JP2019189544A - Composition containing turmeronol a and/or turmeronol b - Google Patents

Abstract

To provide compositions that contain compounds derived from food materials with abundant food experience and high safety, and have anti-inflammatory action or blood CRP value lowering action.SOLUTION: The present invention relates to an orally ingested composition, an anti-inflammatory composition, or a blood CRP value-reducing composition, containing at least one of turmeronol A and turmeronol B in a total amount of 100 μg or more per one intake. The present invention also relates to an orally ingested composition, an anti-inflammatory composition, or a reduced blood CRP value-reducing composition, containing 80 μg or more of turmeronol A and/or 20 μg or more of turmeronol B, per one intake.SELECTED DRAWING: Figure 5

Description

The present invention relates to compositions that are taken orally.
The invention also relates to an anti-inflammatory composition.
The present invention also relates to a composition for lowering blood CRP levels.

  Prostaglandin E2 (PGE2) is produced by leukocytes (macrophages), mast cells, endothelial cells and platelets. Arachidonic acid present as a component of cell membrane phospholipid is cleaved by phospholipase, and PGE2 is synthesized through a cyclooxygenase pathway. The pathway is activated in the process of inflammation, increasing the production of PGE2.

  PGE2 released from specific cells acts on nearby target cells and induces an inflammatory response in the target cells. PGE2 is one of chemical mediators for amplifying an inflammatory response at an inflammatory site, and activates the inflammatory response at the inflammatory site.

  Nitric oxide (NO) is produced by type II nitric oxide synthase (iNOS) of leukocytes (macrophages) induced by inflammatory cytokines and bacterial endotoxins in the course of inflammation (Non-patent Document 1). Since excessively produced NO is converted into peroxynitrite and then shows cytotoxic effects such as DNA damage and LDL oxidation (Non-patent Document 2), excessive NO produced by inflammation can be suppressed. is important. Moreover, since NO activates intracellular signal pathways that promote inflammation such as the NF-κB pathway (Non-patent Document 3), suppressing NO production is also important for exerting anti-inflammatory effects ( Patent Document 1).

  Inflammation is a protective reaction that is caused by stimulating factors such as infections, trauma, and foreign substances, and tries to eliminate self cells and tissues necrotized by the stimulating factor together with the stimulating factor itself. The inflammatory response helps remove harmful stimuli, including infections. On the other hand, since inflammation can also damage normal tissues, it may cause damage to the living body, and it is necessary to suppress an excessive inflammatory reaction.

  Examples of the PGE2 production inhibitor and anti-inflammatory agent containing a natural compound as an active ingredient are those described in Patent Document 2. Further, in Patent Document 1, a mixture of soybean seeds or an extract thereof and chlorophyll activated by light irradiation treatment and / or heat treatment has an activity of suppressing NO production and is useful as an anti-inflammatory agent. It is described that there is.

  On the other hand, turmeric (Curcuma longa) contains a large number of sesquiterpene compounds, and as a turmeric-derived sesquiterpene compound, many bisaborane compounds such as tureronol A (Turmeronol A) and turmeronol B (Turmeronol B) are known. (Non-Patent Document 4).

  Patent Document 3 describes that turmeric rhizomes themselves, polysaccharides in turmeric, and essential oils have anti-inflammatory effects. Patent Document 3 further discloses that the active ingredient of turmeric can be divided into an essential oil fraction, a curcuminoid fraction, a turmerin fraction, and a polysaccharide fraction. In the essential oil fraction, turmeronol A (turmeronol A) and turmeronol B are used together with turmer. It is described that (turmeronol B) is contained, and the essential oil fraction of turmeric rhizome can be extracted by a supercritical carbon dioxide extraction technique.

International Publication WO2012 / 177969 JP 2012-056852 A Special table 2009-530305 gazette

Robins Pathology (8th Edition) Chapter 2 p. 58-59 J Physiol Pharmacol. 2003; 54 (4): 469-87. Curr Drug Targets Inflamm Allergy. 2005; 4 (4): 471-9. S. Li et al. , Pharmaceutical Crops, 2011, 2, 28-54.

