GB2535177A - Composition and use of lactobacillus reuteri GMNL-263 in decreasing blood lipid levels - Google Patents

Composition and use of lactobacillus reuteri GMNL-263 in decreasing blood lipid levels Download PDF

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GB2535177A
GB2535177A GB1502240.3A GB201502240A GB2535177A GB 2535177 A GB2535177 A GB 2535177A GB 201502240 A GB201502240 A GB 201502240A GB 2535177 A GB2535177 A GB 2535177A
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lactobacillus reuteri
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Chen Yi-Hsing
Chen Ya-Hui
Lou Tzu-Chi
Shen Ting-Yun
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Genmont Biotech Inc
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    • A61P3/06Antihyperlipidemics
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K35/00Medicinal preparations containing materials or reaction products thereof with undetermined constitution
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    • A61K2035/115Probiotics

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Abstract

A use of a Lactobacillus reuteri GMNL-263 in decreasing blood lipid levels is disclosed. The bacteria are administered as a composition, which is shown to reduce cholesterol and triglyceride levels in animals suffering from hyperlipidemia, the mechanism of which may be as a result of specific inhibition of gene expression related to pro-inflammatory factor and lipid synthesis, and promotion of gene expression related to cholesterol metabolism. The composition is preferably administered orally, and comprises heat-inactivated bacteria.

Description

COMPOSITION AND USE OF LACTOBACILLUS REUTERI GMNL-263 IN DECREASING BLOOD LIPID LEVELS
BACKGROUND OF THE INVENTION
Field of the Invention
The present invention relates a composition and use of Lactobacillus reuteri GMNL-263 in decreasing blood lipid levels. More particularly, a composition comprising Lactobacillus reuteri could 1() inhibit the gene expression of tumor necrosis factor alpha (TNF-a), fatty acid synthase (FAS), and sterol regulatory element binding protein-lc (SREBP-I c) and promote the gene expression of LDL receptor and cholesterol 7a-hydroxylase (CYP7A I), achieving the aim of decrease of blood lipid levels.
Description of Related Art
Because of the more and more exquisite food and the increase of the chance of eating at the restaurant, it causes that human intake too much calorie and lipids to accumulate in the body, easily arising hyperlipidemia. According to the research reports, hyperlipidemia easily leads to fatty liver disease and atherosclerosis and is also a key risk factor to cause hypertension, heart disease, stroke, diabetes, arteriosclerosis, kidney disease etc. Therefore, people became deeply concerned that how to keep blood lipid levels normal to reduce the chance of suffering from cardiovascular disease.
At present, the way that natural extracts is the major material to produce composition for reducing blood lipid levels is more and more s popular with consumers. For example, the Taiwan Patent application with the Issue No. 1387460, "EXTRACTION METHODS AND COMPOSITIONS TO AMELIORATE HYPERLIPIDEMIA, HYPERGLYCERMIA AND FATTY LIVER", disclosed that extraction methods and compositions of bitter gourd, licorice, soybean protein, and chlorella could exert the highest activation ability of PPAR and further demonstrated the efficacy in animal models and human models to ameliorate hyperlipidemia, hyperglycermia and fatty liver; the Taiwan Patent application with the Issue No. 1441643, "COMPOSITION FOR ADJUSTING BLOOD LIPID AND CARDIOVASCULAR is PROTECTION", disclosed a composition for adjusting blood lipids and cardiovascular protection, comprising rhodiola compound powder, Red Yeast Rice, phytosterols, natto and vitamin B complex, wherein the predetermined ratio of the rhodiola compound powder to the Red Yeast Rice and the phytosterols to natto and vitamin B complex represents 54-79 to 14-39 to 7-32 wt%, and the rhodiola compound powder comprises roselle, rhodiola, salvia miltiorrhiza, folium mori, cassia, lotus leaf, hawthorn, chlorella and the composition thereof; the Taiwan Patent application with the Issue No. 1440465, "HERBAL EXTRACT MIXTURE FOR REDUCING BLOOD LIPID AND A COMBINATION THEREOF", disclosed an herbal extract mixture for reducing blood lipid, comprising 33.4% to 77.7% of Eucheuma okamurai Yamada extract, 11.14% to 33.3% of Acanthopanax senticosus extract, and 11.14% to 33.3% of Dioscorea alata extract, and disclosed a combination for reducing blood lipid, including a herbal extract mixture mentioned above and at least a medically acceptable adjuvant or carrier. However, the natural extracts easily have the problem of unknown ingredients or the remains of organic solvents.
