WO2018072276A1 - Health-care food and preparation method therefor - Google Patents
Health-care food and preparation method therefor Download PDFInfo
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- WO2018072276A1 WO2018072276A1 PCT/CN2016/109045 CN2016109045W WO2018072276A1 WO 2018072276 A1 WO2018072276 A1 WO 2018072276A1 CN 2016109045 W CN2016109045 W CN 2016109045W WO 2018072276 A1 WO2018072276 A1 WO 2018072276A1
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Classifications
-
- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23V—INDEXING SCHEME RELATING TO FOODS, FOODSTUFFS OR NON-ALCOHOLIC BEVERAGES AND LACTIC OR PROPIONIC ACID BACTERIA USED IN FOODSTUFFS OR FOOD PREPARATION
- A23V2002/00—Food compositions, function of food ingredients or processes for food or foodstuffs
Definitions
- the invention relates to the technical field of health foods, in particular to a health food with hypoglycemic function and a preparation method thereof.
- Diabetes mellitus is a non-infectious chronic endocrine metabolic disease with complications. With the development of social economy and the changes in people's diet, the prevalence of diabetes has increased year by year, seriously endangering human health. On December 1, 2015, the newly released data of the International Diabetes Federation (IDF)'s authoritative guide, Diabetes Atlas, shows that the current number of adult diabetes in the world has reached 415 million, while the number of adult diabetes patients in China has reached 110 million. Become the world's largest "diabetes" in diabetes.
- IDF International Diabetes Federation
- Diabetes can occur at any age. With the prolongation of the disease, it is easy to be complicated with systemic nerves, microvessels, and large blood vessels. It can lead to chronic progressive lesions of the heart, brain, kidney, nerves, and eyes. Many complications are increasing. The degree of aggravation is a serious threat to the health and life of patients. At present, most of the drugs for treating diabetes are focused on stimulating insulin production in islets, and the sensitivity of insulin target cells to insulin has not been fundamentally improved, so once the drug is stopped for a while, the blood sugar often rebounds again.
- an object of the present invention is to provide a health food and a preparation method thereof to overcome the deficiencies of the prior art.
- the active ingredient of the health food provided by the present invention is composed of the following raw materials in parts by weight:
- the active ingredient of the health food is composed of the following raw materials in a weight ratio:
- the active ingredient of the health food provided by the present invention is composed of the following raw materials in a weight ratio:
- the active ingredient of the health food is composed of the following raw materials in a weight ratio:
- the health food is used to prepare a hypoglycemic effect Healthy food or medicine, and safe and non-toxic side effects.
- the invention also provides a preparation method of the above health food, comprising the following steps:
- extract II After mixing mulberry, clam meat and spirulina, first add water for boiling extraction, then concentrate, add ethanol to the concentrated liquid, filter and take the precipitate, dry and pulverize to obtain extract II;
- the extract I, the extract II and the notoginseng powder were mixed to obtain the health food.
- the method for preparing the extract I comprises the following steps:
- Extracts first add alcohol for reflux extraction, add 6-10 times of alcohol each time, extract for 1 to 2 hours each time, extract 1 ⁇ 4 times, combine the extracts, concentrate and dry, and dry at 80 to 90 ° C, pulverized through 80 to 120 mesh sieve to obtain extract I.
- the method for preparing the extract I comprises the following steps:
- the method of preparing the extract II comprises the following steps:
- Mix mulberry, clam meat and spirulina first add water for boiling extraction, extract 1 ⁇ 4 times, add 6 ⁇ 10 times of water each time, extract for 1 ⁇ 2 hours each time, combine the decoction and concentrate;
- Extract II Ethanol precipitation was added to the concentrate for 16 to 30 hours, and the precipitate was taken after filtration, dried and pulverized to obtain Extract II.
- the method of preparing the extract II comprises the following steps:
- a volume concentration of 80 to 95% of ethanol to ethanol is added to a volume concentration of 70 to 90%, and then precipitation is carried out for 16 to 30 hours. After filtration, the precipitate is taken, dried at 60 to 75 ° C, and pulverized through 80 to 120 mesh. Sieve to obtain extract II.
- the health food provided by the present invention and the preparation method thereof are prepared by combining the traditional Chinese medicine Pueraria, Gynostemma pentaphyllum, Mulberry, Sanqi and Wenyu meat, and Spirulina to prepare a health food for lowering blood sugar and reducing diabetic complications.
- the health food has the function of assisting blood sugar lowering, and has safe and non-toxic side effects.
- Traditional Chinese medicine has a long history of diabetes prevention and control, and has accumulated rich experience and formed a unique theoretical understanding.
- Traditional Chinese medicine refers to diabetes as a form of diabetes. Many effective prescriptions can significantly improve the symptoms of “three more and one less” in diabetic patients, and can effectively reduce the complications of diabetes.
- traditional Chinese medicine Pueraria, Gynostemma, Mulberry, Sanqi and Wenyu meat, Spirulina to help reduce blood sugar and reduce diabetes complications from the perspective of traditional TCM syndrome differentiation and modern chemical composition and biological activity research. Health food, and safe and non-toxic side effects to make up for the shortcomings of the prior art.
- the extract I, the extract II and the notoginseng powder were mixed for 30 min, and then uniformly mixed with suitable excipients, and loaded with 0# capsule, 0.5 g/granule, 60 capsules/bottle.
- the health food is obtained by sealing and labeling.
- the extract I, the extract II and the notoginseng powder are mixed, and then uniformly mixed with a suitable auxiliary material, and the granules are prepared according to the preparation method, and the health food is obtained by dispensing.
- the extract I, the extract II and the notoginseng powder are mixed for 40 minutes, and then uniformly mixed with a suitable auxiliary material, compressed, and packaged to obtain the health food.
- the extract I, the extract II and the notoginseng powder are mixed for 30 minutes, and then uniformly mixed with a suitable auxiliary material, and the oral liquid is prepared according to the preparation method, and the health food is obtained by encapsulation.
- the extract I, the extract II and the notoginseng powder are mixed, and then uniformly mixed with a suitable auxiliary material, and the pellet is prepared according to the preparation method, and the package is obtained to obtain the health food.
- mice Three doses of the test group (5, 10, 20 times the recommended amount of the human body), and a model control group, a test sample group (high dose) and a blank control group for each normal animal.
- Group 12 mice. Weigh 1.25, 2.50, 5.00g of Gesang Jiangtang Capsules, add pure water to 100mL, mix well, and mix them into 12.5, 25.0, 50.0mg/mL concentration suspension, respectively, and give the corresponding dose groups to the stomach, normal
- the test sample group of animals was given a concentration of 50.0 mg/mL suspension, and the volume of gastric perfusion was 0.2 mL/10 gBW.
- the model control group and the normal animal blank control group were given an equal volume of pure water, once a day, and continuously administered by stomach. 30 days.
- Reagents blood glucose test strips, etc.
- mice were given an intraperitoneal injection of alloxan (120 mg/kg BW) 24 hours after fasting. After 5 days, fasting for 4 hours, blood is taken from the eye to measure blood sugar. If the blood glucose level is 10 to 25 mmol/L, the model for making high blood sugar can be considered successful. 120 mice were selected for modeling, and 102 of them were successfully modeled. 96 mice with successful modeling were included in the experiment, and the mice were divided into 2 batches. The first batch of 48 patients were tested for fasting blood glucose lowering, and the second batch of 48 mice were tested for glucose tolerance.
- the first batch of hyperglycemic model animals were randomly divided into 4 groups according to the fasting 4 hours blood glucose level, 12 in each group.
- the test group was given different concentrations of sample solution, and the model control group was given pure water for 30 consecutive days.
- the fasting blood glucose level was measured by blood sampling (fasting before the test), and the fasting blood glucose level and percentage of blood glucose decreased in each group were compared.
- Percentage of blood glucose drop (pre-experiment blood glucose value - post-experiment blood glucose value) / pre-experiment blood glucose value x 100%.
- test result can be judged as positive.
- test sample group (high dose), 12 in each group.
- the rest of the operation is the same as 1.6.2.
- Glucose tolerance test 48 rats of the second batch of hyperglycemic model mice were randomly divided into 4 groups according to the fasting 4 hours blood glucose level, 12 in each group, and the gavage method was the same as 1.6.2. Mice were fasted for 4 hours on day 31, the test group was given different concentrations of sample solution, and the model control group was given an equal volume of pure water. After 15 minutes, each group was orally administered with a solution of glucose (2.0 g/kg BW). The blood glucose levels at 0, 0.5, and 2 hours after glucose administration were measured, and the changes in the area under the blood glucose curve at each time point after the glucose concentration of the model control group and the test sample group were observed.
- test result can be judged as positive.
- Test data processing Statistical analysis of variance analysis was performed using SPSS11.0 statistical software.
- the initial body weight, mid-term body weight, terminal body weight and weight gain of the mice in each dose group of hyperglycemic model were not significantly different from those in the model control group (P>0.05). See Table 1; mice in the normal animal experimental group. The initial body weight, mid-term weight, terminal body weight and weight gain were not significantly different from the blank control group (P>0.05), as shown in Table 2. The results showed that the sample had no significant effect on the weight gain of hyperglycemic model mice and normal mice.
- mice were given different doses of Gesang Jiangtang Capsules for 30 days.
- the blood glucose levels of the 30th day of each dose group were lower than the model control group.
- the blood glucose drop value and percentage decrease of each dose group were higher than the model control group, and high.
- the blood glucose level, blood glucose decrease value and percentage decrease of the middle dose group were significantly different from the model control group (P ⁇ 0.01 or P ⁇ 0.05), indicating that the sample has the effect of lowering the fasting blood glucose of the hyperglycemic model mice.
- ** indicates P ⁇ 0.01 compared with the model control group.
- Gesang Jiangtang Capsules with 250, 500, 1000mg/kg BW (equivalent to 5, 10, 20 times the recommended amount of human body) were administered to hyperglycemic mice for 30 days, which could reduce the fasting blood glucose level of mice.
- the glucose tolerance test results were positive, and had no significant effect on the weight gain of the mice; the normal mice were continuously gavage for 30 days at a dose of 1000 mg/kg BW. There was no significant effect on fasting blood glucose and weight gain in mice.
- the sample has an auxiliary blood glucose lowering function.
- mice of Kunming mice weighing 18-22 g were selected by the maximum tolerated dose (MTD) test method, half male and half female. Animals were fasted for 16 hours before the test, and were not allowed to drink water. Weigh 20.0g sample, add pure water to 40mL, mix well, prepare 500mg/mL concentration suspension, and then give the animal 2 times (interval 6h), each dose is 0.4mL/20gBW, total dose It is 20,000 mg/kg BW. After the gavage, the animal's poisoning performance was observed and recorded. Weigh once a week and observe for two weeks. At the end of the experiment, dissect the animals for general observation. The acute toxicity of the test substance was evaluated according to the toxicity classification standard.
- Dose selection and test substance administration method 80 SD rats were selected, female and male, and the body weight was 60-80 g. The animals were randomly divided into 4 groups, namely a negative control group and 3 test groups, 20 in each group, half male and half male. The doses of the three test groups were set to 5000, 2500, and 1250 mg/kg BW, respectively, which corresponded to 100, 50, and 25 times the recommended dose of the human body. Weigh 50.0, 25.0, 12.5g samples, add pure water to 100mL, mix well, and mix 500, 250, 125mg/mL concentration suspension, and weigh the corresponding dose group according to the volume of 1.0mL/100g BW. The negative control group was given an equal volume of pure water, and was intragastrically administered once a day for 30 days.
- mice were administered with a dose of 20,000 mg/kg BW, the animals grew well and no body weight was affected. No symptoms of poisoning were observed in the mice tested, and no animal death was observed for 14 days. At the end of the experiment, the animals were dissected and observed in general, and no obvious abnormal changes were observed in the main organs such as liver, kidney, spleen, heart, lung, stomach and intestine. The results showed that the acute oral toxicity MTD of the sample to mice was greater than 20000 mg/kg BW, and the acute oral toxicity was non-toxic.
- the results are shown in Table 7 to Table 8.
- the rats were intragastrically administered with Gesang Jiangtang Capsules at a dose of 5000, 2500, and 1250 mg/kg BW for 30 days.
- the male and female rats in each dose group received weekly weight, weight, and weight.
- the results are shown in Table 11 and Table 12.
- the rats were intragastrically administered with Gesang Jiangtang Capsule at 5000, 2500, 1250 mg/kg BW for 30 days.
- Serum aspartate aminotransferase, alanine aminotransferase and urea were used in the female and male rats in each dose group.
- Nitrogen, creatinine, cholesterol, triglyceride, total protein, albumin, and blood glucose were not significantly different from the control group (P>0.05), indicating that the sample had no significant effect on blood biochemical parameters in rats.
- Hepatocyte dot necrosis was observed in the hepatic lobules of male and 2 female rats; a small amount of inflammatory cell infiltration was observed in the liver portal area of one male and two female rats in the high-dose group and the control group.
- the high-dose group there were 2 males and 1 female, and 1 male and 1 female rats in the control group showed a small amount of inflammatory cell infiltration in the renal cortex.
