Composition for Promoting Anti-Diabetic and Anti-Obesity Effects, Comprising Herbal Extract
20170239310 · 2017-08-24
Inventors
Cpc classification
A61K2300/00
HUMAN NECESSITIES
A61K2300/00
HUMAN NECESSITIES
A61K31/155
HUMAN NECESSITIES
International classification
Abstract
The present invention relates to a composition for improving anti-diabetic and anti-obesity effects, including an extract extracted from any one selected from the group consisting of Lonicera japonica (Lonicerae Flos), Scutellaria baicalensis (Scutellariae Radix), and Houttuynia cordata (Houttuyniae Herba). According to the present invention, it was confirmed that co-administration of the extract of the present invention and metformin, a representative anti-diabetic drug, increases an anti-diabetic effect and reduces side effects caused by metformin, and at the same time, exhibits an anti-obesity effect by suppressing fat accumulation. Therefore, the composition of the present invention is expected to be effective in treatment of diabetes mellitus.
Claims
1-6. (canceled)
7. A method of improving anti-diabetic effect, the method comprising a step of administering an extract extracted from any one selected from the group consisting of Lonicera japonica (Lonicerae Flos), Scutellaria baicalensis (Scutellariae Radix), and Houttuynia cordata (Houttuyniae Herba) to an individual.
8. A method of treating diabetes mellitus, the method comprising a step of administering an extract extracted from any one selected from the group consisting of Lonicera japonica (Lonicerae Flos), Scutellaria baicalensis (Scutellariae Radix), and Houttuynia cordata (Houttuyniae Herba) to an individual.
9. (canceled)
10. The method according to claim 7, wherein the extract is administrated simultaneously with or separately from the anti-diabetic drug, or the pharmaceutical composition and the anti-diabetic drug are administrated sequentially.
11. The method according to claim 7, wherein the method inhibits differentiation of fat cells.
12. The method according to claim 7, wherein the extract is extracted using one or more solvents selected from the group consisting of water, alcohols having 1 to 4 carbons, and a combination thereof.
13. The method according to claim 7, wherein the method increases expression levels of one or more selected from the group consisting of phosphorylated AMP-activated protein kinase (p-AMPK) and genes encoding sirtuin 1 (SirT1), AMP-activated protein kinase-alpha (AMPK-α), peroxisome proliferator-activated receptor-alpha (PPAR-α), and peroxisome proliferator-activated receptor-gamma (PPAR-γ), respectively.
14. The method according to claim 7, wherein method decreases expression levels of one or more selected from the group consisting of genes encoding X-box binding protein 1 (XBP-1), tumor necrosis factor-alpha (TNF-α), and interleukin-6 (IL-6), respectively.
15. The method according to claim 8, wherein the extract is administrated simultaneously with or separately from the anti-diabetic drug, or the pharmaceutical composition and the anti-diabetic drug are administrated sequentially.
16. The method according to claim 8, wherein the extract inhibits differentiation of fat cells.
17. The method according to claim 8, wherein the extract is extracted using one or more solvents selected from the group consisting of water, alcohols having 1 to 4 carbons, and a combination thereof.
18. The method according to claim 8, wherein the method increases expression levels of one or more selected from the group consisting of phosphorylated AMP-activated protein kinase (p-AMPK) and genes encoding sirtuin 1 (SirT1), AMP-activated protein kinase-alpha (AMPK-α), peroxisome proliferator-activated receptor-alpha (PPAR-α), and peroxisome proliferator-activated receptor-gamma (PPAR-γ), respectively.
19. The method according to claim 8, wherein the method decreases expression levels of one or more selected from the group consisting of genes encoding X-box binding protein 1 (XBP-1), tumor necrosis factor-alpha (TNF-α), and interleukin-6 (IL-6), respectively.
Description
BRIEF DESCRIPTION OF DRAWINGS
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BEST MODE FOR CARRYING OUT THE INVENTION
[0085] In the present invention, it was confirmed that combined use of an extract extracted from any one selected from the group consisting of Lonicera japonica (Lonicerae Flos), Scutellaria baicalensis (Scutellariae Radix), and Houttuynia cordata (Houttuyniae Herba) and metformin increases the protein expression level of phosphorylated AMP-activated protein kinase (p-AMPK) and the gene expression levels of sirtuin 1 (SirT1), AMP-activated protein kinase-alpha (AMPK-α), peroxisome proliferator-activated receptor-alpha (PPAR-α), and peroxisome proliferator-activated receptor-gamma (PPAR-γ), which are associated with an anti-diabetic effect and an inhibitory effect on fat accumulation. In addition, it was confirmed that the combined use decreases the gene expression levels of X-box binding protein 1 (XBP-1), tumor necrosis factor-alpha (TNF-α), and interleukin-6 (IL-6), which are associated with the side effects of metformin. The present invention was completed on the basis thereof.