Probiotics are microorganisms for beneficial to improve gastrointestinal (GI) tract health of the host (like human or other animals), which are mainly divided into bacteria and yeast. Bacteria are further divided into Lactobacilli and Bifidobacterium. At present, some research have reported that probiotics not only modulates immune is system and keeps gastrointestinal tract health, but also contributes to cancer prevention. Moreover, please refer to the Taiwan Patent application with the Issue No. 1355939, "COMPOSITION AND USE OF PROBIOTIC STRAIN GM-263 (ADR-1) IN TREATING RENAL FIBROSIS IN DIABETES", disclosed a use of probiotic strain GM-263 (ADR-1) in treating renal fibrosis in diabetes, utilizing the probiotic strain such as Lactobacillus reuteri strain GM-263 (ADR-1) (accession No. CCTCC M 209263) to produce a composition for treating renal fibrosis in diabetes in an effective dose, thereby reducing the concentration of glycated hemoglobin and blood sugar and keeping body weight and kidney weight within normal range, as well as specifically inhibiting phosphorylation of JAK2/STATI signal transduction pathway and renal fibrosis-related protein expression. It showed that probiotics s have beneficial effect of blood sugar regulation and kidney function improvement.
However, according to the above research, probiotics application in reducing blood lipid and the relative mechanism is very few. Therefore, if probiotics could be researched to find beneficial effects for io reducing blood lipid and could be produced to medical composition or food material for consumers, it is beneficial to consumers' health.
SUMMARY OF THE INVENTION
Therefore, the object of the present invention is to provide a is Lactobacillus reuteri GMNL-263 utilizing to produce a composition for decreasing blood lipid levels. Lactobacillus reuteri GMNL-263 (GMNL-263) inhibits the gene expression related to pro-inflammatory factor and lipid synthesis and promotes the gene expression related to cholesterol metabolism to decrease blood lipid levels, achieving the aim of hyperlipidemia treatment.
For the above object, a probiotics composition for decreasing blood lipid levels comprises a therapeutically effective amount of Lactobacillus reuteri GMNL-263 (accession No.: CCTCC M 209263).
Lactobacillus reuteri GMNL-263 specifically inhibits gene expression related to pro-inflammatory factor and lipid synthesis and promotes gene expression related to cholesterol metabolism, achieving the aim of decrease of blood lipid levels.
According to an embodiment of the present invention, the gene related to lipid synthesis is fatty acid synthase (FAS) gene and sterol regulatory element binding protein-lc (SREBP-1c) gene. The gene related to cholesterol metabolism is Low-density Lipid receptor (LDLR) gene and cholesterol 7a-hydroxylase (CYP7A1) gene. The pro-inflammatory factor is tumor necrosis factor alpha (TNF-a).
According to an embodiment of the present invention, the probiotics composition is a medical composition, a food additive, a food or its ingredient, and Lactobacillus reuteri GMNL-263 is heat-inactivated. The medical composition comprises a pharmaceutically acceptable vehicle and is oral administration.
According to an embodiment of the present invention, the blood lipid levels comprises a serum total cholesterol level, a serum low-density lipoprotein level, a serum malondiaidehyde level, a liver total cholesterol level, and a liver malondiaidehyde level. Furthermore, the Lactobacillus reuteri GMNL-263 modulates the intestinal microbiota. Therefore, the composition comprising Lactobacillus reuteri could efficiently regulating blood lipid levels to return to normal range for achieving the aim of hyperlipidemia treatment.