- the above tissue lesions belong to the spontaneous mild lesions of the animals, and the degree of tissue lesions of the two groups of animals is similar, so it can be ruled out by the sample, and no histopathological changes are observed in other organs, indicating that the sample is the above organ tissues of the rats. No damage.
- test strain enrichment solution 0.1 mL of the test strain enrichment solution, 0.1 mL of the test solution and 0.5 mL of the S-9 mixture (when metabolic activation is required) are sequentially added to the maintained top culture medium, and then mixed and poured. On the bottom medium plate.
- the five test doses were 5000, 1000, 200, 40, and 8 ⁇ g/dish, respectively, with spontaneous reversion control, solvent control, and positive mutagen control.
- the spontaneous reversal control was the same as the sample group except that no sample was added.
- the solvent control replaced the sample with sterile pure water, and the rest of the conditions were the same as the sample group.
- Each strain of each dose group was made into 3 parallel dishes.
- the cells were cultured at 37 ° C for 48 hours, and the number of colonies per dish was counted. The entire set of tests was repeated twice under the same conditions. If the number of revertant colonies of the test substance increases more than twice the number of spontaneously reverted colonies and has a dose-response relationship, the mutagenesis test is positive.
- the test was carried out by oral gavage twice at intervals of 24 hours. Choose a weight of 25 ⁇ 30g 50 Kunming mice were randomly divided into 5 groups, 10 in each group, half male and half female. The three doses in the experimental group were 10000, 5000, 2500 mg/kg BW, respectively, with pure water as the negative control and 40 mg/kg BW dose of cyclophosphamide (cp) as the positive control.
- cp cyclophosphamide
- the micronucleus rate was calculated as the micronucleus-containing PCE per thousand; and 200 polychromatic red blood cells were counted at the same time.
- the ratio of polychromatic red blood cells to mature red blood cells (PCE/NCE) was calculated.
- the statistical processing was performed by using the Poisson distribution mean comparison method in the SPSS statistical software. For example, the micronucleus rate of the experimental group was higher than that of the negative control group, and there was a significant dose-response relationship and statistical significance, which was a positive result.
- mice in each dose group of the present invention was not significantly different from that of the negative control group (P>0.05), and the PCE/NCE values of each dose group were not less than that of the negative control group. %, there was no significant difference compared with the negative control group, and the micronucleus rate of the cyclophosphamide positive control group was significantly different from that of the negative control group (P ⁇ 0.01), suggesting that the bone marrow of the sample of the present invention was not observed.
- the cells have damage and inhibition.
- Gavage once a day for 5 consecutive days The animals were sacrificed on the 30th day after the last dose, and the sperm smears of the epididymis were taken, fixed by methanol, and stained with eosin. Under an optical microscope, 1000 sperm counts were counted per animal, and the rate of sperm deformity was calculated. Wilcoxon rank sum test statistical processing in SPSS statistical software was applied. For example, the sperm deformity rate of the experimental group was higher than that of the negative control group, and it was statistically significant, and there was a dose-response relationship, which was a positive result.
- the sample of the present invention did not significantly change the incidence of sperm abnormality in mice.
- the sperm deformity rate of each sample group was not significantly different from that of the negative control group (P>0.05), while cyclophosphamide was not significantly different (P>0.05).
- the difference between the positive control group and the negative control group was very significant (P ⁇ 0.01), suggesting that the sperm of the present invention did not cause spermatogenesis in male mice.
- mice test Three genotoxicity tests (Ames test, mouse bone marrow micronucleus test, mouse sperm abnormality test) were negative. This indicates that the present invention is not genotoxic.
Abstract
A health-care food consisting of the following raw materials in parts by weight: 5-30 parts of radix puerariae extract; 2-20 parts of gynostemma pentaphylla extract; 0.5-8 parts of radix notoginseng extract; 1-20 parts of fructus mori extract; 1-10 parts of clam meat extract; and 2-20 parts of spirulina extract. According to the health-care food and the preparation method therefor, Chinese traditional medicines of radix puerariae, gynostemma pentaphylla, fructus mori and radix notoginseng are compatible with clam meat and spirulina to prepare the health-care food which can aid in reducing blood glucose and diabetic complications; and the health-care food has remarkable blood glucose reduction effect, is safe and has no toxic and side effects.
Description
本发明涉及保健食品技术领域,特别是一种具有降血糖功能的保健食品及其制备方法。The invention relates to the technical field of health foods, in particular to a health food with hypoglycemic function and a preparation method thereof.
糖尿病(diabetes mellitus,DM)是一种非传染性慢性内分泌代谢性疾病,多伴有并发症。随着社会经济的发展,人们饮食结构的变化,糖尿病患病率逐年增高,严重危害人类身体健康。在2015年12月1日,国际糖尿病联合会(IDF)的权威指南《Diabetes Atlas》新发布的数据表明,当前全世界成年糖尿病人数已达4.15亿人,而我国成人糖尿病患者达到1.1亿人,成为世界糖尿病“第一大国”。Diabetes mellitus (DM) is a non-infectious chronic endocrine metabolic disease with complications. With the development of social economy and the changes in people's diet, the prevalence of diabetes has increased year by year, seriously endangering human health. On December 1, 2015, the newly released data of the International Diabetes Federation (IDF)'s authoritative guide, Diabetes Atlas, shows that the current number of adult diabetes in the world has reached 415 million, while the number of adult diabetes patients in China has reached 110 million. Become the world's largest "diabetes" in diabetes.
糖尿病可发生于任何年龄,随着病程延长,容易并发全身神经、微血管、大血管病变,并可导致心、脑、肾、神经及眼等组织器官的慢性进行性病变,诸多并发症日趋增多,程度加重,严重危害着患者健康和生命。目前,治疗糖尿病的药物大多偏重于刺激胰岛产生胰岛素,而胰岛素的靶细胞对胰岛素的敏感性并未得到根本的改善,所以一旦停药一段时间后,血糖往往再次反弹。同时,由于长期用药对胰岛的刺激,使胰岛处于长期紧张的工作状态,而最终导致胰岛功能的疲惫,致使糖尿病人最终不得不借助体外胰岛素来帮助降糖,这样会进一步导致胰岛功能的部分或全部丧失,同时由于血糖反复反弹,仍使血液的粘稠度增加,血液的微循环发生障碍,最终乃会发生心、脑、肾及皮肤神经等方面的并发症。Diabetes can occur at any age. With the prolongation of the disease, it is easy to be complicated with systemic nerves, microvessels, and large blood vessels. It can lead to chronic progressive lesions of the heart, brain, kidney, nerves, and eyes. Many complications are increasing. The degree of aggravation is a serious threat to the health and life of patients. At present, most of the drugs for treating diabetes are focused on stimulating insulin production in islets, and the sensitivity of insulin target cells to insulin has not been fundamentally improved, so once the drug is stopped for a while, the blood sugar often rebounds again. At the same time, due to the stimulation of islets by long-term medication, the islets are in a long-term intense working state, which eventually leads to the fatigue of islet function, so that diabetics eventually have to use insulin in vitro to help reduce blood sugar, which will further lead to the part of islet function or All of them are lost. At the same time, due to the repeated rebound of blood sugar, the viscosity of the blood is increased, and the microcirculation of the blood is impeded. Finally, complications such as heart, brain, kidney and skin nerves occur.
发明内容Summary of the invention
有鉴于此,本发明的目的在于提出一种保健食品及其制备方法,以克服现有技术的不足。In view of the above, an object of the present invention is to provide a health food and a preparation method thereof to overcome the deficiencies of the prior art.
基于上述目的,本发明提供的保健食品的有效成分由以下原料按重量份组成:
Based on the above object, the active ingredient of the health food provided by the present invention is composed of the following raw materials in parts by weight:
5~30份葛根;5 to 30 parts of pueraria;
2~20份绞股蓝;2 to 20 strands of Gynostemma pentaphyllum;
0.5~8份三七;0.5 to 8 parts of Sanqi;
1~20份桑椹子;1 to 20 parts of mulberry;
1~10份文蛤肉;和1 to 10 pieces of meat; and
2~20份螺旋藻。2 to 20 parts of spirulina.
在本发明的一些实施例中,所述保健食品的有效成分由以下原料按重量份配比组成:In some embodiments of the present invention, the active ingredient of the health food is composed of the following raw materials in a weight ratio:
7~25份葛根;7 to 25 parts of Pueraria;
5~15份绞股蓝;5 to 15 parts of Gynostemma pentaphyllum;
1~5份三七;1 to 5 copies of Sanqi;
4~15份桑椹子;4 to 15 parts of mulberry;
2~8份文蛤肉;和2 to 8 pieces of meat; and
4~15份螺旋藻。4 to 15 parts of spirulina.
作为本发明的又一个实施例,本发明提供的保健食品的有效成分由以下原料按重量份配比组成:As still another embodiment of the present invention, the active ingredient of the health food provided by the present invention is composed of the following raw materials in a weight ratio:
5~30份葛根的提取物;5 to 30 parts of Pueraria extract;
2~20份绞股蓝的提取物;2 to 20 parts of Gynostemma pentaphyllum extract;
0.5~8份三七的提取物;0.5 to 8 parts of the extract of Panax notoginseng;
1~20份桑椹子的提取物;1 to 20 parts of the extract of mulberry;
1~10份文蛤肉的提取物;和1 to 10 extracts of clam meat; and
2~20份螺旋藻的提取物。2 to 20 parts of spirulina extract.
在本发明的一些实施例中,所述保健食品的有效成分由以下原料按重量份配比组成:In some embodiments of the present invention, the active ingredient of the health food is composed of the following raw materials in a weight ratio:
7~25份葛根的提取物;7 to 25 parts of Pueraria extract;
5~15份绞股蓝的提取物;5 to 15 parts of Gynostemma pentaphyllum extract;
1~5份三七的提取物;1 to 5 parts of the extract of Panax notoginseng;
4~15份桑椹子的提取物;4 to 15 parts of the extract of mulberry;
2~8份文蛤肉的提取物;和2 to 8 extracts of clam meat; and
4~15份螺旋藻的提取物。4 to 15 parts of Spirulina extract.
在本发明的一些实施例中,所述保健食品用于制备具有降血糖作用的保
健食品或药物,且安全无毒副作用。In some embodiments of the invention, the health food is used to prepare a hypoglycemic effect
Healthy food or medicine, and safe and non-toxic side effects.
本发明还提供一种上述保健食品的制备方法,包括以下步骤:The invention also provides a preparation method of the above health food, comprising the following steps:
将葛根和绞股蓝混合,先加酒精进行回流提取,然后浓缩、干燥,再粉碎得到提取物Ⅰ;Mixing Pueraria and Gynostemma pentaphyllum, first adding alcohol for reflux extraction, then concentrating, drying, and then pulverizing to obtain extract I;
将桑椹子、文蛤肉和螺旋藻混合后,先加水进行沸腾提取,然后浓缩,在浓缩液中加入乙醇,过滤后取沉淀物,干燥、粉碎后得到提取物Ⅱ;After mixing mulberry, clam meat and spirulina, first add water for boiling extraction, then concentrate, add ethanol to the concentrated liquid, filter and take the precipitate, dry and pulverize to obtain extract II;
将三七打成细粉,三七粉备用;Beat the Sanqi into a fine powder and use the Sanqi powder for later use;
将提取物Ⅰ、提取物Ⅱ和三七粉混合,得到所述保健食品。The extract I, the extract II and the notoginseng powder were mixed to obtain the health food.
在本发明的一些实施例中,所述提取物Ⅰ的制备方法包括以下步骤:In some embodiments of the invention, the method for preparing the extract I comprises the following steps:
将葛根和绞股蓝混合,先加酒精进行回流提取,每次加入6~10倍量的酒精,每次提取1~2小时,共提取1~4次,合并提取液后浓缩、干燥,干燥温度为80~90℃,粉碎过80~120目筛,得到提取物Ⅰ。Mix Pueraria and Gynostemma pentaphyllum, first add alcohol for reflux extraction, add 6-10 times of alcohol each time, extract for 1 to 2 hours each time, extract 1~4 times, combine the extracts, concentrate and dry, and dry at 80 to 90 ° C, pulverized through 80 to 120 mesh sieve to obtain extract I.
在本发明的一些实施例中,所述提取物Ⅰ的制备方法包括以下步骤:In some embodiments of the invention, the method for preparing the extract I comprises the following steps:
将葛根和绞股蓝混合,第一次加6~10倍量的酒精,先浸泡30~60min后,回流提取,第二次加6~8倍量的酒精,每次提取1~2小时,合并提取液后浓缩、干燥,干燥温度为80~90℃,粉碎过80~120目筛,得到提取物Ⅰ。Mix Pueraria and Gynostemma pentaphyllum, add 6-10 times of alcohol for the first time, soak for 30~60min, then extract by reflux, add 6~8 times of alcohol for the second time, extract for 1~2 hours each time, combine and extract The solution was concentrated, dried, dried at a temperature of 80 to 90 ° C, and pulverized through a sieve of 80 to 120 mesh to obtain an extract I.
