additive in Japan, and used as an acidulant and pH adjuster for foods and drinks. Since it is possible, it can be said that the agent and composition of the present invention have sufficient safety for animals such as humans.

FIG. 1 is a graph showing the amount of glycerol released from fat cells. The vertical axis of the graph represents the relative value when the measured value of the glycerol release amount in the comparative example is 1. FIG. 2 is a graph showing the amount of free fatty acid released from fat cells. The vertical axis of the graph represents the relative value when the measured value of the amount of released free fatty acid in the comparative example is 1. FIG. 3 is a graph showing the amount of weight loss of rats. The vertical axis of the graph represents the ratio (%) when the weight of the exercise group is 100%. The horizontal axis indicates other groups (Lac + Caf: exercise + LC group, Lac: exercise + L group). FIG. 4 is a graph showing the amount of decrease in visceral fat in rats. The vertical axis of the graph represents the percentage (%) when the visceral fat mass measured in the exercise group is 100%. The horizontal axis indicates other groups (Lac + Caf: exercise + LC group, Lac: exercise + L group). FIG. 5 is a graph showing the amount of reduction in subcutaneous fat in rats. The vertical axis of the graph represents the percentage (%) when the subcutaneous fat mass measured in the exercise group is 100%. The horizontal axis indicates other groups (Lac + Caf: exercise + LC group, Lac: exercise + L group).

  In the process of studying the physiological function of lactic acid, the present inventor has surprisingly found that lactic acid has an action of promoting lipid metabolism when cells are cultured under the condition of adding lactic acid. That is, based on this finding, the present invention provides a lipid metabolism promoter comprising lactic acid and / or a salt thereof as an active ingredient (hereinafter referred to as “the agent of the present invention”).

Lactic acid used in the present invention is a compound represented by the chemical formula CH ₃ —CH (OH) —COOH. As lactic acid, any of D-form (D-lactic acid), L-form (L-lactic acid) and DL-form (DL-lactic acid) can be used. In the present invention, L-form and DL-form are preferred, and more preferred L-form is used. The CAS registration number for D-form is 79-33-4, the CAS registration number for L-form is 10326-41-7, and the CAS registration number for DL-form is 598-82-3 or 50-21-5. It is.

  Moreover, the salt of lactic acid is not particularly limited. For example, alkali metal salts such as sodium and potassium (specifically, sodium lactate and potassium lactate), alkaline earth metal salts such as calcium and magnesium (specifically Examples thereof include calcium lactate and magnesium lactate), aluminum lactate, zinc lactate, manganese lactate and iron lactate. The salt of lactic acid in the present invention is preferably sodium lactate or calcium lactate. In the present invention, the lactic acid salt may be a hydrate.

  The lactic acid and salts thereof used in the present invention are not particularly limited as to how to obtain them, and may be any of those derived from animals or plants, or those obtained by chemical synthesis or fermentation. . Based on the purity and production cost of the obtained lactic acid and its salt, a suitable method for producing lactic acid and its salt can be appropriately selected. In the present invention, commercially available lactic acid and salts thereof can be used. Examples of such commercially available products include products manufactured or sold by Musashino Chemical Laboratory, Inc., Fuso Chemical Industry Co., Ltd., Naito Shoten Co., Ltd., Wako Pure Chemical Industries, Ltd., and the like. In the present invention, lactic acid or a composition containing lactic acid (such as a food or drink) obtained while culturing bacteria (lactic acid bacteria or the like) using a fermentation method can be used as it is or after being processed.

  In vivo, it is known that the concentration of intracellular calcium such as muscle cells increases as a physiological phenomenon caused by exercise or the like. As a substance that is commonly used in foods and can increase intracellular calcium concentration in the living body for the purpose of increasing intracellular calcium concentration such as muscle cells without exercising. Caffeine can be used additionally. That is, the agent of the present invention can further contain caffeine.

  Caffeine is a kind of purine alkaloid having a purine ring, and is a component contained in coffee beans, green tea, black tea, and the like. The IUPAC name for caffeine is 1,3,7-trimethylxanthine, and its CAS registry number is 58-08-2.

  Caffeine in the present invention includes both anhydrous (also referred to as “anhydrous caffeine”) and hydrate (eg, monohydrate) embodiments. Any embodiment can be used in the present invention, but preferably an anhydride is used.