A method for decreasing blood lipid levels is also provided, comprising the step of administrating a therapeutically effective amount of Lactobacillus reuteri GMNL-263 (accession No.: CCTCC M 209263) to specifically inhibit gene expression related to pro-inflammatory factor and lipid synthesis and to promote gene expression related to cholesterol metabolism.
BRIEF DESCRIPTION OF THE DRAWINGS
Fig. 1 shows abdominal anatomical photographs of each group of to experimental mice according to an embodiment of the present invention; Fig. 2 shows a bar diagram of the relative expression of several mRNA in liver tissue of each group of Fig. I; Fig. 3 shows a bar diagram of the relative expression of several mRNA in adipose tissue of each group of Fig.1; and Fig. 4 shows a bar diagram of the relative expression of intestinal microhiota of each group of Fig. I. DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENT A probiotics composition for decreasing blood lipid levels is 20 disclosed, comprising a therapeutically effective amount of Lactobacillus reuteri GMNL-263 (GMNL-263) (accession No.: CCTCC M 209263). Lactobacillus reuteri GMNL-263 specifically inhibits gene expression related to pro-inflammatory factor and lipid synthesis and promotes gene expression related to cholesterol metabolism, achieving the aim of decrease of blood lipid levels. The gene related to lipid synthesis is fatty acid synthase (FAS) gene and sterol regulatory element binding protein-1c (SREBP-1c) gene. The gene related to cholesterol metabolism is Low-density Lipid receptor (LDLR) gene and cholesterol 7a-hydroxylase (CYP7A I) gene. The pro-inflammatory factor is tumor necrosis factor alpha (TNF-a). Therefore, the composition comprising Lactobacillus reuteri is suitable for producing a medical composition, a food additive, a food or its ingredient for hyperlipidemia treatment, achieving the aim of decrease of blood lipid levels.
The probiotics composition of the present invention includes, but not be limited to, food, beverage, health food, additive for use in animal feed and drinking water, medical composition for human use and animal use, food additive, and beverage additive.
The term "pharmaceutically acceptable" means that a substance or a composition should be compatible with other ingredients and harmless to patient. The pharmaceutically acceptable vehicle is selected from the group consisting of a solvent, an emulsifier, a suspending agent, a decomposer, a binding agent, an excipent, a stabilizing agent, a chelating agent, a diluent, a gelling agent, a preservative, a lubricant, and a surfactant.
The foregoing Lactobacillus reuteri isolated strain and a pharmaceutically acceptable vehicle could be made into a formulation suitable for the probiotics composition of the present invention, according to the technique that those skilled in the art known. The formulation includes, but not be limited to, a solution, an emulsion, a suspension, a powder, a tablet, a pill, a lozenge, a troche, a chewing gum, and a capsule.
The "probiotics" described herein refers to Lactobacillus reuteri GMNL-263. Lactobacillus reuteri GMNL-263 has been deposited with the China Center for Type Culture Collection (CCTCC), Wuhan University, Wuhan 430072, People's Republic of China under accession number of CCTCC M 209263.
The foregoing probiotics GMNL-263 is obtained by the prior methods and isolated from the gastrointestinal tract of health human volunteers, for example, followed by a microbiological examination, such as 16S rDNA sequence analysis and any commercially available is product. The isolated probiotics is identified as Lactobacillus reuteri GMNL-263 by the prior method, so the detail identification method is not described here. The effects of the heat-inactivated Lactobacillus reuteri GMNL-263 on blood lipid regulation are mainly evaluated as following.