在本发明的一些实施例中,所述提取物Ⅱ的制备方法包括以下步骤:In some embodiments of the invention, the method of preparing the extract II comprises the following steps:
将桑椹子、文蛤肉和螺旋藻混合,先加水进行沸腾提取,共提取1~4次,每次加6~10倍量的水,每次提取1~2小时,合并煎液后浓缩;Mix mulberry, clam meat and spirulina, first add water for boiling extraction, extract 1~4 times, add 6~10 times of water each time, extract for 1~2 hours each time, combine the decoction and concentrate;
向浓缩液中加入乙醇沉淀16~30小时,过滤后取沉淀物,干燥、粉碎后得到提取物Ⅱ。Ethanol precipitation was added to the concentrate for 16 to 30 hours, and the precipitate was taken after filtration, dried and pulverized to obtain Extract II.
在本发明的一些实施例中,所述提取物Ⅱ的制备方法包括以下步骤:In some embodiments of the invention, the method of preparing the extract II comprises the following steps:
将桑椹子、文蛤肉和螺旋藻混合,第一次加6~10倍量的水,先浸泡30~60min后,加热至沸腾提取,第二次加5~9倍量的水,每次提取1~2小时,合并煎液后浓缩;Mix mulberry, clam meat and spirulina, add 6~10 times of water for the first time, soak for 30~60min, then heat to boiling extraction, add 5~9 times of water for the second time, each extraction 1 to 2 hours, combined with decoction and concentrated;
向浓缩液中加入体积浓度为80~95%的乙醇至乙醇的体积浓度为70~90%,然后沉淀16~30小时,过滤后取沉淀物,60~75℃干燥、粉碎过80~120目筛,得到提取物Ⅱ。To the concentrate, a volume concentration of 80 to 95% of ethanol to ethanol is added to a volume concentration of 70 to 90%, and then precipitation is carried out for 16 to 30 hours. After filtration, the precipitate is taken, dried at 60 to 75 ° C, and pulverized through 80 to 120 mesh. Sieve to obtain extract II.
在本发明的一些实施例中,将所述煎液浓缩至d=1.0~1.5,80℃条件下。
In some embodiments of the invention, the decoction is concentrated to d = 1.0 to 1.5 at 80 °C.
从上面所述可以看出,本发明提供的保健食品及其制备方法,将中药葛根,绞股蓝,桑椹,三七与文蛤肉,螺旋藻配伍制备成辅助降血糖、减少糖尿病并发症的保健食品,该保健食品具有辅助降血糖功能,且安全无毒副作用。It can be seen from the above that the health food provided by the present invention and the preparation method thereof are prepared by combining the traditional Chinese medicine Pueraria, Gynostemma pentaphyllum, Mulberry, Sanqi and Wenyu meat, and Spirulina to prepare a health food for lowering blood sugar and reducing diabetic complications. The health food has the function of assisting blood sugar lowering, and has safe and non-toxic side effects.
为使本发明的目的、技术方案和优点更加清楚明白,以下结合具体实施例,对本发明进一步详细说明。In order to make the objects, the technical solutions and the advantages of the present invention more comprehensible, the present invention will be further described in detail below in conjunction with the specific embodiments.
中医药对糖尿病防治具有悠久的历史,积累了丰富的经验,并形成独特理论认识。中医称糖尿病为消渴症,许多有效方药可明显改善糖尿病病人的“三多一少”症状,并可有效减少糖尿病并发症。我们经过长期的实验研究,从传统中医辨证论治,以及现代化学成分、生物活性研究角度,将中药葛根,绞股蓝,桑椹,三七与文蛤肉,螺旋藻配伍制备成辅助降血糖、减少糖尿病并发症的保健食品,且安全无毒副作用,以弥补现有技术的不足。Traditional Chinese medicine has a long history of diabetes prevention and control, and has accumulated rich experience and formed a unique theoretical understanding. Traditional Chinese medicine refers to diabetes as a form of diabetes. Many effective prescriptions can significantly improve the symptoms of “three more and one less” in diabetic patients, and can effectively reduce the complications of diabetes. After long-term experimental research, we have prepared traditional Chinese medicine Pueraria, Gynostemma, Mulberry, Sanqi and Wenyu meat, Spirulina to help reduce blood sugar and reduce diabetes complications from the perspective of traditional TCM syndrome differentiation and modern chemical composition and biological activity research. Health food, and safe and non-toxic side effects to make up for the shortcomings of the prior art.
实施例1:保健食品胶囊剂的制备Example 1: Preparation of health food capsules
(1)将20千克葛根和12千克绞股蓝混合,第一次加8倍量的体积浓度为75%食用酒精,先浸泡30分钟后,回流提取1小时,第二次加6倍量的体积浓度为75%食用酒精,回流提取1小时,提取2次后将提取液(合并提取液)浓缩和干燥,干燥温度为85℃,粉碎过100目筛,得到提取物Ⅰ;(1) Mix 20 kg of Pueraria and 12 kg of Gynostemma pentaphyllum, add 8 times the volume concentration of 75% edible alcohol for the first time, soak for 30 minutes, then extract for 1 hour under reflux, and add volume of 6 times for the second time. 75% edible alcohol, reflux extraction for 1 hour, after extraction 2 times, the extract (combined extract) is concentrated and dried, drying temperature is 85 ° C, crushed through a 100 mesh sieve to obtain extract I;
(2)先将3.5千克文蛤肉加适量水浸泡20小时后,再与6千克桑椹子和15千克螺旋藻混合,第一次加8倍量的水,先浸泡30分钟后,加热至沸腾提取1小时,第二次加6倍量的水,加热至沸腾提取2小时,合并2次煎液(过滤)后,将煎液浓缩至d≈1.2(80℃);向浓缩液中加入体积浓度为85%的乙醇至乙醇的体积浓度为75%,然后沉淀24小时后,过滤,取沉淀物(多糖),烘箱75℃干燥,粉碎过100目筛,得到提取物Ⅱ;(2) first soak 3.5 kilograms of clam meat with appropriate amount of water for 20 hours, then mix with 6 kilograms of mulberry and 15 kilograms of spirulina, add 8 times of water for the first time, soak for 30 minutes, then heat to boiling extraction. 1 hour, the second time added 6 times the amount of water, heated to boiling extraction for 2 hours, combined with 2 decoctions (filtered), the decoction was concentrated to d≈1.2 (80 ° C); volume concentration was added to the concentrate 85% ethanol to ethanol volume concentration of 75%, and then precipitated for 24 hours, filtered, the precipitate (polysaccharide), dried in an oven at 75 ° C, crushed through a 100 mesh sieve to obtain extract II;
(3)将2千克三七打成粉,过100目筛,湿热灭菌,得到三七粉;(3) Put 2 kg of Sanqi into powder, pass through a 100 mesh sieve, and sterilize with damp heat to obtain Panax notoginseng powder;
(4)将提取物Ⅰ、提取物Ⅱ和三七粉混合30min,再与适宜辅料混合均匀,装0#胶囊,0.5g/粒,60粒/瓶。封口,贴标签,即得到所述保健食品。(4) The extract I, the extract II and the notoginseng powder were mixed for 30 min, and then uniformly mixed with suitable excipients, and loaded with 0# capsule, 0.5 g/granule, 60 capsules/bottle. The health food is obtained by sealing and labeling.
实施例2:保健食品颗粒剂的制备
Example 2: Preparation of health food granules
(1)将8千克葛根和10千克绞股蓝混合,第一次加6倍量的体积浓度为78%食用酒精,先浸泡45分钟后,回流提取1.5小时,第二次加8倍量的体积浓度为70%食用酒精,回流提取2小时,提取2次后将提取液(合并提取液)浓缩和干燥,干燥温度为88℃,粉碎过100目筛,得到提取物Ⅰ;(1) Mix 8 kg of Pueraria and 10 kg of Gynostemma pentaphyllum, add 6 times the volume concentration of 78% edible alcohol for the first time, soak for 45 minutes, then reflux for 1.5 hours, and add the volume concentration of 8 times for the second time. For 70% edible alcohol, reflux extraction for 2 hours, after extraction 2 times, the extract (combined extract) is concentrated and dried, drying temperature is 88 ° C, crushed through a 100 mesh sieve to obtain extract I;
(2)先将8千克文蛤肉加适量水浸泡24小时后,再与11千克桑椹子和9千克螺旋藻混合,第一次加7倍量的水,先浸泡55分钟后,加热至沸腾提取1.2小时,第二次加9倍量的水,加热至沸腾提取1小时,合并2次煎液(过滤)后,将煎液浓缩至d≈1.3(80℃);向浓缩液中加入体积浓度为90%的乙醇至乙醇的体积浓度为86%,然后沉淀28小时后,过滤,取沉淀物(多糖),烘箱65℃干燥,粉碎过120目筛,得到提取物Ⅱ;(2) first soak 8 kg of simmered meat with appropriate amount of water for 24 hours, then mix with 11 kg of mulberry and 9 kg of spirulina, add 7 times of water for the first time, soak for 55 minutes, then heat to boiling extraction. 1.2 hours, the second time added 9 times the amount of water, heated to boiling extraction for 1 hour, combined with 2 decoctions (filtered), the decoction was concentrated to d≈1.3 (80 ° C); volume concentration was added to the concentrate The volume concentration of 90% ethanol to ethanol is 86%, and then precipitated for 28 hours, filtered, and the precipitate (polysaccharide) is taken, dried in an oven at 65 ° C, and pulverized through a 120 mesh sieve to obtain an extract II;
(3)将3.5千克三七打成粉,过100目筛,湿热灭菌,得到三七粉;(3) Beating 3.5 kg of Sanqi into powder, passing through 100 mesh sieve, and sterilizing by damp heat to obtain Panax notoginseng powder;
(4)将提取物Ⅰ、提取物Ⅱ和三七粉混合,再与适宜辅料混合均匀,按制剂方法制成颗粒剂,分装即得到所述保健食品。(4) The extract I, the extract II and the notoginseng powder are mixed, and then uniformly mixed with a suitable auxiliary material, and the granules are prepared according to the preparation method, and the health food is obtained by dispensing.
实施例3:保健食品片剂的制备Example 3: Preparation of health food tablets
(1)将5千克葛根和6千克绞股蓝混合,第一次加6倍量的体积浓度为70%食用酒精,先浸泡40分钟后,回流提取1.2小时,第二次加8倍量的体积浓度为75%食用酒精,回流提取2小时,第三次加7倍量的75%食用酒精,回流提取1小时,提取3次后将提取液(合并提取液)浓缩和干燥,干燥温度为88℃,粉碎过80目筛,得到提取物Ⅰ;(1) Mix 5 kg of Pueraria and 6 kg of Gynostemma pentaphyllum, add 6 times the volume concentration of 70% edible alcohol for the first time, soak for 40 minutes, then reflux for 1.2 hours, and add the volume concentration of 8 times for the second time. It is 75% edible alcohol, reflux extraction for 2 hours, the third addition of 7 times the amount of 75% edible alcohol, reflux extraction for 1 hour, extraction 3 times, the extract (combined extract) is concentrated and dried, drying temperature is 88 ° C , crushed through a 80 mesh sieve to obtain extract I;
(2)先将1.5千克文蛤肉加适量水浸泡18小时后,再与15千克桑椹子和11千克螺旋藻混合,第一次加6倍量的水,先浸泡30分钟后,加热至沸腾提取1.3小时,第二次加5倍量的水,加热至沸腾提取1小时,合并2次煎液(过滤)后,将煎液浓缩至d≈1.15(80℃);向浓缩液中加入体积浓度为92%的乙醇至乙醇的体积浓度为84%,然后沉淀20h后,过滤,取沉淀物(多糖),烘箱65℃干燥,粉碎过110目筛,得到提取物Ⅱ;(2) first soak 1.5 kg of clam meat with appropriate amount of water for 18 hours, then mix with 15 kg of mulberry and 11 kg of spirulina, add 6 times of water for the first time, soak for 30 minutes, then heat to boiling extraction. 1.3 hours, the second addition of 5 times the amount of water, heated to boiling extraction for 1 hour, combined with 2 decoctions (filtered), the decoction was concentrated to d≈ 1.15 (80 ° C); volume concentration was added to the concentrate 92% ethanol to ethanol volume concentration of 84%, and then precipitated for 20h, filtered, the precipitate (polysaccharide), dried in an oven at 65 ° C, crushed through a 110 mesh sieve to obtain extract II;
(3)将2.8千克三七打成粉,过120目筛,湿热灭菌,得到三七粉;(3) Put 2.8 kg of Sanqi into powder, pass through a 120 mesh sieve, and sterilize with damp heat to obtain Panax notoginseng powder;
(4)将提取物Ⅰ、提取物Ⅱ和三七粉混合40min,再与适宜辅料混合均匀,压片,封装,即得到所述保健食品。(4) The extract I, the extract II and the notoginseng powder are mixed for 40 minutes, and then uniformly mixed with a suitable auxiliary material, compressed, and packaged to obtain the health food.