  Although it has been conventionally known that turmeric contains tureronol A and tureronol B as described in Non-Patent Document 4 and Patent Document 3, the effect of turmonol A and turmonol B itself has not been clear. In Patent Document 3, quantification of turmeronol A and tureronol B in the turmeric extract is not performed.

  An object of this invention is to provide the composition which has the anti-inflammatory effect or the blood CRP value lowering effect including the compound derived from the food material with rich food experience and high safety | security.

The present inventors have a composition containing at least one of turmeronol A and turmeronol B in a total amount of 100 μg or more and a composition containing 80 μg or more of turmonol A and / or 20 μg or more of turmeronol B per one intake. The product has been found to have an anti-inflammatory action or a blood CRP value lowering action, and has led to the completion of the present invention described below.
(1) A composition that is orally ingested and contains at least one of turmeronol A and turmeronol B in a total amount of 100 μg or more per one intake.
(2) A composition that is orally ingested and contains 80 μg or more of turmeronol A and / or 20 μg or more of turmeronol B per intake.
(3) The composition according to (1) or (2), wherein the turmonol A and the turmonol B are derived from a turmeric extract.
(4) The composition according to any one of (1) to (3), wherein the curcumin content per intake is less than 30 mg.
(5) An anti-inflammatory composition comprising at least one of tureronol A and turmeronol B in a total amount of 100 μg or more per one intake.
(6) A composition for lowering CRP levels in blood, comprising at least one of turmeronol A and turmeronol B in a total amount of 100 μg or more per one intake.
(7) An anti-inflammatory composition comprising 80 μg or more of turmeronol A and / or 20 μg or more of turmeronol B per intake.
(8) A composition for lowering the CRP level in blood, comprising 80 μg or more of turmeronol A and / or 20 μg or more of turmeronol B per intake.

  ADVANTAGE OF THE INVENTION According to this invention, the composition which contains the compound derived from the food material with abundant food experience and high safety | security, and has an anti-inflammatory effect or a blood CRP value reduction effect | action is provided.

FIG. 1 shows the PGE2 concentration in the culture supernatant of RAW264.7 treated with turmeronol A. FIG. 2 shows the concentration of PGE2 in the culture supernatant of RAW 264.7 treated with tureronol B. FIG. 3 shows the NO ₂ ⁻ concentration in the culture supernatant of RAW264.7 treated with turmeronol A. FIG. 4 shows the NO ₂ ⁻ concentration in the culture supernatant of RAW 264.7 treated with tureronol B. FIG. 5 shows a group of subjects who took a tablet containing turmeric extract containing tureronol A and turmeronol B every day for 12 weeks and a group of subjects who took a placebo tablet every day for 12 weeks before the start of the study, 4 weeks and 8 weeks later. The average value of the CRP value in the blood after 12 weeks is shown.

<Active ingredient>
Tameronol A and Tameronol B are compounds having the following planar structures, respectively.

  In the natural product separated from the turmeric extract, tureronol A and tureronol B are known to have the S configuration in the 6-position carbon in the partial structure of 2-methyl-2-hepten-4-one. is there. However, in the present invention, tereronol A and tereronol B only have to have the above-described planar structure, and the configuration may be S-form, R-form, S-form and R-form. And a mixture thereof.

  In the present invention, turmeronol A and / or turmeronol B is preferably turmonol A and / or turmonol B derived from a turmeric extract. Here, the turmonol A and / or turmonol B derived from the turmeric extract may be turmonol A and / or turmonol B separated from the turmeric extract, or turmonol A existing as a component in the turmeric extract. And / or tureronol B.

  Here, the turmeric extract refers to an extract (turmeric extract) of a plant raw material derived from a plant belonging to the genus Turmeric belonging to the ginger family. The turmeric extract is not limited to the solvent extract obtained by extraction with an extraction solvent, but also includes those obtained by further fractionating and purifying the solvent extract by column chromatography or the like. The turmeric extract used in the present invention is obtained from an extract obtained by completing the extraction operation (including fraction purification in the case of fraction purification), a concentrate obtained by partially removing the solvent from the extract, or an extract. It can be in the form of a dry product from which the solvent has been removed. The removal of the solvent from the extract can be performed by volatilizing the solvent by heating and / or reduced pressure. These heating and decompression methods are not particularly limited, and for example, conventionally known methods can be used.