  The caffeine used in the present invention is not particularly limited, and may be, for example, a crystal obtained by chemical synthesis or the like, or a plant extract containing caffeine as it is or after being concentrated or purified (ie, In addition, a component other than caffeine may be selectively removed from a plant extract containing caffeine to increase the content of caffeine). A suitable method for producing caffeine can be appropriately selected based on the purity and production cost of the obtained caffeine. The plant extract containing caffeine is not particularly limited. For example, it is known per se in solvents such as coffee beans, cola fruits, tea leaves, cacao, etc., water (or hot water), methanol, ethanol, isopropanol, ethyl acetate and the like. It is manufactured by extracting using a method.

  In the present invention, commercially available caffeine can be used. As such a commercial item, the goods manufactured or sold by Shiratori Pharmaceutical Co., Ltd., Wako Pure Chemical Industries, Ltd., etc. are mentioned, for example.

  The content ratio of lactic acid and / or salt thereof to caffeine in the agent of the present invention (lactic acid and / or salt thereof: caffeine) is usually 0.9: 1 to 1000: 1 as a weight ratio. The content ratio is preferably 0.9: 1 to 500: 1, more preferably 0.928: 1 to 100: 1, and still more preferably 0.928: 1 to 22.32: 1. It is. When the ratio between the two is within the above range, lipid metabolism can be efficiently promoted. In addition, when using the salt of lactic acid, the said weight ratio shall be calculated after converting into the free body (free body) of lactic acid. In the present invention, the weight converted in this way is handled as “a value converted into the weight as lactic acid”. Moreover, when each active ingredient forms the hydrate, the said weight ratio shall be calculated after converting into the free body (anhydride) except the water molecule.

  In the present invention, when referred to as “lipid metabolism promoter”, the agent of the present invention has an action of “facilitating lipid metabolism”, where “facilitating lipid metabolism” refers to promoting lipid metabolism in vivo. It means having an action. As used herein, “lipid” is a general term for water-insoluble substances existing in a living body. In the present invention, the lipid may be solid at room temperature or liquid, but is preferably solid. In addition, normal temperature shows that it is 15-25 degreeC normally according to the 16th revision Japanese Pharmacopoeia general rule. Lipids include, for example, simple lipids (neutral fats, waxes, etc.), complex lipids (phospholipids, glycolipids, etc.), derived lipids and the like. Among these, the lipid targeted in the present invention is preferably a simple lipid, more preferably a neutral fat, and most preferably triacylglycerol (triglyceride). In the present specification, “metabolism” of lipid mainly indicates degradation of lipid, but is not particularly limited as long as the amount of lipid can be reduced.

  In the present invention, “facilitation of lipid metabolism” includes the concept of reducing lipid in the living body (sometimes referred to as “burning of lipid”) and reducing the amount of lipid ingested from outside the body. And the concept of inhibiting lipid accumulation. In the present invention, although not particularly limited, promotion of lipid metabolism preferably means reducing lipids in the living body. Examples of the lipid in the present invention include body fat (subcutaneous fat, visceral fat, etc.) and blood lipid, but body fat is preferred.

  The agent of the present invention can prevent and treat obesity (also referred to as “obesity”) through the action of promoting lipid metabolism. Furthermore, the agent of the present invention can also prevent and treat diseases that develop due to obesity. Examples of such diseases include, but are not limited to, metabolic syndrome, diabetes (including type 2 diabetes), hyperlipidemia, hypertension, arteriosclerosis and the like. Thereby, this invention can also provide the preventive and therapeutic agent of the said disease.

  The agent of the present invention is useful as a medicine and food, and the application target thereof can be a mammal. Examples of such mammals include primates (eg, humans, monkeys, chimpanzees), rodents (eg, mice, rats, guinea pigs), pets (eg, dogs, cats, rabbits), working animals or livestock. (For example, cows, horses, pigs, sheep, goats) can be mentioned, but humans are preferred in the present invention. When applied to mammals other than humans, the dose (intake amount) of the agent of the present invention may be appropriately adjusted depending on the body weight or size of the animal.