Preparation of the heat-inactivated GMNL-263 Lactobacillus reuteri GMNL-263 is stored in Genmont Biotech Incorporation, Taiwan. A standard strain of Lactobacillus reuteri GMNL-263 stored in a cryogenic vial was cultured in MRS broth at 37± 1 for 18-36 hours. Then, the fermentation broth was concentrated, and the probiotics of the fermentation broth was made inactive by a heating process under high temperature. Finally, the heat-inactivated probiotics s was added with a protection agent and was lyophilized to be a heat-inactivated Lactobacillus reuteri GMNL-263 powder with a dosage of 2 x 1010 cells/g.
First, 6 week-old male Syrian hamsters purchased from National Laboratory Animal Center (Taipei, Taiwan) were maintained in a plastic cage. Ambient temperature was controlled at 23±1 C with a relative humidity of 60%, in addition, the animals were housed on a reverse 12 hours light/dark cycle and provided with standard laboratory chow and water ad libitum. All animals were normally maintained for 1 week and then were used for a 12-week experiment. Total 32 hamsters were is randomly divided into four groups described below, and each group had eight hamsters: 1. Control group, fed standard chow and RO water everyday for 12 weeks; 2. HFD group, fed high-fat diet (HFD) and RO water everyday for 20 12 weeks; 3. HFD with low dose of the heat-inactivated GMNL-263 group (HFD+GMNL-263(L)), fed with high-fat diet for 4 weeks, and then fed 4 x 109 cells of the heat-inactivated GMNL-263 everyday for 8 weeks; and 4. HFD with high dose of the heat-inactivated GMNL-263 group (HFD+GMNL-263(H)), fed with high-fat diet for 4 weeks, and then fed 2 x 1010 cells of the heat-inactivated GMNL-263 everyday for 8 weeks. The preparation method of high-fat diet (HFD) was modified from a normal diet for adult mice, which was added with clarified butter and soybean oil, with reference to a high-energy diet from a experiment method for evaluating the function of blood lipid regulation of health 10 food published by Ministry of Health and Welfare, Taiwan. The high-fat diet was stored at 4°C. The ingredients of the normal diet and the high-fat diet are listed as Table I.
Table I
Ingredients (e/kg) Normal diet HFD Casein 200 232 L-Cystine 3.0 3.0 DL-Mcthioninc 3.5 Corn Starch 397.48 137 Maltodextrin 132 150 Sucrose 100 162.58 Cellulose 50 50 Cholesterol 1.9 Mineral Mix (AIN-93) 35 40.60 Calcium phosphate dibasic 4.64 Vitamin Mix (AIN-93) 10 16.24 Choli ne B i tartrate 2.5 5 tert-butylhydroquinone 0.014 0.04 Soybean oil 70 40 Lard 153.5 After 12-weeks experiment, all animals were sacrificed, and tissue samples were collected for various analysis. Fig. 1 shows abdominal anatomical photographs of each group of experimental animal according to an embodiment of the present invention.
Example 1 Biochemical analysis of serum, liver, and feces Biochemical analysis of serum including the concentration of triglyceride (TG), total cholesterol (T-CHO), high-density lipoprotein cholesterol (HDL-CHO), and low-density lipoprotein cholesterol (LDL-CHO) was entrusted to National Laboratory Animal Center in Taiwan.
The malondialdehyde (MDA) content of serum was measured by using a commercially available TBARS Assay Kit (Cayman) according to the manufacturer's instruction. Absorbance at 530 nm was measured by using a microplate spectrophotometer, and the MDA concentration of serum was calculated according to the standard curve established by the concentration of the standard MDA sample.
The lipid content of liver tissue and feces was analyzed. 0.1 g of analyzed tissue was homogenized in I ml of chloroform-methanol 20 (volume ratio 2:1). The homogenized tissue was filtered, and the filtrate contained the most of lipid of analyzed tissue. After the volume of the filtrate was adjusted to 5 ml by adding chlorofoi -methanol (volume ratio 2:1), the analysis of triglyceride content and the total cholesterol content of the filtrate was entrusted by Nanguang clinical laboratory (Tainan, Taiwan).