  Examples of plant raw materials include Curcuma longa (turmeric), Curcuma aromatica, Curcuma zedoaria, Curcuma phaeocaulis, Curcuma kwansiens, Curcumin, and Curcuma urgen. Curcuma longa rhizome and the like are suitable. As the rhizome, one collected from soil may be used, and an appropriate portion of the rhizome may be used as it is, cut into an appropriate size or shape, or pulverized. These plant materials may be appropriately dried.

  Examples of the extraction solvent include at least one selected from the group consisting of water and a hydrophilic organic solvent, a liquid solvent such as hexane, water vapor, and a supercritical fluid.

  The at least one extraction solvent selected from the group consisting of water and a hydrophilic organic solvent may be any of water, a hydrophilic organic solvent, and a mixed solvent of water and a hydrophilic organic solvent. The hydrophilic organic solvent may be a mixed solvent of plural kinds of hydrophilic organic solvents. “Water” includes hot water. As hot water, for example, hot water of 95 ° C. or higher can be used. Examples of the hydrophilic organic solvent include at least one alcohol (may be a mixed solvent of a plurality of alcohols), and the alcohol is not particularly limited, but ethanol is preferable. The mixing ratio in the case of using a mixed solvent of alcohol and water as the extraction solvent is not particularly limited. For example, the weight ratio is preferably in the range of 10:90 to 90:10, more preferably in the range of 20:80 to 50:50. .

Extraction using steam is also called steam distillation.
Supercritical carbon dioxide is preferred as the supercritical fluid.
From the viewpoint of efficiently extracting tureronol A and tureronol B from turmeric, it is preferable to use ethanol, hexane or supercritical fluid as the extraction solvent.

Curcumin contained in turmeric is a kind of curcuminoid. The international organization JECFA (FAO / WHO Joint Expert Committee on Food Additives) sets the ADI (permissible daily intake) of curcuminoids to 3 mg / kg body weight / day (eg, 150 mg per day for a person with a body weight of 50 kg). Therefore, when using turmeronol A and / or turmonol B in the form of a turmeric extract, it is preferable to use a turmeric extract containing turmonol A and / or turmonol B and having a low curcuminoid concentration. In order to obtain such a turmeric extract, it is preferable to use water (particularly hot water), hexane, water vapor or a supercritical fluid as an extraction solvent.
The method for preparing the turmeric extract using the extraction solvent is not particularly limited.

  Turmeronol A and / or Turmeronol B may be used in the form of a plant material containing it. Examples of the plant raw material containing turmonol A and / or turmonol B include the raw materials of the ginger family turmeric genus described above. On the other hand, the rhizomes of the ginger family turmeric genus plants contain relatively much iron together with turmonol A and / or turmonol B. Ingestion of large amounts of iron may adversely affect people with certain symptoms such as hepatitis C patients and NASH (non-alcoholic steatohepatitis), so the recommended upper limit of iron intake is 1 6 mg per day. For this reason, it is preferable that turmeronol A and / or turmeronol B are forms other than the rhizome form of the ginger family turmeric genus plant.

<Content of active ingredient>
In the first aspect, the composition of the present invention contains at least one of turmeronol A and turmeronol B in a total amount of 100 μg or more per one intake. In the case where the composition according to the first aspect includes only one of turmonol A and turmonol B, it is sufficient that the content of one of them is 100 μg or more per one intake, both turmonol A and turmonol B When the total content of both is included, it may be 100 μg or more per one intake. The composition according to the first aspect has an action of suppressing inflammation, particularly chronic inflammation, and an action of reducing CRP (c-reactive protein) level in blood when ingested by animals such as humans. Played. More preferably, the composition according to the first aspect contains a total of 100 μg or more of turmeronol A and turmeronol B per intake, and more preferably 80 μg or more of turmeronol per intake. A and / or 20 μg or more of turmeronol B, most preferably 80 μg or more of turmeronol A and 20 μg or more of turmeronol B per serving.