  The agent of the present invention can be formulated into a composition by a conventional method using an appropriate pharmaceutically acceptable carrier as necessary in the formulation (hereinafter referred to as “the composition of the present invention”). ). Thereby, it can be said that the composition of this invention contains the agent of this invention. Since the composition of this invention contains the agent of this invention, it can have all the effects exhibited by the agent of this invention. That is, the composition of the present invention is characterized by having an action of promoting lipid metabolism, wherein “facilitating lipid metabolism” means having an action of promoting lipid metabolism in a living body. Although not particularly limited, promoting lipid metabolism preferably means reducing lipids in the living body. Examples of the lipid in the present invention include body fat (subcutaneous fat, visceral fat, etc.) and blood lipid, but body fat is preferred.

  The carrier can be appropriately selected depending on the dosage form of the preparation (composition), and is not particularly limited. For example, the excipient, binder, lubricant, disintegrant, solvent, stabilizer, solubilizer And additives such as antioxidants, coloring agents, flavoring agents, sweetening agents and the like.

  Excipients include sugars (sucrose, lactose, glucose, mannitol, etc.), starches (corn starch, etc.), crystalline cellulose, calcium phosphate, calcium sulfate, magnesium sulfate, etc., and binders include pregelatinized starch, gelatin, tragacanth gum, Gum arabic, methylcellulose, carboxymethylcellulose, sodium carboxymethylcellulose, crystalline cellulose, hydroxypropylcellulose, hydroxypropylmethylcellulose, polyvinylpyrrolidone, polyvinyl alcohol, etc., lubricants include magnesium stearate, talc, polyethylene glycol, silica, hydrogenated vegetable oil As disintegrants, starch, crystalline cellulose, carboxymethylcellulose, agar, calcium citrate, calcium carbonate, charcoal Sodium hydrogen, dextrin, etc., the solvent is water, ethanol, glycerol, physiological saline, soybean oil, etc., and the stabilizer is benzoic acid, sodium benzoate, ethyl paraoxybenzoate, propylene glycol, etc. Examples of solubilizers include fumaric acid, succinic acid, and malic acid, and examples of antioxidants include ascorbic acid, tocopherol, sodium bisulfite, sodium thiosulfate, sodium pyrosulfite, and citric acid. Examples of the agent and sweetener include those that are normally allowed to be added in the fields of medicine and food.

  As in the case of the agent of the present invention, the composition of the present invention can further contain caffeine, and the content ratio of lactic acid and / or a salt thereof to caffeine in the composition of the present invention (lactic acid and (Or salt thereof: caffeine) is also generally in a weight ratio of 0.9: 1 to 1000: 1, preferably 0.9: 1 to 500: 1, as in the case of the agent of the present invention. More preferably, it is 0.928: 1-100: 1, More preferably, it is 0.928: 1-22.32: 1. When the ratio between the two is within the above range, lipid metabolism can be efficiently promoted. In addition, when using the salt of lactic acid, the said weight ratio shall be calculated after converting into the free body (free body) of lactic acid. In the present invention, the weight converted in this way is handled as “a value converted into the weight as lactic acid”. Moreover, when each active ingredient forms the hydrate, the said weight ratio shall be calculated after converting into the free body (anhydride) except the water molecule.

  The above-mentioned lactic acid, lactic acid salt and caffeine may be formulated simultaneously in a single formulation, or may be formulated in separate formulations. When separate preparations are used, the preparations are used in combination. In the present invention, it is preferable to use lactic acid and / or a salt thereof and caffeine in a single preparation for ease of administration or ingestion.

  The content of lactic acid and / or a salt thereof in the composition of the present invention is usually 0.10 to 99.99% by weight, preferably 0.60 to 99.90, based on the total weight of the composition of the present invention. % By weight, more preferably 1.00 to 99.90% by weight. In addition, the content of caffeine in the composition of the present invention is usually 0.01 to 33.33% by weight, preferably 0.02 to 33.30% by weight, based on the total weight of the composition of the present invention. More preferably, it is 0.04 to 33.30% by weight. As with the above weight ratio, when using a salt of lactic acid, the content is calculated after conversion to a free form of lactic acid, and when each active ingredient forms a hydrate, The content is calculated after conversion to a free form (anhydride) excluding water molecules. The above content range can also be adopted when lactic acid and / or a salt thereof and caffeine are formulated in separate formulations.