[0086] Hereinafter, the present invention will be described in detail.
[0087] It is an objective of the present invention to provide a pharmaceutical composition for improving an anti-diabetic effect, which is used in combination with metformin, an anti-diabetic drug, and includes an extract extracted from any one selected from the group consisting of Lonicera japonica (Lonicerae Flos), Scutellaria baicalensis (Scutellariae Radix), and Houttuynia cordata (Houttuyniae Herba).
[0088] In the present invention, the extracts may be extracted according to general methods of extracting extracts from natural products, which are known in the art, i.e., using general solvents under general temperature and pressure conditions. For example, in the present invention, a Houttuynia cordata extract may be extracted using, preferably ethanol, one or more solvents selected from the group consisting of water, alcohols having 1 to 4 carbons, and a combination thereof. In addition, extracts may be extracted from Houttuynia cordata using various methods such as hot water extraction, cold extraction, reflux extraction, and ultrasonic extraction, without being limited thereto.
[0089] The solvents may be removed from the prepared extracts by performing a filtration, concentration, or drying process or by performing all of filtration, concentration, and drying processes after finishing an extraction process. For example, the filtration process may be performed using a filter paper or a vacuum filter, the concentration process may be performed using a vacuum concentrator, and the drying process may be performed using a freeze-drying method and the like, without being limited thereto.
[0090] In addition, the extracts extracted by the solvents may be further subjected to a fractionation process using a solvent selected from the group consisting of hexane, methylene chloride, acetone, ethyl acetate, ethyl ether, chloroform, water and a mixture thereof. The fractionation may be performed at 4 to 120° C., but the present invention is not limited thereto.
[0091] The term “treatment” used in the present invention refers to all actions that improve the symptoms of diabetes mellitus or advantageously change the state of a diabetic patient by administration of a pharmaceutical composition according to the present invention.
[0092] “Diabetes mellitus”, a chronic metabolic disease that is an object to be prevented or treated by the composition of the present invention, can cause vascular disorders and malfunction of nerves, kidneys and retinas and the like over time, which may lead to loss of life. Diabetes mellitus, depending on generation mechanisms, is broadly divided into insulin-dependent diabetes mellitus (type 1 diabetes mellitus) and insulin-independent diabetes mellitus (type 2 diabetes mellitus), and in the present invention, diabetes mellitus preferably refers to insulin-independent diabetes mellitus. Generally, insulin-independent diabetes mellitus exhibits insulin resistance, and in an individual with diabetes mellitus, a high blood sugar level is maintained due to the failure of insulin action. Since chronic high blood sugar can cause cell death by damaging pancreatic beta-cells, effective regulation of blood sugar levels is needed when treating individuals with type 2 diabetes mellitus.
[0093] Gliclazide, glibenclamide, repaglinide, nateglinide, mitiglinide, rosiglitazone, pioglitazone, acarbose, voglibose and the like, preferably metformin, may be an anti-diabetic drug used in combination with the composition of the present invention, but the invention is not limited thereto.
[0094] For example, “metformin”, which is used as an anti-diabetic drug in the present invention, belongs to the biguanide class and has been used as a drug for primary treatment of patients with type 2 diabetes mellitus. However, use of metformin can cause side effects, such as loss of appetite, abdominal distension, nausea, diarrhea, and skin rashes, and thus special attention should be paid when using metformin.
[0095] Accordingly, to improve an anti-diabetic effect and decrease side effects of the anti-diabetic drug, the composition according to the present invention may be administrated simultaneously with or separately from the anti-diabetic drug, or the composition and the anti-diabetic drug may be administrated sequentially.
[0096] In addition, the composition according to the present invention may improve an anti-diabetic effect and at the same time, prevent or treat obesity.