实施例4:保健食品膏剂的制备
Example 4: Preparation of health food ointment
(1)将26千克葛根和9千克绞股蓝混合,第一次加10倍量的体积浓度为70%食用酒精,先浸泡60分钟后,回流提取1小时,第二次加7倍量的体积浓度为70%食用酒精,回流提取1小时,提取2次后将提取液(合并提取液)浓缩和干燥,干燥温度为80℃,粉碎过80目筛,得到提取物Ⅰ;(1) Mix 26 kg of Pueraria and 9 kg of Gynostemma pentaphyllum, add 10 times the volume concentration of 70% edible alcohol for the first time, soak for 60 minutes, then extract for 1 hour under reflux, and add volume of 7 times for the second time. For 70% edible alcohol, reflux extraction for 1 hour, after extraction 2 times, the extract (combined extract) is concentrated and dried, drying temperature is 80 ° C, crushed through 80 mesh sieve, to obtain extract I;
(2)先将7.5千克文蛤肉加适量水浸泡22小时后,再与13千克桑椹子和18千克螺旋藻混合,第一次加9倍量的水,先浸泡38分钟后,加热至沸腾提取1.6小时,第二次加7倍量的水,加热至沸腾提取1.5小时,第二次加8倍量的水,加热至沸腾提取1小时,合并3次煎液(过滤)后,将煎液浓缩至d≈1.25(80℃);向浓缩液中加入体积浓度为80%的乙醇至乙醇的体积浓度为72%,然后沉淀29小时后,过滤,取沉淀物(多糖),烘箱68℃干燥,粉碎过100目筛,得到提取物Ⅱ;(2) Soak 7.5 kg of clam meat with appropriate amount of water for 22 hours, then mix with 13 kg of mulberry and 18 kg of spirulina, add 9 times of water for the first time, soak for 38 minutes, then heat to boiling extraction. 1.6 hours, the second time adding 7 times the amount of water, heating to boiling extraction for 1.5 hours, the second time adding 8 times the amount of water, heating to boiling extraction for 1 hour, combining 3 times of decoction (filtration), the decoction Concentrated to d≈1.25 (80 ° C); a volume concentration of 80% ethanol to ethanol was added to the concentrate at a volume concentration of 72%, and then precipitated for 29 hours, filtered, and the precipitate (polysaccharide) was taken and dried in an oven at 68 ° C. , crushed through a 100 mesh sieve to obtain extract II;
(3)将4.5千克三七打成粉,过120目筛,湿热灭菌,得到三七粉;(3) Put 4.5 kg of Sanqi into powder, pass through a 120 mesh sieve, and sterilize with damp heat to obtain Panax notoginseng powder;
(4)将提取物Ⅰ、提取物Ⅱ和三七粉混合,再与适宜辅料混合均匀,按制剂方法制成膏剂,封装,即得到所述保健食品。(4) The extract I, the extract II and the notoginseng powder are mixed, and then uniformly mixed with a suitable auxiliary material, and the paste is prepared according to a preparation method, and the package is obtained to obtain the health food.
实施例5:保健食品口服液的制备Example 5: Preparation of health food oral liquid
(1)将14千克葛根和13千克绞股蓝混合,第一次加7.5倍量的体积浓度为80%食用酒精,先浸泡44分钟后,回流提取1.8小时,第二次加6倍量的体积浓度为75%食用酒精,回流提取2小时,提取2次后将提取液(合并提取液)浓缩和干燥,干燥温度为90℃,粉碎过120目筛,得到提取物Ⅰ;(1) Mix 14 kg of Pueraria and 13 kg of Gynostemma pentaphyllum, add 7.5 times the volume concentration of 80% edible alcohol for the first time, soak for 44 minutes, then reflux for 1.8 hours, and add a volume of 6 times for the second time. 75% edible alcohol, reflux extraction for 2 hours, after extraction 2 times, the extract (combined extract) is concentrated and dried, drying temperature is 90 ° C, crushed through a 120 mesh sieve to obtain extract I;
(2)先将7千克文蛤肉加适量水浸泡17小时后,再与10千克桑椹子和5千克螺旋藻混合,第一次加7倍量的水,先浸泡55分钟后,加热至沸腾提取1.7小时,第二次加5.5倍量的水,加热至沸腾提取2小时,合并2次煎液(过滤)后,将煎液浓缩至d≈1.2(80℃);向浓缩液中加入体积浓度为93%的乙醇至乙醇的体积浓度为87%,然后沉淀20小时后,过滤,取沉淀物(多糖),烘箱72℃干燥,粉碎过100目筛,得到提取物Ⅱ;(2) first soak 7 kg of clam meat with appropriate amount of water for 17 hours, then mix with 10 kg of mulberry and 5 kg of spirulina, add 7 times of water for the first time, soak for 55 minutes, then heat to boiling extraction. 1.7 hours, the second time added 5.5 times the amount of water, heated to boiling extraction for 2 hours, combined with 2 decoctions (filtered), the decoction was concentrated to d≈1.2 (80 ° C); volume concentration was added to the concentrate The volume concentration of 93% ethanol to ethanol is 87%, and then precipitated for 20 hours, filtered, and the precipitate (polysaccharide) is taken, dried in an oven at 72 ° C, and pulverized through a 100 mesh sieve to obtain an extract II;
(3)将2千克三七打成粉,过100目筛,湿热灭菌,得到三七粉;(3) Put 2 kg of Sanqi into powder, pass through a 100 mesh sieve, and sterilize with damp heat to obtain Panax notoginseng powder;
(4)将提取物Ⅰ、提取物Ⅱ和三七粉混合30min,再与适宜辅料混合均匀,按制剂方法制成口服液,封装,即得到所述保健食品。(4) The extract I, the extract II and the notoginseng powder are mixed for 30 minutes, and then uniformly mixed with a suitable auxiliary material, and the oral liquid is prepared according to the preparation method, and the health food is obtained by encapsulation.
实施例6:保健食品丸剂的制备
Example 6: Preparation of health food pellets
(1)将15千克葛根和13千克绞股蓝混合,第一次加6.5倍量的体积浓度为76%食用酒精,先浸泡45分钟后,回流提取1.9小时,第二次加7.5倍量的体积浓度为72%食用酒精,回流提取1.1小时,提取2次后将提取液(合并提取液)浓缩和干燥,干燥温度为82℃,粉碎过100目筛,得到提取物Ⅰ;(1) Mix 15 kg of Pueraria and 13 kg of Gynostemma pentaphyllum, add 6.5 times the volume of the first time to 76% edible alcohol, soak for 45 minutes, then extract for 1.9 hours under reflux, and add 7.5 times the volume concentration for the second time. For 72% edible alcohol, reflux extraction for 1.1 hours, after extracting 2 times, the extract (combined extract) is concentrated and dried, drying temperature is 82 ° C, crushed through a 100 mesh sieve to obtain extract I;
(2)先将9千克文蛤肉加适量水浸泡24小时后,再与3千克桑椹子和9千克螺旋藻混合,第一次加6倍量的水,先浸泡58分钟后,加热至沸腾提取1小时,第二次加5.5倍量的水,加热至沸腾提取1小时,第三次加5.5倍量的水,加热至沸腾提取1.5小时,第四次加5倍量的水,加热至沸腾提取1.2小时,合并4次煎液(过滤)后,将煎液浓缩至d≈1.1(80℃);向浓缩液中加入体积浓度为78%的乙醇至乙醇的体积浓度为70%,然后沉淀18小时后,过滤,取沉淀物(多糖),烘箱73℃干燥,粉碎过100目筛,得到提取物Ⅱ;(2) first soak 9 kg of clam meat with appropriate amount of water for 24 hours, then mix with 3 kg of mulberry and 9 kg of spirulina, add 6 times of water for the first time, soak for 58 minutes, then heat to boiling extraction. 1 hour, the second time adding 5.5 times the amount of water, heating to boiling extraction for 1 hour, the third time adding 5.5 times the amount of water, heating to boiling extraction for 1.5 hours, the fourth time adding 5 times the amount of water, heating to boiling After extracting for 1.2 hours and combining 4 times of decoction (filtration), the decoction was concentrated to d≈1.1 (80 ° C); a volume concentration of 78% ethanol to ethanol was added to the concentrate to a volume concentration of 70%, and then precipitated. After 18 hours, the mixture was filtered, and the precipitate (polysaccharide) was taken, dried in an oven at 73 ° C, and pulverized through a 100 mesh sieve to obtain an extract II;
(3)将4千克三七打成粉,过100目筛,湿热灭菌,得到三七粉;(3) Dilute 4 kg of Sanqi into a powder, pass through a 100 mesh sieve, and sterilize with damp heat to obtain Panax notoginseng powder;
(4)将提取物Ⅰ、提取物Ⅱ和三七粉混合,再与适宜辅料混合均匀,按制剂方法制成丸剂,封装,即得到所述保健食品。(4) The extract I, the extract II and the notoginseng powder are mixed, and then uniformly mixed with a suitable auxiliary material, and the pellet is prepared according to the preparation method, and the package is obtained to obtain the health food.
辅助降血糖功能动物实验Auxiliary hypoglycemic function animal experiment
1材料和方法1 Materials and methods
1.1样品:葛桑降糖胶囊,规格:0.5g/粒,产品批号:150201,置干燥处保存。人口服推荐用量为每人(成人)每日2次,每次3粒,成人体重按60kg计算,折合剂量为50mg/kgBW。取胶囊内容物进行实验。1.1 Sample: Gesang hypoglycemic capsule, specification: 0.5g / grain, product batch number: 150201, stored in a dry place. The recommended dosage for oral administration is 2 times per person (adult) per person, 3 capsules per time, and the adult weight is calculated as 60kg, and the equivalent dose is 50mg/kg BW. Capsule contents were taken for experiments.
1.2实验动物:选用广东省医学实验动物中心繁殖的SPF级健康成年昆明种雄性小鼠1441.2 Experimental animals: SPF-class healthy adult Kunming male mice 144 were selected from Guangdong Medical Experimental Animal Center.
只,体重为24~28克,实验动物生产许可证号:SCXK(桂)2013-0002,实验动物质量合格证号:44007200027357。Only, the weight is 24 ~ 28 grams, the experimental animal production license number: SCXK (Gui) 2013-0002, laboratory animal quality certificate number: 44007200027357.
1.3实验动物房环境条件:动物实验室为屏障系统,使用许可证号:SYXK(桂)2011-0005。1.3 Experimental animal room environmental conditions: animal laboratory is a barrier system, use license number: SYXK (Gui) 2011-0005.
动物实验室温度:22~25℃,相对湿度:55~70%。Animal laboratory temperature: 22 ~ 25 ° C, relative humidity: 55 ~ 70%.
1.4剂量选择与受试物给予方式:根据该样品的人体推荐用量,设250、500、1000mg/kgBW
1.4 Dose selection and administration of the test substance: According to the recommended dosage of the sample, 250, 500, 1000 mg/kg BW
(分别相当于人体推荐用量的5、10、20倍)3个剂量的试验组,同时设一个模型对照组,另设一个正常动物的受试样品组(高剂量)和空白对照组,每组12只小鼠。分别称取葛桑降糖胶囊1.25、2.50、5.00g,各加纯水至100mL,混匀,配成12.5、25.0、50.0mg/mL浓度混悬液,分别给予相应剂量组动物灌胃,正常动物的受试样品组给予50.0mg/mL浓度混悬液,灌胃体积为0.2mL/10gBW,模型对照组及正常动物空白对照组给予等体积的纯水,每天灌胃一次,连续灌胃30天。Three doses of the test group (5, 10, 20 times the recommended amount of the human body), and a model control group, a test sample group (high dose) and a blank control group for each normal animal. Group 12 mice. Weigh 1.25, 2.50, 5.00g of Gesang Jiangtang Capsules, add pure water to 100mL, mix well, and mix them into 12.5, 25.0, 50.0mg/mL concentration suspension, respectively, and give the corresponding dose groups to the stomach, normal The test sample group of animals was given a concentration of 50.0 mg/mL suspension, and the volume of gastric perfusion was 0.2 mL/10 gBW. The model control group and the normal animal blank control group were given an equal volume of pure water, once a day, and continuously administered by stomach. 30 days.
1.5主要仪器与试剂1.5 main instruments and reagents
仪器:罗康全卓越型血糖仪、电子分析天平等。Instrument: Luo Kangquan excellent blood glucose meter, electronic analysis of the same day.
试剂:血糖试纸等。Reagents: blood glucose test strips, etc.
1.6实验方法:依据国家食品药品监督管理局发布的国食药监保化[2012]107号《关于印发抗氧化功能评价方法等9个保健功能评价方法的通知》的附件3—辅助降血糖功能评价方法,采用动物试验方案一—胰岛损伤高血糖模型法。1.6 Experimental method: According to the National Food and Drug Administration issued the National Food and Drug Administration [2012] No. 107 "Notice on Printing and Evaluation of Antioxidant Function Evaluation Methods, 9 Applicable Methods for Evaluation of Health Function", Annex 3 - Auxiliary Hypoglycemic Function The evaluation method uses an animal test protocol--islet damage high blood glucose model method.