  In the second embodiment, the composition of the present invention contains 80 μg or more of turmeronol A and / or 20 μg or more of turmeronol B per one intake. The composition according to the second aspect has an action of suppressing inflammation, particularly chronic inflammation, and an action of lowering CRP (c-reactive protein) level in blood when ingested by animals such as humans. Played. More preferably, the composition according to the second aspect contains 80 μg or more of turmeronol A and 20 μg or more of turmeronol B per serving.

  A method for quantifying turmeronol A and turmeronol B is not particularly limited, and for example, it can be carried out by LC / MS analysis shown in Examples.

  In the composition according to the first aspect or the second aspect of the present invention, the tereronol A and / or the turmeronol B is added to the tereronol A and / or tereronol B at the time of completion of production, that is, at the stage of shipment of the production factory as a finished product. It only has to be included in the range.

  More preferably, the composition according to the first aspect or the second aspect of the present invention has a curcumin content of less than 30 mg per intake. Compositions with a curcumin content of less than 30 mg per dose will reduce inflammation and blood CRP without exceeding the curcuminoid ADI (permissible daily intake) (150 mg for a 50 kg person). Since it is easy to ingest an amount of turmeronol A and / or turmeronol B effective for lowering the value, it is preferable.

  In the present invention, “a single intake” means an amount at which the composition of the present invention is ingested at a time, or continuously over a short time interval (for example, 10 minutes or less, preferably 5 minutes or less). This means the total amount taken multiple times. When the composition of the present invention is in the form of a liquid or fluid composition, for example, 0.1 ml to 500 ml (typically 50 ml, 100 ml, 150 ml, 200 ml, 250 ml, 300 ml, 350 ml, 400 ml, 450 ml or 500 ml) ) Is the amount, and in the case of a composition in another shape such as gel, semi-solid or solid, for example, 0.1 g to 500 g (typically 50 g, 100 g, 150 g, 200 g, 250 g, 300g, 350g, 400g, 450g or 500g) is the amount. In the following, “one intake” is used in this sense.

<Compositions taken orally>
In a preferred embodiment, the composition according to the first aspect or the second aspect of the present invention is a composition to be taken orally.

  The orally ingested composition of the present invention exhibits favorable effects such as suppression of inflammation and reduction of blood CRP value when animals such as humans are orally ingested.

  The composition to be orally ingested according to the present invention may be a composition in various forms such as pharmaceuticals, foods and drinks, feeds, food additives, feed additives, etc. It is more preferable. The foods and drinks include foods in the form of functional display foods, foods for specified health use, supplements for nutritional supplements, and the like.

  The orally ingested composition of the present invention may be continuously ingested or may be ingested when necessary.

  The specific form of the composition taken orally of the present invention will be described later.

<Anti-inflammatory composition>
In another preferable embodiment, the composition according to the first aspect or the second aspect of the present invention is an anti-inflammatory composition.

  The anti-inflammatory composition of the present invention is useful for the prevention or treatment of inflammation, particularly chronic inflammation, in animals such as humans.

  The anti-inflammatory composition of the present invention may be a composition of various forms such as pharmaceuticals, foods and drinks, feeds, food additives, feed additives, etc., and may be pharmaceuticals or foods and drinks taken by humans. More preferred. The foods and drinks include foods in the form of functional display foods, foods for specified health use, supplements for nutritional supplements, and the like. The anti-inflammatory composition of the present invention is preferably in the form of a composition taken orally or nasally, and more preferably in the form of a composition taken orally.

  The anti-inflammatory composition of the present invention may be taken continuously or taken when necessary.

  Specific forms of the anti-inflammatory composition of the present invention will be described later.

<Composition for lowering CRP level in blood>
In still another preferred embodiment, the composition according to the first aspect or the second aspect of the present invention is a composition for lowering the blood CRP value.

  The composition for lowering the blood CRP level of the present invention has an action of lowering the blood CRP (c-reactive protein) level, which is an indicator of inflammation, particularly chronic inflammation, in animals such as humans.