  The composition of the present invention can be used as a medicament (ie, a pharmaceutical composition). In this case, the pharmaceutical composition of the present invention can be handled as a preventive or therapeutic agent for diseases associated with abnormal lipid metabolism, and such diseases are as described above.

  The administration method of the pharmaceutical composition of the present invention is not particularly limited, and generally includes an oral administration method. Depending on the condition, severity, etc. of the subject patient, parenteral administration (intravascular ( (Intravenous, intraarterial) administration, subcutaneous administration, transdermal administration, intrarectal administration, etc.) may be appropriately selected. Since any of lactic acid and / or a salt thereof and caffeine, which are active ingredients, can be consumed, it is preferable to employ oral administration in the present invention.

  The dosage form of the pharmaceutical composition of the present invention is not particularly limited, and can be in a form suitable for the administration method. Forms suitable for oral administration include, for example, tablets, lozenges, hard or soft capsules, aqueous or oily suspensions, emulsions, dispersible powders or granules, syrups or elixirs, and the like. Suitable forms for parenteral administration include, for example, sterile solutions, suspensions, emulsions, and the like for intravenous, subcutaneous, intramuscular, intravascular or infusion administration as forms suitable for parenteral injection. Suitable forms for administration include creams, ointments, gels, aqueous or oily solutions (including suspensions) and the like.

  The composition of the present invention can also be used as a food or drink (ie, a food or drink composition). In this case, the food / beverage composition of the present invention can be formulated by a conventional method using a carrier usually used in the field of food / beverage products in addition to the pharmaceutically acceptable carrier described above.

  The food and drink in the present invention means all food and drink, but in addition to general foods including so-called health foods, special-purpose foods specified by the Consumer Affairs Agency (specific health foods, sick foods, difficult to swallow) Foods for consumers, etc.) and functional foods, and supplements, feeds and the like are also included in the food and drink of the present invention.

  The dosage form of the food / beverage composition of the present invention is not particularly limited. Fine granules, granules, pills, tablets (including coated tablets and dragees), capsules (including hard capsules, soft capsules, and microcapsules) , Beverages, drinks, liquids (including syrups, emulsions, suspensions), powdered foods, jellies, rice cakes and the like.

  The dose (intake) of the agent and composition of the present invention is not particularly limited as long as it is within the effective amount range in which the lipid metabolism promoting action can be expressed in the body. It can be set appropriately according to the administration method and the like. Further, the daily dose (intake) can be administered (intake) at one time or divided into several times (for example, two or three times). Administration (intake) of the agent and composition of the present invention is not particularly limited as long as the effect of the present invention is exhibited, regardless of whether it is before, after, or between meals. Hereinafter, when the term “administration” is used herein, the term is meant to encompass the concept of “ingestion”.

  As described above, lactic acid and / or a salt thereof and caffeine can be formulated into separate formulations, in which case both formulations can be used in combination in the present invention. Lactic acid and / or its salt and caffeine may be administered simultaneously or may be administered sequentially in any order.

  When using the agent and composition of the present invention, it can also be used in combination with existing components having a lipid metabolism promoting action. In such a case, the order of administering the agent and composition of the present invention and the existing component may be simultaneous or separate. In separate cases, administration of the agents and compositions of the present invention may be either before or after the existing components.

  Examples of the existing components include tea extract, cacao extract, coffee bean manno-oligosaccharide, apple-derived procyanidins, transglycosyl hesperidin, resveratrol, green citrus extract, citrus nalidinine, glucosamine, mushroom chitosan, chitosan, diacyl. Glycerol, medium chain fatty acid, EPA, DHA, soybean protein, plant sterol (β-sitosterol, etc.), psyllium seed coat-derived dietary fiber, low molecular weight sodium alginate, guarana, ginger, garcinia, globin proteolysate, carnitine, α- Examples include lipoic acid, plant stanol esters, phospholipid-bound soybean peptides, or combinations thereof, but are not particularly limited thereto.

  The present invention will be described more specifically with reference to the following examples. However, these are merely examples and do not limit the scope of the present invention.