1.6.1高血糖模型动物造模1.6.1 Hyperglycemia model animal modeling
小鼠禁食24小时后给予四氧嘧啶(120mg/kgBW)一次腹腔注射造模。5天后禁食4小时,眼内眦取血测血糖,若血糖值为10~25mmol/L,则可认为造高血糖模型成功。选取120只小鼠进行造模,结果其中造模成功102只。选用造模成功的小鼠96只纳入试验,将小鼠分为2批,第一批48只进行降低空腹血糖试验,第二批48只进行糖耐量试验。The mice were given an intraperitoneal injection of alloxan (120 mg/kg BW) 24 hours after fasting. After 5 days, fasting for 4 hours, blood is taken from the eye to measure blood sugar. If the blood glucose level is 10 to 25 mmol/L, the model for making high blood sugar can be considered successful. 120 mice were selected for modeling, and 102 of them were successfully modeled. 96 mice with successful modeling were included in the experiment, and the mice were divided into 2 batches. The first batch of 48 patients were tested for fasting blood glucose lowering, and the second batch of 48 mice were tested for glucose tolerance.
1.6.2降低空腹血糖试验1.6.2 Reduce the fasting blood glucose test
第一批高血糖模型动物,按禁食4小时血糖水平进行分层随机分成4组,每组12只。试验组给予不同浓度的样品溶液,模型对照组给纯水,连续30天,采血测空腹血糖值(禁食同试验前),比较各组动物空腹血糖值及血糖下降百分率。The first batch of hyperglycemic model animals were randomly divided into 4 groups according to the fasting 4 hours blood glucose level, 12 in each group. The test group was given different concentrations of sample solution, and the model control group was given pure water for 30 consecutive days. The fasting blood glucose level was measured by blood sampling (fasting before the test), and the fasting blood glucose level and percentage of blood glucose decreased in each group were compared.
血糖下降百分率=(实验前血糖值-实验后血糖值)/实验前血糖值×100%。Percentage of blood glucose drop = (pre-experiment blood glucose value - post-experiment blood glucose value) / pre-experiment blood glucose value x 100%.
在模型成立条件下,如试验组空腹血糖实测值比模型对照组降低或血糖下降百分率有统计学意义,可判定该项试验结果为阳性。Under the condition of model establishment, if the measured value of fasting blood glucose in the experimental group is lower than the model control group or the percentage of blood glucose drop is statistically significant, the test result can be judged as positive.
1.6.3正常动物:选健康成年动物24只,按禁食4小时血糖水平分组,随机分成空白对照组
1.6.3 Normal animals: 24 healthy adult animals were selected and grouped according to fasting blood glucose levels for 4 hours, randomly divided into blank control groups.
和受试样品组(高剂量),每组12只。余操作同1.6.2。And the test sample group (high dose), 12 in each group. The rest of the operation is the same as 1.6.2.
1.6.4糖耐量试验:第二批高血糖模型小鼠48只,按禁食4小时血糖水平进行分层随机分成4组,每组12只,灌胃方式同1.6.2。第31天将小鼠禁食4小时,试验组给予不同浓度的样品溶液,模型对照组给予等体积纯水。15分钟后,各组经口灌胃给予葡萄糖(2.0g/kgBW)溶液。测定给葡萄糖后0、0.5、2小时血糖值,观察模型对照组与受试样品组给葡萄糖后各时间点血糖曲线下面积的变化。1.6.4 Glucose tolerance test: 48 rats of the second batch of hyperglycemic model mice were randomly divided into 4 groups according to the fasting 4 hours blood glucose level, 12 in each group, and the gavage method was the same as 1.6.2. Mice were fasted for 4 hours on day 31, the test group was given different concentrations of sample solution, and the model control group was given an equal volume of pure water. After 15 minutes, each group was orally administered with a solution of glucose (2.0 g/kg BW). The blood glucose levels at 0, 0.5, and 2 hours after glucose administration were measured, and the changes in the area under the blood glucose curve at each time point after the glucose concentration of the model control group and the test sample group were observed.
血糖曲线下面积=0.25×(0小时血糖值+4×0.5小时血糖值+3×2小时血糖值)Area under the blood glucose curve = 0.25 × (0 hour blood glucose level + 4 × 0.5 hour blood glucose value + 3 × 2 hours blood glucose value)
在模型成立条件下,如试验组在给葡萄糖后0、0.5、2小时血糖曲线下面积比模型对照组低并有统计学意义,即可判定该项试验结果为阳性。Under the condition of the model establishment, if the area under the blood glucose curve of the test group at 0, 0.5, and 2 hours after glucose administration is lower than the model control group and has statistical significance, the test result can be judged as positive.
1.7试验数据处理:采用SPSS11.0统计软件进行方差分析统计处理。1.7 Test data processing: Statistical analysis of variance analysis was performed using SPSS11.0 statistical software.
1.8结果判定:在模型成立条件下,空腹血糖和糖耐量二项指标中有一项指标阳性,且对正常动物空腹血糖无影响,即可判定该受试样品辅助降血糖功能动物实验结果阳性。1.8 Result judgment: Under the condition of model establishment, one of the two indicators of fasting blood glucose and glucose tolerance is positive, and it has no effect on the fasting blood glucose of normal animals. It can be determined that the test sample is positive for the blood glucose-reducing animal.
2试验结果2 test results
2.1样品对小鼠体重的影响2.1 The effect of sample on mouse body weight
高血糖模型动物样品各剂量组小鼠的初始体重、中期体重、末期体重及增重与模型对照组比较,差异均无显著性(P>0.05),见表1;正常动物实验组的小鼠初始体重、中期体重、末期体重及增重与空白对照组比较,差异均无显著性(P>0.05),见表2。结果表明,该样品对高血糖模型小鼠和正常小鼠的体重增长无明显影响。The initial body weight, mid-term body weight, terminal body weight and weight gain of the mice in each dose group of hyperglycemic model were not significantly different from those in the model control group (P>0.05). See Table 1; mice in the normal animal experimental group. The initial body weight, mid-term weight, terminal body weight and weight gain were not significantly different from the blank control group (P>0.05), as shown in Table 2. The results showed that the sample had no significant effect on the weight gain of hyperglycemic model mice and normal mice.
表1.葛桑降糖胶囊对高血糖模型小鼠体重的影响
Table 1. Effect of Gesang Jiangtang Capsule on body weight of hyperglycemic model mice
注:各剂量组小鼠的初始体重、中期体重、末期体重及增重与模型对照组比较,差异均无显著性(P>0.05)。
Note: The initial body weight, mid-term weight, terminal body weight and weight gain of the mice in each dose group were not significantly different from the model control group (P>0.05).
(续)表1.葛桑降糖胶囊对高血糖模型小鼠体重的影响
(Continued) Table 1. Effect of Gesang Jiangtang Capsule on body weight of hyperglycemic model mice
注:各剂量组小鼠的初始体重、中期体重、末期体重及增重与模型对照组比较,差异均无显著性(P>0.05)。Note: The initial body weight, mid-term weight, terminal body weight and weight gain of the mice in each dose group were not significantly different from the model control group (P>0.05).
表2.葛桑降糖胶囊对正常小鼠体重的影响
Table 2. Effect of Gesang Jiangtang Capsule on normal mouse weight
注:试验组小鼠的初始体重、中期体重、末期体重及增重与空白对照组比较,差异均无显著性(P>0.05)。Note: The initial body weight, mid-term body weight, terminal body weight and weight gain of the experimental group were not significantly different from the blank control group (P>0.05).
2.2样品对高血糖模型小鼠空腹血糖的影响2.2 Effect of sample on fasting blood glucose in hyperglycemic model mice
从表3可见,造模后4小时禁食后血糖值>10mmol/L,可见模型成立。经口给予小鼠不同剂量的葛桑降糖胶囊30天,各剂量组的第30天血糖值均低于模型对照组,各剂量组血糖下降值及下降百分率均大于模型对照组,且高、中剂量组的血糖值、血糖下降值及下降百分率与模型对照组的差异具有显著性(P<0.01或P<0.05),表明该样品具有降低高血糖模型小鼠的空腹血糖的作用。It can be seen from Table 3 that the blood glucose level after fasting is >10 mmol/L after 4 hours of modeling, and the model is established. The mice were given different doses of Gesang Jiangtang Capsules for 30 days. The blood glucose levels of the 30th day of each dose group were lower than the model control group. The blood glucose drop value and percentage decrease of each dose group were higher than the model control group, and high. The blood glucose level, blood glucose decrease value and percentage decrease of the middle dose group were significantly different from the model control group (P<0.01 or P<0.05), indicating that the sample has the effect of lowering the fasting blood glucose of the hyperglycemic model mice.
表3.高血糖模型小鼠的空腹血糖结果
Table 3. Fasting blood glucose results in hyperglycemic model mice
注:*表示与模型对照组比较,P<0.05、**表示与模型对照组比较,P<0.01。Note: * indicates that compared with the model control group, P < 0.05, ** indicates comparison with the model control group, P < 0.01.
2.3样品对高血糖模型小鼠糖耐量试验的影响2.3 Effect of sample on glucose tolerance test in hyperglycemic model mice
表4.高血糖模型小鼠糖耐量试验结果
Table 4. Results of glucose tolerance test in hyperglycemic model mice
注:**表示与模型对照组比较,P<0.01。Note: ** indicates P<0.01 compared with the model control group.
从表4可见,经口给予高血糖模型小鼠不同剂量的葛桑降糖胶囊30天后,样品各剂量组的血糖曲线下面积均低于模型对照组,且高、中剂量组与模型对照组的差异具有非常显著性(P<0.01),表明该样品具有降低高血糖小鼠糖耐量试验各时点血糖曲线下面积的作用,糖耐量试验结果阳性。。It can be seen from Table 4 that after 30 days of oral administration of different doses of Gesang Jiangtang Capsules in hyperglycemic model mice, the area under the blood glucose curve of each dose group was lower than that of the model control group, and the high and middle dose groups and the model control group. The difference was very significant (P<0.01), indicating that the sample has the effect of reducing the area under the blood glucose curve at each time point in the glucose tolerance test of hyperglycemic mice, and the glucose tolerance test results are positive. .
2.4样品对正常小鼠空腹血糖的影响2.4 Effect of sample on fasting blood glucose in normal mice
由表5可见,经口给予正常小鼠1000mg/kg BW剂量的葛桑降糖胶囊30天,小鼠的空腹血糖值与空白对照组比较无显著性差异(P>0.05),表明该样品对正常小鼠的空腹血糖没有明显影响。As can be seen from Table 5, there was no significant difference in the fasting blood glucose level between the mice and the normal control group (P>0.05). Fasting blood glucose in normal mice had no significant effect.
表5.正常小鼠空腹血糖结果
Table 5. Fasting blood glucose results in normal mice
注:试验前后样品组与空白对照组的血糖值比较,差异无显著性(P>0.05)。Note: There was no significant difference in blood glucose values between the sample group before and after the test and the blank control group (P>0.05).
3结论:3 Conclusion:
分别以250、500、1000mg/kg BW(相当于人体推荐量5、10、20倍)剂量的葛桑降糖胶囊给高血糖模型小鼠连续灌胃30天,能降低小鼠的空腹血糖值,降低小鼠的糖耐量试验各时点血糖曲线下面积,糖耐量试验结果阳性,对小鼠的体重增长无明显影响;以1000mg/kg BW剂量的样品给正常小鼠连续灌胃30天,对小鼠的空腹血糖值和体重增长无明显影响。综上结果,该样品具有辅助降血糖功能。Gesang Jiangtang Capsules with 250, 500, 1000mg/kg BW (equivalent to 5, 10, 20 times the recommended amount of human body) were administered to hyperglycemic mice for 30 days, which could reduce the fasting blood glucose level of mice. To reduce the area under the blood glucose curve at the time of the glucose tolerance test in mice, the glucose tolerance test results were positive, and had no significant effect on the weight gain of the mice; the normal mice were continuously gavage for 30 days at a dose of 1000 mg/kg BW. There was no significant effect on fasting blood glucose and weight gain in mice. In summary, the sample has an auxiliary blood glucose lowering function.
急性与慢性毒性研究Acute and chronic toxicity studies
1材料和方法1 Materials and methods
1.1样品:葛桑降糖胶囊,规格:0.5g/粒,产品批号:150201,置阴凉
干燥处保存。人口服推荐用量为每人(成人)每日2次,每次3粒,成人体重按60kg计算,折合剂量为50mg/kg BW。1.1 sample: Gesang hypoglycemic capsule, specification: 0.5g / grain, product batch number: 150201, set in the shade
Store in a dry place. The recommended dosage for oral administration is 2 times per person (adult) per person, 3 capsules per time, and the adult weight is calculated as 60kg, and the equivalent dose is 50mg/kg BW.
1.2实验动物及环境:SPF级健康昆明种小鼠和SD种大鼠,均由广西医科大学实验动物中心繁殖,实验动物生产许可证号:SCXK(桂)2014-0002,实验动物质量合格证号:45000300000170、45000300000223;45000300000379。动物实验室为屏障系统,使用许可证号:SYXK(桂)2011-0005。动物实验室温度:22~25℃,相对湿度:55~70%。1.2 Experimental animals and environment: SPF-grade healthy Kunming mice and SD rats were all propagated by the Experimental Animal Center of Guangxi Medical University. The experimental animal production license number: SCXK (Gui) 2014-0002, the experimental animal quality certificate number : 45000300000170, 45000300000223; 45000300000379. The animal laboratory is a barrier system, using the license number: SYXK (Gui) 2011-0005. Animal laboratory temperature: 22 ~ 25 ° C, relative humidity: 55 ~ 70%.