  The composition for lowering the CRP value in blood of the present invention may be a composition of each form such as a pharmaceutical, food and drink, feed, food additive, feed additive, etc. More preferably. The foods and drinks include foods in the form of functional display foods, foods for specified health use, supplements for nutritional supplements, and the like. The composition for lowering the blood CRP value of the present invention is preferably in the form of a composition taken orally or nasally, more preferably in the form of a composition taken orally.

  The composition for lowering the blood CRP value of the present invention may be taken continuously or taken as needed.

  The specific form of the composition for lowering blood CRP value of the present invention will be described later.

<Form of the composition of the present invention>
The orally ingested composition, anti-inflammatory composition, or blood CRP value-reducing composition of the present invention (hereinafter referred to as “the composition of the present invention”) is an active ingredient (termeronol A and / or turmeronol). B, or a turmeric extract or a raw material of a plant raw material) itself, or a composition containing the active ingredient and at least one other ingredient. When the composition of the present invention contains the active ingredient and at least one other component, the composition may be a mixture of the active ingredient and at least one other component, A composition in which the active ingredient and at least one other ingredient are formulated by an appropriate means may be used, or a formulation in which the active ingredient and at least one other ingredient are formulated. Further, it may be a composition mixed with other components.

  The shape of the composition of the present invention is not particularly limited, and may be any shape such as liquid, fluid, gel, semi-solid, or solid.

  The at least one other component that can be contained in the composition of the present invention is not particularly limited, but is preferably acceptable in a final form such as pharmaceuticals, foods and drinks, feeds, food additives, feed additives, and the like. Examples of such components that can be taken orally can be exemplified.

  Examples of such other components include sweeteners, acidulants, vitamins, minerals, thickeners, emulsifiers, antioxidants, and water. Moreover, you may add a pigment | dye, a fragrance | flavor, a preservative, an antiseptic | preservative, a fungicide, a further physiologically active substance, etc. as needed.

  Sweeteners include monosaccharides and disaccharides such as glucose, fructose, sucrose, lactose, maltose, palatinose, trehalose, and xylose, isomerized sugar (glucose fructose liquid sugar, fructose glucose liquid sugar, sugar mixed isomerized sugar, etc.) Sugar alcohols (erythritol, xylitol, lactitol, palatinit, sorbitol, reduced starch syrup, etc.), honey, high intensity sweeteners (sucralose, acesulfame potassium, thaumatin, stevia, aspartame, etc.).

  Examples of the acidulant include citric acid, malic acid, gluconic acid, tartaric acid, lactic acid, phosphoric acid, and salts thereof, and one or more of these can be used.

  Examples of vitamins include vitamin A, vitamin B1, vitamin B2, vitamin B6, vitamin E, niacin, inositol and the like.

  Examples of minerals include calcium, magnesium, zinc, iron and the like.

  Examples of the thickener include carrageenan, gellan gum, xanthan gum, gum arabic, tamarind gum, guar gum, locust bean gum, karaya gum, agar, gelatin, pectin, soybean polysaccharide, carboxymethyl cellulose (CMC) and the like.

  Examples of the emulsifier include glycerin fatty acid ester, sucrose fatty acid ester, sorbitan fatty acid ester, lecithin, vegetable sterol, saponin and the like.

  Examples of the antioxidant include vitamin C, tocopherol (vitamin E), enzyme-treated rutin, catechin and the like.

  Each of the other components can be appropriately blended in an amount within the range usually employed by those skilled in the art for compositions such as foods and drinks and pharmaceuticals.

  Composition forms in which the active ingredient and at least one other ingredient are formulated by appropriate means are powders, granules, capsules, tablets (coated tablets such as sugar-coated tablets or multilayer tablets, mouth disintegrants, chewables) It may be in the form of a solid composition such as a tablet or the like, or it may be in the form of a liquid composition such as a solution.