Example I. Effects of lactic acid and caffeine in cell tests (in vitro)
Mouse preadipocytes 3T3-L1 (purchased from ATCC) are differentiated with 12 well-dish, and then lactic acid (manufactured by Wako Pure Chemical Industries, Ltd.) and caffeine (concentrated in units of mmol) shown in Table 1 The medium was changed to 10% serum-containing DMEM medium (Wako Pure Chemical Industries, Ltd.) supplemented with Wako Pure Chemical Industries, Ltd., and static culture was performed at 37 ° C. for 18 hours.

  The adipocytes treated as described above were washed twice with Hank's buffer and washed with 1 mL of DMEM medium containing 2% BSA (no fatty acid), 20 mM HEPES, 0.5 mM IBMX, 10 μM isoprotenol at 37 ° C. For 6 hours. Thereafter, the culture supernatant was collected, and the amounts of glycerol and free fatty acids in the supernatant were measured. The amount of glycerol and fatty acid was determined using an absorbance method (measurement wavelength glycerol: 600 nm, Triglyceride E-test kit (manufactured by Wako Pure Chemical Industries, Ltd.) and NEFA C-test kit (manufactured by Wako Pure Chemical Industries, Ltd.), respectively. Free fatty acid: 550 nm, measuring instrument: xMark (manufactured by BIO-RAD)). The measurement results and the relative values with the comparative examples are shown in Tables 2 and 3.

As shown in Table 2 and Table 3, it was revealed that the glycerol release amount and the free fatty acid release amount in Examples 1 to 7 were larger than those in Comparative Examples. Further, in Examples 5 and 6 in which lactic acid and caffeine were combined, it was shown that the amount of glycerol released and the amount of released free fatty acid were higher than those in Examples 1 to 4 in which only lactic acid was added. Furthermore, the relative value of the glycerol release amount and the relative value of the free fatty acid release amount were the same in all examples.
From the above results, it was suggested that lactic acid and the combination of lactic acid and caffeine degrade fat in cells, that is, have a body fat reducing action.

Example II. Effects of lactic acid and caffeine in animal studies (in vivo)
1. Test materials and methods 1.1. Test substance and medium 1.1.1. Test substances Sodium lactate (Wako Pure Chemical Industries, Ltd.) and caffeine (Wako Pure Chemical Industries, Ltd.) were used. After acquisition, all were stored in the storage of the test substance storage room of the test facility at room temperature (set temperature: 23 ° C., allowable range: 18.0 to 28.0 ° C.).

1.1.2. Medium Water for injection (manufactured by Otsuka Pharmaceutical Factory) was used. After acquisition, it was stored in the test substance storage room of the test facility under conditions of room temperature (set temperature: 23 ° C., actual measurement: 18.0 to 28.0 ° C.).

1.2. Samples to be administered Weighed the required amounts of sodium lactate and caffeine, and then mixed and dissolved with water for injection so that the final concentrations were 200 mg / mL and 7.2 mg / mL, respectively (the mixture was the test substance LC )

1.3. Test system 1.3.1. Test animals and rearing conditions In the test, male F344 rats (SPF, Japan SLC Co., Ltd.), which is an animal species generally used in pharmacological pharmacological tests and whose lineage is clearly maintained, were used.
The animals were bred in an animal breeding facility set at a preset temperature: 23 ° C. and light and dark for 12 hours each (lighting: 8 am to 8 pm). Cages and feeders were changed at least once a week.
For the feed, a solid high-fat feed (HFD-60, Oriental Yeast Co., Ltd.) within 5 months after production was placed in a feeder and allowed to feed freely.

1.3.2. Grouping High-fat diet HFD-60 was ad libitum for 6 weeks to 5-week-old rats. At the age of 11 weeks, the rats were randomly classified into exercise group (n = 9), exercise + L group (n = 9), exercise + LC group (n = 9).

1.3.3. Individual Identification Method and Cage Label Animals were identified on the date of acquisition by combining the method of filling the tail with oil-based ink and the method of applying dye to the limbs using oil-based ink. After grouping, it was identified by entering the animal number (last 3 digits) on the tail using oil-based ink. Each cage is labeled with the test number, date of acquisition, and the number of the pre-reserved animal during the pre-breeding period. After the grouping, the test number, group name, and animal number are entered, and each group is color-coded. A label was attached.