1.3小鼠急性经口毒性试验:采用最大耐受剂量(MTD)试验法,选体重18~22g的昆明种小鼠20只,雌雄各半。试验前动物禁食16小时,不限饮水。称取20.0g样品,加纯水至40mL,混匀,配成500mg/mL浓度混悬液,然后给动物灌胃2次(间隔6h),每次灌胃量为0.4mL/20gBW,合计剂量为20000mg/kg BW。灌胃后观察、记录动物的中毒表现。每周称重一次,观察两周时间,试验结束解剖动物进行大体观察。按毒性分级标准评价受试物的急性毒性。1.3 Acute oral toxicity test of mice: 20 mice of Kunming mice weighing 18-22 g were selected by the maximum tolerated dose (MTD) test method, half male and half female. Animals were fasted for 16 hours before the test, and were not allowed to drink water. Weigh 20.0g sample, add pure water to 40mL, mix well, prepare 500mg/mL concentration suspension, and then give the animal 2 times (interval 6h), each dose is 0.4mL/20gBW, total dose It is 20,000 mg/kg BW. After the gavage, the animal's poisoning performance was observed and recorded. Weigh once a week and observe for two weeks. At the end of the experiment, dissect the animals for general observation. The acute toxicity of the test substance was evaluated according to the toxicity classification standard.
1.4大鼠30天喂养试验1.4 Rat 30-day feeding test
1.4.1剂量选择与受试物给予方式:选SD种大鼠80只,雌、雄性各半,体重60~80g。将动物随机分为4组,即阴性对照组和3个试验组,每组20只,雌、雄各半。3个试验组剂量分别设为以5000、2500、1250mg/kgBW,分别相当于人体推荐剂量的100、50、25倍。分别称取50.0、25.0、12.5g样品,各加纯水至100mL,混匀,配成500、250、125mg/mL浓度混悬液,按1.0mL/100g BW的体积给相应剂量组动物灌胃,阴性对照组灌给等体积的纯水,每天灌胃一次,连续灌胃30天。1.4.1 Dose selection and test substance administration method: 80 SD rats were selected, female and male, and the body weight was 60-80 g. The animals were randomly divided into 4 groups, namely a negative control group and 3 test groups, 20 in each group, half male and half male. The doses of the three test groups were set to 5000, 2500, and 1250 mg/kg BW, respectively, which corresponded to 100, 50, and 25 times the recommended dose of the human body. Weigh 50.0, 25.0, 12.5g samples, add pure water to 100mL, mix well, and mix 500, 250, 125mg/mL concentration suspension, and weigh the corresponding dose group according to the volume of 1.0mL/100g BW. The negative control group was given an equal volume of pure water, and was intragastrically administered once a day for 30 days.
1.4.2实验方法:实验期间所有动物给予普通饲料,单笼饲养,自由摄食饮水。每天观察动物的活动和生长情况,每周加食2次,记录给食量和剩食量,每周称一次体重,计算每周进食量和食物利用率。实验结束动物隔夜禁食(禁食16h,不限饮水),然后称动物空腹体重,处死大鼠,采2份血样,一份血抗凝用血球计数仪检测Hb、RBC、WBC及其分类、PLT等;另一份血不抗凝分离血清,用试剂盒和全自动生化分析仪检测血清AST、ALT、BUN、Cr、TC、TG、Glu、TP、Alb等项目。采血后解剖动物,进行大体观察,取肝脏、肾脏、脾脏和睾丸等脏器进行称重,计算脏/体比值,取肝脏、肾脏、脾脏、胃、十二指肠、睾丸和卵巢等脏器进行病理组织学检查。在对
各剂量组动物作大体检查未发现明显病变和生化指标改变时,只进行高剂量组和对照组动物的主要脏器的组织病理学检查,如发现病变则对中、低剂量组相应器官及组织进行检查。1.4.2 Experimental method: All animals were given normal feed during the experiment, fed in a single cage, and fed freely. Animals were observed daily for activity and growth, fed twice a week, recorded for food intake and leftovers, weekly weight, and weekly food intake and food utilization. At the end of the experiment, the animals were fasted overnight (fasting for 16 hours, not limited to drinking water), then the animals were weighed, the rats were sacrificed, 2 blood samples were taken, and a blood anticoagulation blood cell counter was used to detect Hb, RBC, WBC and its classification. PLT and the like; another blood is not anticoagulated to separate serum, and the serum AST, ALT, BUN, Cr, TC, TG, Glu, TP, Alb and other items are detected by a kit and an automatic biochemical analyzer. After blood collection, the animals were dissected and grossly observed. The liver, kidney, spleen and testicles were weighed to calculate the ratio of the body to the body. The liver, kidney, spleen, stomach, duodenum, testis and ovary were taken. Perform a histopathological examination. In the right
Animals in each dose group were examined for gross lesions and biochemical indicators. Only the histopathological examination of the main organs of the high-dose group and the control group was performed. If the lesions were found, the corresponding organs and tissues of the middle- and low-dose groups were found. checking.
1.4.3实验数据统计:应用SPSS统计软件进行单因素方差分析。在统计分析时,先对数据进行方差齐性检验,若方差齐,采用单因素方差分析进行总体比较,发现差异再用Dunnett检验进行多个剂量组与对照组均数间的两两比较。若方差不齐则对数据进行适当的变量转换,满足方差齐性检验后,用转换后的数据进行统计;若转换数据仍未达到方差齐要求,改用秩和检验进行统计分析。1.4.3 Experimental data statistics: One-way ANOVA was performed using SPSS statistical software. In the statistical analysis, the data were first tested for homogeneity of variance. If the variances were homogeneous, one-way analysis of variance was used for the overall comparison. The difference was found by Dunnett test to compare the two groups between the multiple dose groups and the control group. If the variance is not uniform, the data is subjected to appropriate variable conversion, and after the homogeneity test of the variance is satisfied, the converted data is used for statistics; if the converted data still does not meet the variance requirement, the rank sum test is used for statistical analysis.
2结果2 results
2.1急性经口毒性试验2.1 Acute oral toxicity test
表6 葛桑降糖胶囊对小鼠的急性毒性试验结果
Table 6 Results of acute toxicity test of Gesang Jiangtang Capsule on mice
从表6可见,以20000mg/kg BW剂量的样品给予小鼠灌胃后,动物生长良好,未见体重受到影响。受试小鼠均未见有中毒症状,观察14天无动物死亡。试验结束解剖动物、大体观察,肝、肾、脾、心、肺、胃、肠等主要脏器均未见明显异常改变。结果表明,该样品对小鼠的急性经口毒性MTD大于20000mg/kg BW,急性经口毒性属无毒级。As can be seen from Table 6, after the mice were administered with a dose of 20,000 mg/kg BW, the animals grew well and no body weight was affected. No symptoms of poisoning were observed in the mice tested, and no animal death was observed for 14 days. At the end of the experiment, the animals were dissected and observed in general, and no obvious abnormal changes were observed in the main organs such as liver, kidney, spleen, heart, lung, stomach and intestine. The results showed that the acute oral toxicity MTD of the sample to mice was greater than 20000 mg/kg BW, and the acute oral toxicity was non-toxic.
2.2大鼠30天喂养试验2.2 Rat 30-day feeding test
2.2.1动物一般表现:实验期间,各组动物生长发育良好,未见动物有异常行为和中毒表现,各组动物均无死亡。2.2.1 General performance of animals: During the experiment, the animals in each group had good growth and development. No abnormal behavior and poisoning performance were observed in the animals, and no deaths were observed in each group.
2.2.2样品对大鼠体重及食物利用率的影响2.2.2 Effect of sample on body weight and food utilization rate in rats
结果见表7~表8,以5000、2500、1250mg/kg BW剂量的葛桑降糖胶囊给大鼠灌胃30天,实验期间,样品各剂量组雌雄鼠每周的体重、增重量、每周进食量及总进食量、每周食物利用率及总食物利用率与对照组比较,差异均无显著性(P>0.05),表明该样品对大鼠的体重增长和食物利用率无明显影响。
The results are shown in Table 7 to Table 8. The rats were intragastrically administered with Gesang Jiangtang Capsules at a dose of 5000, 2500, and 1250 mg/kg BW for 30 days. During the experiment period, the male and female rats in each dose group received weekly weight, weight, and weight. There was no significant difference in weekly food intake and total food intake, weekly food utilization rate and total food utilization rate compared with the control group (P>0.05), indicating that the sample had no significant effect on body weight gain and food utilization rate. .
表7 葛桑降糖胶囊对大鼠体重的影响
Table 7 Effect of Gesang Jiangtang Capsule on Rat Body Weight
注:表中各剂量组与阴性对照组比较,差异均无显著性(P>0.05)。Note: There was no significant difference between the dose groups in the table and the negative control group (P>0.05).
表8 葛桑降糖胶囊对大鼠总食物利用率的影响
Table 8 Effect of Gesang Jiangtang Capsule on total food utilization rate in rats
注:表中各剂量组与阴性对照组比较,差异均无显著性(P>0.05)。Note: There was no significant difference between the dose groups in the table and the negative control group (P>0.05).
2.5.3样品对大鼠血常规指标的影响2.5.3 Effect of sample on blood routine indicators in rats
表9 葛桑降糖胶囊30天喂养试验结束大鼠血常规指标检查结果
Table 9 Results of blood routine indicators of rats after the 30-day feeding test of Gesang Jiangtang Capsule
注:表中各剂量组与阴性对照组比较,差异均无显著性(P>0.05)。Note: There was no significant difference between the dose groups in the table and the negative control group (P>0.05).
表10 葛桑降糖胶囊30天喂养试验结束大鼠血常规指标检查结果
Table 10 Results of blood routine indicators of rats after the 30-day feeding test of Gesang Jiangtang Capsule
注:表中各剂量组与阴性对照组比较,差异均无显著性(P>0.05)。Note: There was no significant difference between the dose groups in the table and the negative control group (P>0.05).
从表9、表10可见,以5000、2500、1250mg/kgBW剂量的葛桑降糖胶囊给大鼠灌胃30天,样品各剂量组雌、雄性大鼠的血红蛋白、红细胞总数、白细胞总数及其分类、血小板数与对照组比较,差异均无显著性(P>0.05),表明该样品对大鼠的血常规指标无明显影响。It can be seen from Tables 9 and 10 that Gesang Jiangtang Capsules at the doses of 5000, 2500, and 1250 mg/kg BW were administered to rats for 30 days. The hemoglobin, total number of red blood cells, total number of white blood cells and their total number of male and female rats in each dose group were There was no significant difference in the classification and platelet counts compared with the control group (P>0.05), indicating that the sample had no significant effect on the blood routine parameters of the rats.
2.5.4样品对大鼠血液生化指标的影响2.5.4 Effect of sample on blood biochemical parameters in rats
结果见表11、表12,以5000、2500、1250mg/kgBW剂量的葛桑降糖胶囊给大鼠灌胃30天,样品各剂量组雌、雄性大鼠的血清谷草转氨酶、谷丙转氨酶、尿素氮、肌酐、胆固醇、甘油三酯、总蛋白、白蛋白、血糖与对照组比较,差异均无显著性(P>0.05),表明该样品对大鼠的血液生化指标无明显影响。The results are shown in Table 11 and Table 12. The rats were intragastrically administered with Gesang Jiangtang Capsule at 5000, 2500, 1250 mg/kg BW for 30 days. Serum aspartate aminotransferase, alanine aminotransferase and urea were used in the female and male rats in each dose group. Nitrogen, creatinine, cholesterol, triglyceride, total protein, albumin, and blood glucose were not significantly different from the control group (P>0.05), indicating that the sample had no significant effect on blood biochemical parameters in rats.
表11 葛桑降糖胶囊30天喂养试验结束大鼠血液生化指标检查结果
Table 11 Results of blood biochemical indicators in rats after the 30-day feeding test of Gesang Jiangtang Capsule
注:表中各剂量组与阴性对照组比较,差异均无显著性(P>0.05)。Note: There was no significant difference between the dose groups in the table and the negative control group (P>0.05).
表12 葛桑降糖胶囊30天喂养试验结束大鼠血液生化指标检查结果
Table 12 Results of blood biochemical indicators in rats after the 30-day feeding test of Gesang Jiangtang Capsule
注:表中各剂量组与阴性对照组比较,差异均无显著性(P>0.05)。Note: There was no significant difference between the dose groups in the table and the negative control group (P>0.05).
2.5.5样品对大鼠脏器重量及脏器/体重比值的影响2.5.5 Effect of sample on organ weight and organ/body weight ratio in rats
结果,以5000、2500、1250mg/kgBW剂量的葛桑降糖胶囊给大鼠灌胃30天,样品各剂量组大鼠的肝、肾、脾、雄鼠睾丸重量和肝/体、肾/体、脾/体、雄鼠睾/体比值与对照组比较,差异均无显著性(P>0.05),表明该样品对大鼠的脏器重量及脏器/体重比值无明显影响。Results: Gesang Jiangtang Capsules at 5000, 2500, 1250mg/kg BW were administered to rats for 30 days. The testis weight and liver/body, kidney/body of liver, kidney, spleen and male rats in each dose group The spleen/body and male testicular/body ratios were not significantly different from the control group (P>0.05), indicating that the sample had no significant effect on the organ weight and organ/body weight ratio.