[0097] “Obesity”, a disease that is an object to be prevented or treated by the composition of the present invention, refers to a condition in which excessive fat is accumulated in the body, which is attributed to proliferation and differentiation of fat cells due to metabolic disorders. When energy absorption is increased relative to energy consumption, the number and volume of fat cells are increased and consequently the mass of fat tissues is increased. Obesity at the cellular level refers to the increase in the number and volume of fat cells due to promotion of proliferation and differentiation of fat cells.
[0098] Obesity is closely associated with increase of insulin resistance, which is a major pathophysiological feature of type 2 diabetes mellitus. Insulin resistance, a condition in which blood sugar levels are not reduced despite a large amount of injected insulin, refers to a decrease in insulin sensitivity. It has been known that such decrease in insulin sensitivity is attributed to accumulation of fatty acids in beta-cells or insulin sensitive tissues such as the kidney, liver, and heart due to irregular secretion of adipokines and free fatty acids and consequent lipotoxicity.
[0099] In addition, the pharmaceutical composition according to the present invention may increase expression levels of one or more selected from the group consisting of phosphorylated AMP-activated protein kinase (p-AMPK) and genes encoding sirtuin 1 (SirT1), AMP-activated protein kinase-alpha (AMPK-α), peroxisome proliferator-activated receptor-alpha (PPAR-α), and peroxisome proliferator-activated receptor-gamma (PPAR-γ), respectively.
[0100] p-AMPK, SirT1, AMPK-α, PPAR-α and PPAR-γ, described above, are proteins that are associated with anti-diabetic effects and inhibitory effects on fat accumulation. AMP-activated protein kinase (AMPK) is activated when intracellular energy is deficient (i.e., when the amount of AMP is increased relative to the amount of ATP), and then the activated AMPK stimulates production of ATP, in which the synthesis of fatty acids, cholesterol, and the like is inhibited, whereas ATP is produced, i.e., the processes of fatty acid oxidation and glycolysis, resulting in restored normal energy balance. SirT1 has a deacetylase activity toward histone proteins and various transcription factors associated with cell growth, stress responses, endocrine regulation and the like. In addition, PPAR-α regulates the metabolism of glycolipids involved in lipolysis of neutral fat, and has a role in reducing triglyceride (TG) levels by activating lipoprotein lipase (LPL). PPAR-γ, one of transcriptional regulators in fat cells, has an important role in improving insulin sensitivity as well as a role in regulating the expression levels of enzymes responsible for differentiation of fat cells and fat synthesis/storage.
[0101] In addition, the composition according to the present invention may decrease expression levels of one or more selected from the group consisting of genes encoding X-box binding protein 1 (XBP-1), tumor necrosis factor-alpha (TNF-α), and interleukin-6 (IL-6), respectively.
[0102] The XBP-1, TNF-α and IL-6, described above, are proteins involved in the side effects of metformin. The XBP-1 is involved in endoplasmic reticulum stress, and the TNF-α and IL-6, as inflammatory cytokines involved in stimulating M2 macrophages, have roles in increasing inflammatory responses.
[0103] In one embodiment of the present invention, it was confirmed when a Lonicera japonica extract is administered alone or the Lonicera japonica extract and metformin are co-administered, cytotoxicity was not observed. In addition, it was experimentally confirmed that co-administration of the Lonicera japonica extract and metformin reduces intracellular reactive oxygen species, removes free radicals, inhibits nitrogen monoxide generation, and suppresses differentiation of fat cells (see Examples 1 to 5). In addition, it was confirmed that co-administration of the Lonicera japonica extract and metformin increases glucose uptake and insulin secretion and improves insulin resistance, and the co-administration inhibited the protein expression level of DPP-4 while increasing the protein expression levels of PPAR-γ, p-AMPK, and SirT1 (see Examples 6 to 9). In addition, it was confirmed that the co-administration improves an anti-diabetic effect and inhibits fat accumulation by increasing the gene expression levels of AMPK-α, PPAR-α, and PPAR-γ and decreases side effects caused by metformin by decreasing the gene expression levels of XBP-1, TNF-α, and IL-6. And it was confirmed, through in vivo animal experiments, that the co-administration decreases insulin resistance while not affecting the pharmacokinetic properties of metformin (see Examples 10 to 12).