The data was analyzed by one-way analysis of variance (ANOVA) to determine the significant difference between every experimental groups. The symbol * means that the group has significant difference (p<0.05) in comparison with the HFD group.
The results are shown as TABLE 2. The changes in lipid content of serum are the indexes of the ability of the heat-inactivated GMNL-263 to regulate blood lipid levels. Comparison with the HFD group, the T-CHO content of serum was significantly decreased by 23%, and the MDA production was also decreased in HFD+GMNL-263(H) group. However, the content of TG, LDL-CHO, HDL-CHO, the ratio of is LDL-CHO to HDL-CHO, and the ratio of HDL-CHO to T-CHO were no significant difference between the HFD+GMNL-263(H) group and the HFD group.
The results about the content of TG, T-CHO, and MDA of liver and feces are also shown in TABLE 2. In liver tissue, comparison with the HFD group, the TG content was decreased by 10% and the MDA production was decreased in HFD+GMNL-263(H) group; however, the T-CHO content was no significant difference. In feces sample, comparison with the HFD group, the content of TG and T-CHO was increased by 110% and 93% respectively in the HFD+GMNL-263(H) group.
Therefore, the heat-inactivated GMNL-263 promotes the cholesterol to be excreted in the feces, thereby reducing the cholesterol absorption in an animal to decrease the cholesterol content of body.
TABLE 2
Item Control RFD HED+GMNL-263(L) HED+GMNL-263(H) Serum TG (mg/di) 130±8* 351±66 382±107 305±75 T-CHO (mg/d1) 127+8* 287±37 243+61 222+26* LDL-CHO (mg/d1) 18+3* 86+42 91+53 65+32 HDL-CHO (rng/d1) 87±7* 140±7 125+13* 128+8 LDL-CHO/ 0.20±0.04* 0.64±0.36 0.69±0.37 0.49±0.23
HDL-CHO
HDL-CHO/ 68.58±1.88* 55.11±4.15 48.56±10.74 54.00±2 43
T-CHO
MDA (µg/ml) 4.42±0.63* 6.30±0.84 5.72±0.99 4.99±0.15 Liver TO (mg/dI) 85.0±6.5* 93.3±5.3 90.7±3.4 84.0±4.3* T-CHO (mg/di) 89.7±0.5* 130.0±4.9 118.3±12.8 127.3±6.0 MDA (tighnl) 4.37±0.49* 8.58±0.68 6.95±1.32* 5.53±0.40* feces TG (mg/di) 5.8±0.8 5.0+1.7 7.5±1.1 10.5±2.0* T-CHO (mg/dl) 6.7±0.8 5.6±1.6 8.0±1.7* 10.8+_0.8* Example 2 Analysis mRNA expression affected by the heat-inactivated GMNL-263 in liver tissue and adipose tissue The mRNA expression in (I) liver tissue and (II) adipose tissue was detected by RT-PCR. The detected genes are described as following: 1. the gene related to proinflammatory factor: interleukin-6 (IL-6) gene and tumor necrosis factor alpha (TNF-a) gene, the expression of s which induces the inflammation; 2. the gene related to lipid synthesis: fatty acid synthase (FAS) gene, sterol regulatory element binding protein-1 (SREBP-1c) gene, and peroxisome prolifera proliferator-activated receptor g (PPARy) gene, wherein the gene expression of FAS and SREBP-lc are related to lipid synthesis, and the gene expression of PPARy is related to fatty acid metabolism; 3. the gene related to cholesterol metabolism: 3-Hydroxy-3-methylglutaryl-coenzyme A reductase (HMG-CoA R) gene, LDL-cholesterol receptor (LDLR) gene, and cholesterol 7a-hydroxylase is (CYP7A1) gene, wherein the gene expression of HMG-CoA R is related to cholesterol synthesis, and the gene expression of LDLR and CYP7A1 are related to cholesterol metabolism.
The data was analyzed by one-way analysis of variance (ANOVA) to determine the significant difference between every experimental 20 groups. The symbol * means that the group has significant difference (p<0.05) in comparison with the HFD group.