2.5.6解剖大体观察及组织学检查结果2.5.6 Anatomical gross observation and histological examination results
实验结束解剖动物,大体观察各组动物均未发现明显病变。故只选样品的高剂量组和阴性对照组动物的主要脏器进行组织病理切片检查,结果见表18~表24。结果显示,高剂量组有1只雄性、对照组有1只雄性和1只雌性大鼠的肝小叶可见肝细胞空泡变性;高剂量组有1只雄性和1只雌性、对照组有1只雄性和2只雌性大鼠的肝小叶可见肝细胞点状坏死;高剂量组和对照组各有1只雄性和2只雌性大鼠的肝脏汇管区可见少量炎细胞浸润。高剂量组有2只雄性和1只雌性、对照组有1只雄性和1只雌性大鼠的肾脏皮质部间质可见少量炎细胞浸润。以上组织病变属动物的自发轻型病变,且两组动物的组织病变程度相似,故可以排除是样品所致,其他脏器组织未见病理组织学改变,表明该样品对大鼠的上述脏器组织无损害作用。
At the end of the experiment, the animals were dissected, and no obvious lesions were observed in the animals in each group. Therefore, only the high-dose group of the sample and the main organs of the negative control group were examined for histopathological examination. The results are shown in Table 18 to Table 24. The results showed that 1 male in the high-dose group and 1 male and 1 female in the control group showed hepatocyte vacuolar degeneration in the hepatic lobules; 1 male and 1 female in the high-dose group and 1 in the control group. Hepatocyte dot necrosis was observed in the hepatic lobules of male and 2 female rats; a small amount of inflammatory cell infiltration was observed in the liver portal area of one male and two female rats in the high-dose group and the control group. In the high-dose group, there were 2 males and 1 female, and 1 male and 1 female rats in the control group showed a small amount of inflammatory cell infiltration in the renal cortex. The above tissue lesions belong to the spontaneous mild lesions of the animals, and the degree of tissue lesions of the two groups of animals is similar, so it can be ruled out by the sample, and no histopathological changes are observed in other organs, indicating that the sample is the above organ tissues of the rats. No damage.
3结论:3 Conclusion:
以20000mg/kg BW剂量的本发明样品给予小鼠灌胃后,未见动物有中毒症状和死亡,本发明样品对小鼠的急性经口毒性MTD大于20000mg/kg BW,急性经口毒性属无毒级。30天喂养试验(慢性毒性试验):以5000、2500、1250mg/kgBW(分别相当于人体推荐用量100、50、25倍)3个剂量的样品连续给大鼠灌胃30天,实验期间动物的生长发育良好,各剂量组的动物体重、增重量、进食量、食物利用率、血常规指标、血生化指标、脏器重量及脏器/体重比值与对照组比较,均无显著性差异(P>0.05);大体解剖观察和组织病理学检查未见与样品有关的异常改变。在受试剂量范围内未见该样品对大鼠各项观察指标产生毒副作用。After administration of the sample of the present invention at a dose of 20,000 mg/kg BW to the mice, no symptoms of poisoning and death were observed in the animals. The acute oral toxicity of the samples of the present invention to the mice was greater than 20000 mg/kg BW, and the acute oral toxicity was none. Toxic level. 30-day feeding test (chronic toxicity test): Rats were continuously administered with a dose of 5000, 2500, 1250 mg/kg BW (100, 50, 25 times recommended by the human body, respectively) for 30 days. Animals during the experiment The growth and development were good. There was no significant difference in body weight, weight gain, food intake, food utilization rate, blood routine index, blood biochemical index, organ weight and organ/body weight ratio of the animals in each dose group. >0.05); gross anatomical observation and histopathological examination showed no abnormal changes associated with the sample. The sample was not seen to have toxic side effects on various observation indexes of the rats within the range of the amount of the reagent.
三项遗传毒性试验:Three genotoxicity tests:
1.Ames试验1.Ames test
1.1方法:采用经鉴定符合要求的鼠伤寒沙门氏菌组氨酸缺陷型TA97a、TA98、TA100、TA102四种菌株进行试验。称取5.0g本发明样品,加纯水至100mL,混匀,配成50mg/mL浓度溶液,再依次5倍稀释(取10mL加纯水至50mL),分别配成10、2、0.4、0.08mg/mL浓度溶液,受试溶液经高压灭菌(0.103Mpa 20min)处理后供试验用。以多氯联苯诱导的大鼠肝微粒体酶(S-9)作为体外代谢活化系统。采用平板掺入法,在保温的顶层培养基中依次加入0.1mL试验菌株增菌液、0.1mL受试物溶液和0.5mL S-9混合液(当需要代谢活化时),混匀后倒入底层培养基平板上。5个试验剂量分别为5000、1000、200、40、8μg/皿,同时设自发回变对照、溶剂对照和阳性突变剂对照。自发回变对照除不加样品外,其余条件与样品组相同。溶剂对照用灭菌纯水替代样品,其余条件与样品组相同。每个剂量组的各种菌株均做3个平行皿。在37℃下培养48小时,计数每皿的菌落数。整套试验在相同条件下重复做两次。如果受试物的回变菌落数增加超过自发回变菌落数的2倍以上,并具有剂量-反应关系者,即为诱变试验阳性。1.1 Method: The strains of Salmonella typhimurium histidine-deficient strains TA97a, TA98, TA100 and TA102 which were identified to meet the requirements were tested. Weigh 5.0g of the sample of the invention, add pure water to 100mL, mix well, prepare a 50mg/mL concentration solution, and then dilute it 5 times (take 10mL plus pure water to 50mL), respectively, and make 10, 2, 0.4, 0.08 The solution of mg/mL concentration is treated by autoclaving (0.103Mpa 20min) for testing. Polychlorinated biphenyl-induced rat liver microsomal enzyme (S-9) was used as an in vitro metabolic activation system. Using the plate incorporation method, 0.1 mL of the test strain enrichment solution, 0.1 mL of the test solution and 0.5 mL of the S-9 mixture (when metabolic activation is required) are sequentially added to the maintained top culture medium, and then mixed and poured. On the bottom medium plate. The five test doses were 5000, 1000, 200, 40, and 8 μg/dish, respectively, with spontaneous reversion control, solvent control, and positive mutagen control. The spontaneous reversal control was the same as the sample group except that no sample was added. The solvent control replaced the sample with sterile pure water, and the rest of the conditions were the same as the sample group. Each strain of each dose group was made into 3 parallel dishes. The cells were cultured at 37 ° C for 48 hours, and the number of colonies per dish was counted. The entire set of tests was repeated twice under the same conditions. If the number of revertant colonies of the test substance increases more than twice the number of spontaneously reverted colonies and has a dose-response relationship, the mutagenesis test is positive.
1.2结果:对TA97a、TA98、TA100、TA102四种试验菌株,无论是否加入S-9,样品各剂量组的回变菌落数均未超过自发回变菌落数的两倍,亦无剂量-反应关系,表明本发明物诱变试验结果为阴性。1.2 Results: For the four test strains of TA97a, TA98, TA100 and TA102, the number of revertant colonies in each dose group did not exceed twice the number of spontaneously reverted colonies, and there was no dose-response relationship. It indicates that the mutagenesis test result of the present invention is negative.
2.小鼠骨髓细胞微核试验2. Micronucleus test of mouse bone marrow cells
2.1方法:采用间隔24小时两次经口灌胃法进行试验。选体重为25~30g
的昆明种小鼠50只,随机分成5组,每组10只,雌雄各半。试验组3个剂量分别设10000、5000、2500mg/kg BW,以纯水为阴性对照,40mg/kg BW剂量的环磷酰胺(cp)作阳性对照。分别称取20.0、10.0、5.0g样品,各加纯水至40mL,混匀,配成500、250、125mg/mL浓度混悬液,然后按0.4mL/20g BW的体积给动物灌胃,阴性对照组灌给等体积的纯水,阳性对照组灌给等体积的2mg/mL环磷酰胺溶液。第二次给样后6小时颈椎脱臼处死动物,取胸骨骨髓用小牛血清稀释涂片,甲醇固定,Giemsa染色。在光学显微镜下,每只动物计数1000个嗜多染红细胞(PCE),观察含微核的PCE数,微核率以含微核的PCE千分率计;同时计数200个嗜多染红细胞,计算嗜多染红细胞与成熟红细胞的比值(PCE/NCE)。应用SPSS统计软件中的泊松分布均数比较法统计处理。如试验组的微核率比阴性对照组增高,并有明显的剂量-反应关系和统计学意义,即为阳性结果。2.1 Method: The test was carried out by oral gavage twice at intervals of 24 hours. Choose a weight of 25 ~ 30g
50 Kunming mice were randomly divided into 5 groups, 10 in each group, half male and half female. The three doses in the experimental group were 10000, 5000, 2500 mg/kg BW, respectively, with pure water as the negative control and 40 mg/kg BW dose of cyclophosphamide (cp) as the positive control. Weigh 20.0, 10.0, 5.0g samples, add pure water to 40mL, mix well, prepare 500, 250, 125mg/mL concentration suspension, then weigh the animals according to the volume of 0.4mL/20g BW, negative The control group was given an equal volume of pure water, and the positive control group was given an equal volume of 2 mg/mL cyclophosphamide solution. The animals were sacrificed by cervical dislocation 6 hours after the second administration. The scaphoid bone marrow was diluted with calf serum, fixed with methanol, and stained with Giemsa. Under the light microscope, 1000 polychromatic red blood cells (PCE) were counted per animal, and the number of PCEs containing micronuclei was observed. The micronucleus rate was calculated as the micronucleus-containing PCE per thousand; and 200 polychromatic red blood cells were counted at the same time. The ratio of polychromatic red blood cells to mature red blood cells (PCE/NCE) was calculated. The statistical processing was performed by using the Poisson distribution mean comparison method in the SPSS statistical software. For example, the micronucleus rate of the experimental group was higher than that of the negative control group, and there was a significant dose-response relationship and statistical significance, which was a positive result.
2.2结果:本发明样品各剂量组小鼠的骨髓细胞微核率与阴性对照组比较,差异均无显著性(P>0.05),各剂量组PCE/NCE值均不少于阴性对照组的20%,与阴性对照组比较也无明显差异,而环磷酰胺阳性对照组的微核率与阴性对照组的差异有非常显著性(P<0.01),提示未见本发明样品对小鼠的骨髓细胞有损伤和抑制作用。2.2 Results: The micronucleus rate of bone marrow cells of mice in each dose group of the present invention was not significantly different from that of the negative control group (P>0.05), and the PCE/NCE values of each dose group were not less than that of the negative control group. %, there was no significant difference compared with the negative control group, and the micronucleus rate of the cyclophosphamide positive control group was significantly different from that of the negative control group (P<0.01), suggesting that the bone marrow of the sample of the present invention was not observed. The cells have damage and inhibition.
3.小鼠精子畸形试验3. Mouse sperm abnormality test
3.1方法:选体重为25~35g的昆明种雄性小鼠50只,随机分成5组,每组10只。试验组3个剂量分别设10000、5000、2500mg/kg BW,以纯水为阴性对照,40mg/kgBW剂量的环磷酰胺(cp)作阳性对照。分别称取20.0、10.0、5.0g样品,各加纯水至40mL,混匀,配成500、250、125mg/mL浓度混悬液,然后按0.4mL/20g BW的体积给动物灌胃,阴性对照组灌给等体积的纯水,阳性对照组灌给等体积的2mg/mL环磷酰胺溶液。每天灌胃一次,连续5天。末次给样后第30天处死动物,取副睾的精子涂片,甲醇固定,伊红染色。在光学显微镜下,每只动物计数完整精子1000个,计算精子畸形率。应用SPSS统计软件中的Wilcoxon秩和检验统计处理。如试验组的精子畸形率比阴性对照组增高,经统计有显著意义,并有剂量反应关系,即为阳性结果。3.1 Methods: 50 Kunming male mice weighing 25-35 g were randomly divided into 5 groups, 10 in each group. The three doses in the experimental group were 10000, 5000, 2500 mg/kg BW, respectively, with pure water as the negative control and 40 mg/kg BW dose of cyclophosphamide (cp) as the positive control. Weigh 20.0, 10.0, 5.0g samples, add pure water to 40mL, mix well, prepare 500, 250, 125mg/mL concentration suspension, then weigh the animals according to the volume of 0.4mL/20g BW, negative The control group was given an equal volume of pure water, and the positive control group was given an equal volume of 2 mg/mL cyclophosphamide solution. Gavage once a day for 5 consecutive days. The animals were sacrificed on the 30th day after the last dose, and the sperm smears of the epididymis were taken, fixed by methanol, and stained with eosin. Under an optical microscope, 1000 sperm counts were counted per animal, and the rate of sperm deformity was calculated. Wilcoxon rank sum test statistical processing in SPSS statistical software was applied. For example, the sperm deformity rate of the experimental group was higher than that of the negative control group, and it was statistically significant, and there was a dose-response relationship, which was a positive result.