[0104] In addition, in one embodiment of the present invention, it was confirmed when a Scutellaria baicalensis extract is administered alone or the Scutellaria baicalensis extract and metformin are co-administered, cytotoxicity was not observed. In addition, it was experimentally confirmed that co-administration of the Scutellaria baicalensis extract and metformin reduces intracellular reactive oxygen species, removes free radicals, inhibits nitrogen monoxide generation, and suppresses differentiation of fat cells (see Examples 13 to 17). In addition, it was confirmed that the co-administration increases glucose uptake and the protein expression levels of PPAR-γ and AMPK (see Examples 18 to 19). In addition, it was confirmed that the co-administration improves an anti-diabetic effect and inhibits fat accumulation by increasing the gene expression levels of AMPK-α and PPAR-α and decreases side effects caused by metformin by decreasing the gene expression levels of XBP-1, TNF-α, and IL-6. And it was confirmed, through in vivo animal experiments, that the co-administration decreases insulin resistance while not affecting the pharmacokinetic properties of metformin (see Examples 20 to 22).
[0105] In addition, in one embodiment of the present invention, it was confirmed when a Houttuynia cordata extract is administered alone or the Houttuynia cordata extract and metformin are co-administered, cytotoxicity was not observed. In addition, it was experimentally confirmed that co-administration of the Houttuynia cordata extract and metformin reduces intracellular reactive oxygen species, removes free radicals, inhibits nitrogen monoxide generation, and suppresses differentiation of fat cells (see Examples 23 to 27). In addition, it was confirmed that co-administration of the Houttuynia cordata extract and metformin increases glucose uptake and insulin secretion and improves insulin resistance, and the co-administration inhibited the protein expression level of DPP-4 while increasing the protein expression levels of PPAR-γ and AMPK (see Examples 28 to 31). In addition, it was confirmed that the co-administration improves an anti-diabetic effect and inhibits fat accumulation by increasing the gene expression levels of AMPK-α, PPAR-α, and PPAR-γ and decreases side effects caused by metformin by decreasing the gene expression level of XBP-1. In addition, it was confirmed, through in vivo animal experiments, that the co-administration decreases insulin resistance while not affecting the pharmacokinetic properties of metformin (see Examples 32 to 34).
[0106] The pharmaceutical composition according to the present invention may include a pharmaceutically acceptable carrier in addition to active ingredients. Pharmaceutically acceptable carriers, which are generally used in pharmaceutical preparations, include lactose, dextrose, sucrose, sorbitol, mannitol, starch, acacia gum, calcium phosphate, alginate, gelatin, calcium silicate, microcrystalline cellulose, polyvinylpyrrolidone, cellulose, water, syrup, methyl cellulose, methyl hydroxybenzoate, propyl hydroxybenzoate, talc, magnesium stearate, mineral oil and the like, but the present invention is not limited thereto. In addition, the pharmaceutical composition may additionally include lubricants, wetting agents, sweeteners, flavoring agents, emulsifying agents, suspensions, preservatives and the like in addition to the carriers.
[0107] The pharmaceutical composition of the present invention may be administered orally or parenterally (for example, intravenous, subcutaneous, intraperitoneal or topical application) depending upon the desired method, and the dose, although varying depending on patient status and weight, degree of disease, drug type, route and time of administration, may be properly selected by those skilled in the art.
[0108] The pharmaceutical composition of the present invention is administered in a pharmaceutically effective dose. The term “pharmaceutically effective dose” according to the present invention refers to an amount sufficient to treat a disease at a reasonable benefit/risk ratio applicable to medical treatment, and the effective amount level may be determined by factors, including the disease type of a patient, severity, drug activity, sensitivity to a drug, administration time and route, emission rate, treatment period, and co-treated drugs, and other factors well known in medicine. The pharmaceutical composition according to the present invention may be administered as an individual therapeutic agent or in combination with other therapeutic agents, the composition may be administered sequentially or concurrently with conventional therapeutic agents, and the composition may be administered once or multiple times. Considering all of the above factors, it is important to administer a dose that can achieve the maximum effect in a minimal amount without side effects, which may be easily determined by those skilled in the art.
[0109] Specifically, the effective dose of the pharmaceutical composition of the present invention may be varied depending upon patient's age, sex, condition and body weight, the absorption degree of active ingredients in the body, the degree of inactivity, excretion rate, disease type, and co-treated drugs, and generally, 0.001 to 150 mg/kg body weight, preferably 0.01 to 100 mg, may be administered daily or every other day or one to three times a day. However, since the effective dose may be increased or decreased depending upon administration routes, the severity of obesity, sex, body weight, age and the like, the effective dose is not intended to limit the scope of the present invention in any way.