(I) mRNA expression affected by heat-inactivated GMNL-263 in liver tissue Fig.2 shows a bar diagram of the relative expression of several mRNA in liver tissue of each group of Fig.l. About the gene related to proinflammatory factor, the TNF-a gene expression was inhibited in the mice that were fed with high dose of heat-inactivated GMNL-263 ((HFD+GMNL-263(H) group). About the gene related to lipid synthesis, the gene expression of FAS and SREBP-I were inhibited in the HFD+GMNL-263(H) group, but there was no significant difference in the PPARy gene expression. About the gene related to cholesterol metabolism, the gene expression of CYP7A1 and LDLR were promoted in the HFD+GMNL-263(H) group, but the HMG-CoA R gene expression in the same group has no significant change compared with the HFD group.
(II) mRNA expression affected by heat-inactivated GMNL-263 in adipose tissue About the mRNA expression in adipose tissue, the change of gene expression which is related to proinflammatory factor lipid synthesis was observed. Fig. 3 shows a bar diagram of the relative expression of several mRNA in adipose tissue of each group of Fig.l. The gene expression of TNF-a and SREBP-lc were inhibited in the HFD+GMNL-263(H) group, and the gene of PPARy was activated in the HFD+GMNL-263(H) group.
According to the results of the foregoing experiment, the heat-inactivated GMNL-263 inhibits the proinflammatory gene expression in liver tissue and adipose tissue and decreases the production of lipid peroxide in the body. It means that the heat-inactivated GMNL-263 has anti-inflammatory and anti-oxidation effects, thereby regulating blood lipid levels. Moreover, the results of gene expression s showed that the heat-inactivated GMNL-263 inhibits fatty acid synthesis in liver tissue and promote fatty acid and cholesterol metabolism, and the similar situation was shown in adipose tissue. Therefore, the heat-inactivated GMNL-263 decreases the accumulation of fatty acid and cholesterol in the body.
Example 3 Analysis the changes in the intestinal microbiota affected by the heat-inactivated GMNL-263 Whether the intestinal microbiota affected by the heat-inactivated GMNL-263 has changes was determined by RT-PCR. The content of is Bifidobacterium and Clostridium in the feces was detected.
The data was analyzed by one-way analysis of variance (ANOVA) to determine the significant difference between every experimental groups. The symbol * means that the group has significant difference (p<0.05) in comparison with the HFD group.
The results are shown in Fig. 4, showing a bar diagram of the relative expression of intestinal microbiota of each group of Fig.l. Comparison with the HFD group, the content of Clostridium was not significantly decreased in the HFD+GMNL-263(H) group, but the content of Bifidobacterium was significantly changed in the HED+GMNL-263(H) group.
According to the above description and embodiments, the composition and use of Lactobacillus reuteri GMNL-263 in decreasing s blood lipid levels of the present invention have the advantages as following: 1. Lactobacillus reuteri GMNL-263 could be used to decrease the blood lipid levels. Lactobacillus reuteri GMNL-263 specifically inhibits the gene expression related to lipid synthesis and promote the gene expression related to cholesterol metabolism, thereby promoting the cholesterol to be excreted and reducing the cholesterol absorption in an animal to decrease the cholesterol content of body, achieving the aim of decreasing the blood lipid levels.
2. Lactobacillus reuteri GMNL-263 inhibits the gene expression is of proinflammatory factor in the liver tissue and adipose tissue and decreases the production of lipid peroxide in the body. It means that the heat-inactivated GMNL-263 has anti-inflammatory and anti-oxidation effects.
3. Comparison with the Chinese herbal medicine containing 20 complex composition, Lactobacillus reuteri GMNL-263 of the present invention could not only keep the intestinal health, but also regulate blood lipid levels. Therefore, Lactobacillus reuteri GMNL-263 could further be form a composition for decreasing blood lipid levels, thereby providing a better choice to the consumers.
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