1.3.4. Exercise load The exercise load was a voluntary running exercise with a frequency of three times a week and once every two days. For the spontaneous running exercise, a rotary exercise machine (Lafayette Instrument, model No. 80859) was used.

1.3.5. Administration Administration was forcibly orally administered using a disposable syringe (made by Terumo Corporation) made of polypropylene with a metal gastric sonde for rats attached in accordance with the usual method used in the test facility. During the administration operation, the required amount was aspirated into the syringe while stirring the administration specimen by inversion mixing.
Within 30 minutes after the end of spontaneous running (from 10:00 am), the liquid volume was calculated at 5 mL / kg from the body weight value on the measurement day closest to the administration day, and administered once a day for 5 weeks.

1.3.6. Group composition

1.4. Test method 1.4.1. General condition The general condition and the presence or absence of death were observed once a day in the dark period (the day of administration before administration).

1.4.2. Body weight measurement It was measured once a week before administration and on the day of necropsy.

1.4.3. Measurement of food intake It was measured once a week before administration.

1.4.4. Necropsy On day 35 after administration, blood was collected from the abdominal aorta using a winged intravenous needle under anesthesia with 4% sodium pentobarbital. The animals were then euthanized by pentobarbital sodium overdose, and the fat (peri-testicular fat and subcutaneous fat) and the heart, liver, adrenal gland, and brain were removed. Then, the weight of fat was measured.

2. Results The body weight in the exercise group, the weight of the built-in fat and the weight of the subcutaneous fat were taken as 100%, and the ratios in the exercise + L group and exercise + LC group were calculated respectively, and the rat's body weight and weight were measured around the accessory testicular fat ( Visceral fat) and subcutaneous fat were evaluated for reduction in each group.
As a result, in the exercise + L group, the body weight of the rats was decreased as compared with the exercise group, and the amounts of visceral fat and subcutaneous fat were also decreased as compared with the exercise group. Similarly, in the exercise + LC group, the body weight of the rat and the amounts of visceral fat and subcutaneous fat were decreased from those in the exercise group, but the decreased amounts were more than those in the exercise + L group. From these results, it was suggested that lactic acid has a lipid metabolism improving action in vivo, and the action is further enhanced by using it together with caffeine.

Formulation example:
Based on the results of Example I and Example II, the following formulation examples are presented.

Formulation Example 1
Beverages were produced with the compositions shown in Table 5.

Formulation example 2
Beverages were produced with the compositions shown in Table 6.

Formulation Example 3
Beverages were produced with the compositions shown in Table 7.

Formulation Example 4
Beverages were produced with the compositions shown in Table 8.

Formulation Example 5
Beverages were produced with the compositions shown in Table 9.

Formulation Example 6
Hard capsules were produced with the compositions shown in Table 10.

Formulation Example 7
Hard capsules were produced with the compositions shown in Table 11.

Formulation Example 8
Hard capsules were produced with the compositions shown in Table 12.

Formulation Example 9
Beverages were produced with the compositions shown in Table 13.

Formulation Example 10
Beverages were produced with the compositions shown in Table 14.

  The agent and composition of the present invention have a lipid metabolism promoting action and are useful in the pharmaceutical field, and from the viewpoint of extremely high safety, they are useful not only in the pharmaceutical field but also in the food field.

Claims (8)

A lipid metabolism promoter for reducing body fat, comprising lactic acid and / or a salt thereof as an active ingredient (except for those containing lactic acid bacteria) .   The agent according to claim 1, further comprising caffeine. The content ratio of lactic acid and / or a salt thereof and caffeine is 0.9: 1 to 1000 as a weight ratio (however, in the weight of lactate, a value converted to the weight as lactic acid is used).
The agent according to claim 2, wherein the ratio is 1. A composition for reducing body fat, comprising lactic acid and / or a salt thereof as an active ingredient (excluding those containing lactic acid bacteria) .   The composition according to claim 4, further comprising caffeine. The content ratio of lactic acid and / or a salt thereof and caffeine is 0.9: 1 to 1000 as a weight ratio (however, in the weight of lactate, a value converted to the weight as lactic acid is used).
6. The composition of claim 5, wherein: 1.   The composition according to any one of claims 4 to 6, which is a medicine.   The composition according to any one of claims 4 to 6, which is a food or drink.