<Experiment 1: Anti-inflammatory action of tureronol A and tureronol B>
1. Preparation Method Hot water extraction was performed from turmeric rhizomes to obtain a hot water extract. Next, 90% methanol (methanol / water = 90/10 (v / v)) was extracted from the hot water extract to obtain a 90% methanol extract. Next, the 90% methanol extract was subjected to ethyl acetate / water liquid-liquid partition to obtain an ethyl acetate fraction. Turmeronol A was used in the test after the ethyl acetate fraction was purified by reverse phase column chromatography and then dissolved in dimethyl sulfoxide.

The structure of isolated turomerol A is based on the results of instrumental analysis such as ¹ H NMR, ¹³ C NMR, LCMS, and known information (Agric. Biol. Chem., 1990; 54 (9): 2367-71). Identified.

  Turmeronol B was purchased from Nagara Science Co., Ltd., dissolved in dimethyl sulfoxide, and used for the test.

2. Evaluation of anti-inflammatory effect The mouse macrophage cell line RAW264.7 was used for the experiment, seeded in a 96-well plate with DMEM (10% FBS) medium to a number of 1.5 × 10 ⁵ cells, and a CO ₂ incubator for 24 hours. Incubated until confluent. The mouse macrophage cell line RAW264.7 cultured in a 96-well plate was selected from predetermined concentrations (1.7 μg / mL, 3.2 μg / mL, 6.3 μg / mL, 12.5 μg / mL, and 25 μg / mL). (2) at 20 mg / mL lipopolysaccharide (LPS, inflammation-inducing factor), and cultured for 12 hours. Thereafter, the supernatant was recovered, and the amount of prostaglandin E2 (PGE2) released into the supernatant was measured by a competitive ELISA method. Further, the NO ₂ ⁻ amount released into the supernatant (NO oxide, reflecting the NO amount) was measured by the Griess method. In addition, in the process by each component, DMEM which does not contain 10% FBS was used. Control / LPS (+) is the test group in which the same operation is performed except that the cells are not treated with tureronol A or tureronol B. The test section where the test was performed was defined as control / LPS (−).

3. Results The PGE2 concentration in the culture supernatant of RAW264.7 treated with tureronol A is shown in FIG.

  The PGE2 concentration in the culture supernatant of RAW264.7 treated with turmeronol B is shown in FIG.

The NO ₂ ⁻ concentration in the culture supernatant of RAW264.7 treated with turmeronol A is shown in FIG.

The NO ₂ ⁻ concentration in the culture supernatant of RAW264.7 treated with turmeronol B is shown in FIG.

  1-4, “+” indicates that 20 ng / mL LPS was added to the medium during the 12-hour culture, and “−” indicates that LPS was not added.

  The results shown in FIGS. 1 to 4 support that turmeronol A and tureronol B have PEG2 production inhibitory activity and NO production inhibitory activity.

<Experiment 2: Anti-inflammatory action in human of turmeric extract containing tureronol A and tureronol B>
1. Turmeric extract The turmeric extract was prepared by hot water extraction of the curcuma longa rhizome part, vacuum concentration and spray drying to remove moisture.

2. Test food Tablets ingested by subjects in the turmeric extract intake group were prepared using the above-mentioned turmeric extract, maltose, fine silicon dioxide, sucrose fatty acid ester, and brightener. The amount of turmeronol A and turmeronol B in this tablet was measured using LC / MS according to the procedure described later. Similarly, the amount of curcumin in the tablet was measured using HPLC according to the procedure described later. As a result, it was confirmed that the single dose (3 tablets) per subject of this tablet contained 86.5 μg of tureronol A, 24.7 μg of turmeronol B, and 471 μg of curcumin.

  Tablets ingested by subjects in the placebo intake group were prepared using maltose, pigment, fine silicon dioxide, sucrose fatty acid ester, and brightener.