3.2结果:本发明样品对小鼠精子畸形发生率未产生明显改变,样品各剂量组的精子畸形率与阴性对照组比较,差异均无显著性(P>0.05),而环磷酰胺
阳性对照组与阴性对照组的差异有非常显著性(P<0.01),提示未见本发明样品对雄性小鼠的精子产生畸变作用。3.2 Results: The sample of the present invention did not significantly change the incidence of sperm abnormality in mice. The sperm deformity rate of each sample group was not significantly different from that of the negative control group (P>0.05), while cyclophosphamide was not significantly different (P>0.05).
The difference between the positive control group and the negative control group was very significant (P<0.01), suggesting that the sperm of the present invention did not cause spermatogenesis in male mice.
4.结论:4 Conclusion:
三项遗传毒性试验(Ames试验、小鼠骨髓细胞微核试验、小鼠精子畸形试验)结果均为阴性。表明本发明物无遗传毒性。Three genotoxicity tests (Ames test, mouse bone marrow micronucleus test, mouse sperm abnormality test) were negative. This indicates that the present invention is not genotoxic.
上述试验研究证实本发明提供的保健食品具有明显的降血糖保健作用,且安全无毒福作用。The above experimental research confirmed that the health food provided by the invention has obvious hypoglycemic health-care effect, and is safe and non-toxic.
所属领域的普通技术人员应当理解:以上任何实施例的讨论仅为示例性的,并非旨在暗示本公开的范围(包括权利要求)被限于这些例子;在本发明的思路下,以上实施例或者不同实施例中的技术特征之间也可以进行组合,并存在如上所述的本发明的不同方面的许多其它变化,为了简明它们没有在细节中提供。因此,凡在本发明的精神和原则之内,所做的任何省略、修改、等同替换、改进等,均应包含在本发明的保护范围之内。
It should be understood by those of ordinary skill in the art that the discussion of any of the above embodiments is merely exemplary, and is not intended to suggest that the scope of the disclosure (including the claims) is limited to these examples; Combinations of the technical features in the different embodiments are also possible, and there are many other variations of the various aspects of the invention as described above, which are not provided in the details for the sake of brevity. Therefore, any omissions, modifications, equivalents, improvements, etc., which are within the spirit and scope of the invention, are intended to be included within the scope of the invention.
Claims (10)
- 一种保健食品,其特征在于,所述保健食品的有效成分由以下中药原料按重量份组成:A health food product, characterized in that the active ingredient of the health food product is composed of the following traditional Chinese medicine raw materials in parts by weight:5~30份葛根;5 to 30 parts of pueraria;2~20份绞股蓝;2 to 20 strands of Gynostemma pentaphyllum;0.5~8份三七;0.5 to 8 parts of Sanqi;1~20份桑椹子;1 to 20 parts of mulberry;1~10份文蛤肉;和1 to 10 pieces of meat; and2~20份螺旋藻。2 to 20 parts of spirulina.
- 根据权利要求1所述的保健食品,其特征在于,所述保健食品的有效成分由以下中药原料按重量份配比组成:The health food according to claim 1, wherein the active ingredient of the health food is composed of the following traditional Chinese medicine raw materials in a weight ratio:7~25份葛根;7 to 25 parts of Pueraria;5~15份绞股蓝;5 to 15 parts of Gynostemma pentaphyllum;1~5份三七;1 to 5 copies of Sanqi;4~15份桑椹子;4 to 15 parts of mulberry;2~8份文蛤肉;和2 to 8 pieces of meat; and4~15份螺旋藻。4 to 15 parts of spirulina.
- 一种保健食品,其特征在于,所述保健食品的有效成分由以下中药原料按重量份组成:A health food product, characterized in that the active ingredient of the health food product is composed of the following traditional Chinese medicine raw materials in parts by weight:5~30份葛根的提取物;5 to 30 parts of Pueraria extract;2~20份绞股蓝的提取物;2 to 20 parts of Gynostemma pentaphyllum extract;0.5~8份三七的提取物;0.5 to 8 parts of the extract of Panax notoginseng;1~20份桑椹子的提取物;1 to 20 parts of the extract of mulberry;1~10份文蛤肉的提取物;和1 to 10 extracts of clam meat; and2~20份螺旋藻的提取物。2 to 20 parts of spirulina extract.
- 根据权利要求3所述的保健食品,其特征在于,所述保健食品的有效成分由以下中药原料按重量份配比组成:The health food according to claim 3, wherein the active ingredient of the health food is composed of the following traditional Chinese medicine raw materials in a weight ratio:7~25份葛根的提取物;7 to 25 parts of Pueraria extract;5~15份绞股蓝的提取物;5 to 15 parts of Gynostemma pentaphyllum extract;1~5份三七的提取物; 1 to 5 parts of the extract of Panax notoginseng;4~15份桑椹子的提取物;4 to 15 parts of the extract of mulberry;2~8份文蛤肉的提取物;和2 to 8 extracts of clam meat; and4~15份螺旋藻的提取物。4 to 15 parts of Spirulina extract.
- 一种如权利要求1~4中任意一项所述的保健食品,所述保健食品可用于制备具有降血糖作用的保健食品或药物,可以制成口服固体、半固体或口服液体等任意剂型,且安全无毒副作用。A health food according to any one of claims 1 to 4, which can be used for preparing a health food or a medicine having hypoglycemic action, and can be prepared into any dosage form such as oral solid, semi-solid or oral liquid. And safe and non-toxic side effects.
- 一种如权利要求1~4中任意一项所述的保健食品的制备方法,其特征在于,包括以下步骤:A method for preparing a health food according to any one of claims 1 to 4, comprising the steps of:将葛根和绞股蓝混合,先加酒精进行回流提取,然后浓缩、干燥,再粉碎得到提取物Ⅰ;Mixing Pueraria and Gynostemma pentaphyllum, first adding alcohol for reflux extraction, then concentrating, drying, and then pulverizing to obtain extract I;将桑椹子、文蛤肉和螺旋藻混合后,先加水进行沸腾提取,然后浓缩,再浓缩物中加入乙醇,过滤后取沉淀物,干燥、粉碎后得到提取物Ⅱ;After mixing mulberry, clam meat and spirulina, first add water for boiling extraction, then concentrate, add ethanol to the concentrate, filter and take the precipitate, dry and pulverize to obtain extract II;将三七打成粉,得到三七粉;Beat the three seven into powder to get the notoginseng powder;将提取物Ⅰ、提取物Ⅱ和三七粉混合,得到所述保健食品。The extract I, the extract II and the notoginseng powder were mixed to obtain the health food.
- 根据权利要求1所述的保健食品的制备方法,其特征在于,所述提取物Ⅰ的制备方法包括以下步骤:The method for preparing a health food according to claim 1, wherein the method for preparing the extract I comprises the following steps:将葛根和绞股蓝混合,先加酒精进行回流提取,每次加入6~10倍量的酒精,每次提取1~2小时,共提取1~4次,合并提取液后浓缩、干燥,干燥温度为80~90℃,粉碎过80~120目筛,得到提取物Ⅰ。Mix Pueraria and Gynostemma pentaphyllum, first add alcohol for reflux extraction, add 6-10 times of alcohol each time, extract for 1 to 2 hours each time, extract 1~4 times, combine the extracts, concentrate and dry, and dry at 80 to 90 ° C, pulverized through 80 to 120 mesh sieve to obtain extract I.
- 根据权利要求7所述的保健食品的制备方法,其特征在于,所述提取物Ⅰ的制备方法包括以下步骤:The method for preparing a health food according to claim 7, wherein the method for preparing the extract I comprises the following steps:将葛根和绞股蓝混合,第一次加6~10倍量的酒精,先浸泡30~60min后,回流提取,第二次加6~8倍量的酒精,每次提取1~2小时,合并提取液后浓缩、干燥,干燥温度为80~90℃,粉碎过80~120目筛,得到提取物Ⅰ。Mix Pueraria and Gynostemma pentaphyllum, add 6-10 times of alcohol for the first time, soak for 30~60min, then extract by reflux, add 6~8 times of alcohol for the second time, extract for 1~2 hours each time, combine and extract The solution was concentrated, dried, dried at a temperature of 80 to 90 ° C, and pulverized through a sieve of 80 to 120 mesh to obtain an extract I.
- 根据权利要求6所述的保健食品的制备方法,其特征在于,所述提取物Ⅱ的制备方法包括以下步骤:The method for preparing a health food according to claim 6, wherein the method for preparing the extract II comprises the following steps:将桑椹子、文蛤肉和螺旋藻混合,先加水进行沸腾提取,共提取1~4次,每次加6~10倍量的水,每次提取1~2小时,合并煎液后浓缩;Mix mulberry, clam meat and spirulina, first add water for boiling extraction, extract 1~4 times, add 6~10 times of water each time, extract for 1~2 hours each time, combine the decoction and concentrate;向浓缩液中加入乙醇沉淀16~30小时,过滤后取沉淀物,干燥、粉碎后得到提取物Ⅱ。 Ethanol precipitation was added to the concentrate for 16 to 30 hours, and the precipitate was taken after filtration, dried and pulverized to obtain Extract II.
- 根据权利要求9所述的保健食品的制备方法,其特征在于,所述提取物Ⅱ的制备方法包括以下步骤:The method for preparing a health food according to claim 9, wherein the method for preparing the extract II comprises the following steps:先将文蛤肉加水浸泡12~24小时后,再与桑椹子和螺旋藻混合,第一次加6~10倍量的水,先浸泡30~60min后,加热至沸腾提取,第二次加5~9倍量的水,每次提取1~2小时,合并煎液后浓缩;Soak the meat with water for 12 to 24 hours, then mix with mulberry and spirulina. Add 6 to 10 times of water for the first time. Soak for 30 to 60 minutes, then heat to boiling extraction. Add 5 for the second time. ~ 9 times the amount of water, each extraction for 1 to 2 hours, combined with decoction and concentrated;向浓缩液中加入体积浓度为80~95%的乙醇至乙醇的体积浓度为70~90%,然后沉淀16~30小时,过滤后取沉淀物,60~75℃干燥、粉碎过80~120目筛,得到提取物Ⅱ。 To the concentrate, a volume concentration of 80 to 95% of ethanol to ethanol is added to a volume concentration of 70 to 90%, and then precipitation is carried out for 16 to 30 hours. After filtration, the precipitate is taken, dried at 60 to 75 ° C, and pulverized through 80 to 120 mesh. Sieve to obtain extract II.
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| CN107897613A (en) * | 2017-10-25 | 2018-04-13 | 宁国平衡健康管理有限公司 | A kind of health food of blood pressure lowering and preparation method thereof |
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| CN101879278A (en) * | 2010-06-24 | 2010-11-10 | 武汉市健恒生物科技有限责任公司 | Medicine composition with hyperglycemic function, and preparation method and application thereof |
| CN102526264A (en) * | 2012-01-04 | 2012-07-04 | 山东省中医药研究院 | Chinese medicinal preparation with blood fat reducing effect and preparation method thereof |
| CN102552635A (en) * | 2012-03-20 | 2012-07-11 | 广西中医学院 | Health-care food with hypoglycemic function and preparation method thereof |
| CN104311630A (en) * | 2014-09-25 | 2015-01-28 | 广西中医药大学 | Clam bioactive peptide and its extraction method and use |
| CN104336596A (en) * | 2013-08-01 | 2015-02-11 | 陕西百年健康药业有限公司 | Medicine composition capable of lowering blood lipid and preparation method thereof |
| CN104522664A (en) * | 2014-12-29 | 2015-04-22 | 广西中医药大学 | Health food with capability of improving immunity and preparation method of health food |
| CN104997878A (en) * | 2015-08-18 | 2015-10-28 | 北京挚诚科技发展有限公司 | Auxiliary blood pressure and blood fat reducing health product and preparation process thereof |
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| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN101879278A (en) * | 2010-06-24 | 2010-11-10 | 武汉市健恒生物科技有限责任公司 | Medicine composition with hyperglycemic function, and preparation method and application thereof |
| CN102526264A (en) * | 2012-01-04 | 2012-07-04 | 山东省中医药研究院 | Chinese medicinal preparation with blood fat reducing effect and preparation method thereof |
| CN102552635A (en) * | 2012-03-20 | 2012-07-11 | 广西中医学院 | Health-care food with hypoglycemic function and preparation method thereof |
| CN104336596A (en) * | 2013-08-01 | 2015-02-11 | 陕西百年健康药业有限公司 | Medicine composition capable of lowering blood lipid and preparation method thereof |
| CN104311630A (en) * | 2014-09-25 | 2015-01-28 | 广西中医药大学 | Clam bioactive peptide and its extraction method and use |
| CN104522664A (en) * | 2014-12-29 | 2015-04-22 | 广西中医药大学 | Health food with capability of improving immunity and preparation method of health food |
| CN104997878A (en) * | 2015-08-18 | 2015-10-28 | 北京挚诚科技发展有限公司 | Auxiliary blood pressure and blood fat reducing health product and preparation process thereof |
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