使用カラム：ＵＮＩＳＯＮ ＵＫ−Ｃ１８（２５０ｍｍ×４．６ｍｍ、３μｍ）
カラム温度：３０℃ 3. Analysis of tureronol A and tureronol B After pulverizing and weighing the tablets ingested by the subjects of the above-mentioned turmeric extract ingestion group, adding water and ethyl acetate, and passing the supernatant obtained by centrifugation through an activated carbon column Concentrated with nitrogen and dissolved in acetonitrile. The obtained liquid was subjected to LC / MS analysis as a measurement sample. LC / MS analysis was performed under the following conditions.
Analyzer: Thermo Fisher Scientific Orbitrap LCMS (Orbitrap Velos Pro)
Flow rate: 0.5 mL / min Mobile phase: Acetonitrile, 0.1% formic acid aqueous solution Feed gradient:

Column used: UNISON UK-C18 (250 mm × 4.6 mm, 3 μm)
Column temperature: 30 ° C

4). Curcumin analysis The tablets ingested by the subjects of the above-mentioned turmeric extract intake group were crushed and weighed, added with an aqueous methanol solution, centrifuged after shaking and stirring, and then subjected to HPLC analysis as a measurement sample. . HPLC analysis was performed under the following conditions.
Analyzer: Hitachi High-Technologies Corporation Chromamaster 5000 HPLC
Flow rate: 1 mL / min Mobile phase: Acetonitrile: Trifluoroacetic acid aqueous solution (pH 3.3) = 45%: 55%
Column used: L-Column ODS (250 mm × 4.6 mm, 5 μm)
Column temperature: 40 ° C

5. Subjects Each of the turmeric extract intake group and the placebo intake group consists of 45 subjects who satisfy the following conditions.
Men and women aged 50 to 69 years BMI is normal high to obesity 1 degree (BMI: 23 to less than 30), or blood pressure is normal blood pressure to I degree hypertension (systolic blood pressure: 120 mmHg to 160 mmHg, or Diastolic blood pressure: 80mmHg or more and less than 100mmHg)
A certain number was selected.

6). Placebo-controlled double-blind parallel group comparison study 45 subjects in the turmeric extract intake group orally ingested 3 tablets containing the turmeric extract daily for 12 weeks before dinner. In the turmeric extract intake group, 2 subjects during the 12-week study became dropouts or exclusion criteria subjects and 43 completed the study.

  Forty-five subjects in the placebo intake group took the three tablets containing no turmeric extract every day for 12 weeks before dinner. In the placebo ingestion group, one subject was a dropout or exclusion criteria subject during the 12-week study, and 44 subjects completed the study.

  Before the start of the test, 4 weeks, 8 weeks, and 12 weeks later, the blood CRP (c-reactive protein) value of each subject was measured to obtain an average value. The blood CRP value was measured by the nephelometry method and the latex agglutination turbidimetry. The measurement by the nephelometry method was performed according to Siemens Healthcare Diagnostics N-latex CRP II kit. The measurement by latex agglutination turbidimetry was performed according to the Iatro CRP-EX kit of LSI Medience.

  The results are shown in FIG. In the turmeric extract ingestion group, the CRP level in blood significantly decreased compared to the placebo group 8 and 12 weeks after the start of ingestion of the turmeric extract-containing tablet. Since the blood CRP value is an index of inflammation, it was confirmed that the turmeric extract containing tureronol A and tureronol B has an anti-inflammatory effect.

  The present invention is useful in the field of food and drink or pharmaceutical products.

Claims (8)

  An orally ingested composition comprising at least one of turmeronol A and tureronol B in a total amount of 100 μg or more per ingestion.   An orally ingested composition comprising 80 μg or more of turmeronol A and / or 20 μg or more of turmeronol B per intake.   The composition according to claim 1 or 2, wherein the turmonol A and the turmonol B are derived from a turmeric extract.   The composition according to any one of claims 1 to 3, wherein the content of curcumin per intake is less than 30 mg.   An anti-inflammatory composition containing at least one of turmeronol A and turmeronol B in a total amount of 100 μg or more per one intake.   A composition for reducing CRP levels in blood, comprising at least one of turmeronol A and turmeronol B in a total amount of 100 μg or more per one intake.   An anti-inflammatory composition comprising 80 μg or more of tureronol A and / or 20 μg or more of turmeronol B per intake.   A composition for lowering the CRP level in blood, comprising 80 μg or more of tureronol A and / or 20 μg or more of turmeronol B per intake.

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