[0110] As another aspect of the present invention, the present invention provides a method of treating diabetes mellitus, which includes a step of administering the pharmaceutical composition to an individual. The term “individual” in the present invention refers to a subject who needs treatment for a disease, and more specifically, refers to humans or mammals such as non-human primates, mice, dogs, cats, horses and cattle.
[0111] Hereafter, the present invention will be described in more detail with reference to the following preferred examples. These examples are provided for illustrative purposes only and should not be construed as limiting the scope and spirit of the present invention.
Example 1. Cytotoxicity Experiments for Lonicera japonica Extracts
[0112] 100 μl of 3T3-L1 cells was aliquoted to each well of a 96-well plate at 3×10.sup.3 cells/well and incubated in a CO.sub.2 incubator for 24 hours. Samples at various concentrations were added to each well and incubated for 24 hours, and thereafter 10 μl of EZ-Cytox was added to each well. After incubation for 2 hours in an incubator, the plate was shaken for 1 minute before measuring absorbance and then absorbance was measured at 450 nm using a 96-well plate reader. Cytotoxicity was measured according to extraction methods (water extract: GEH, 30% ethanol extract: GEH30, 100% ethanol extract: GEH100), whether metformin was co-administered, and concentration changes of Lonicera japonica extracts (20, 50, 100, 200 μg/ml).
[0113] As a result, as illustrated in
Example 2. Measurement of Changes in Intracellular Reactive Oxygen Species (ROS) Activity by Administration of Lonicera japonica Extracts
[0114] 2 ml of HepG2 cells was aliquoted to each well of a 6-well plate at 3×10.sup.5 cells/well and incubated in a CO.sub.2 incubator for 8 hours, and then the HepG2 cells were either treated with metformin alone or with metformin in combination with a Lonicera japonica extract and incubated for 6 hours, followed by cell harvesting. After centrifugation at 1200 g for 5 minutes, a supernatant was discarded, and the remaining HepG2 cells were treated with 5 μg/ml of DHR123, followed by incubation at 37° C. for 30 minutes. After additional centrifugation for 5 minutes, PBS washing was performed two times and filtration was performed. Intracellular reactive oxygen species activity was measured based on the value of fluorescence intensity obtained from FACS analysis.
[0115] As a result, as illustrated in
Example 3. Measurement of DPPH Free Radical Scavenging Activity by Administration of Lonicera japonica Extracts
[0116] 40 μl of a sample was mixed with 760 μl of 300 μM 2,2-diphenyl-1-picrylhydrazyl (DPPH) and the mixture was incubated at 37° C. for 30 minutes, and then the mixture was aliquoted to each well of a 96-well plate in triplicate and absorbance was measured at 515 nm using a microplate reader. BHT was used as a positive control group. In Example 3, depending upon 3 extraction methods (water, 30% ethanol, and 100% ethanol extractions), the DPPH free radical scavenging capacity of a Lonicera japonica extract was measured and IC.sub.50 values were calculated.
[0117] As a result, BHT, a control group, showed a value of 113.85 μg/ml. In addition, when a Lonicera japonica water extract, a Lonicera japonica 30% ethanol extract, and a Lonicera japonica 100% ethanol extract were administered, as illustrated in the following Table 1, IC.sub.50 values were 143.36 μg/ml, 154.35 μg/ml, and 146.93 μg/ml, respectively, demonstrating that these extracts have an excellent free radical scavenging capacity. The most significant effect was observed in a Lonicera japonica water extract (Water extract).
TABLE-US-00001 TABLE 1 IC.sub.50 Lonicera japonica Water extract 143.36 μg/μl 30% EtoH 154.35 μg/μl 100% EtoH 146.93 μg/μl
Example 4. Measurement of Capacity of Lonicera japonica Extracts for Inhibiting Nitrogen Monoxide Generation
[0118] To compare an anti-inflammatory function, an in vitro model of LPS-induced nitrogen monoxide (NO) generation was used in an experiment, and NO measurement was carried out using a cell supernatant based on the GRIESS reaction (Green et al., 1982). RAW 264.7 cells were seeded at a density of 1.5×10.sup.5 cells/ml and pre-treated with samples diluted at various concentrations, and after 1 hour, the pretreated cells were treated with 1 μg/ml of lipopolysaccharide (LPS: Sigma, St Louis, Mo., USA), followed by incubation for 24 hours. 50 μl of a cell culture supernatant and 50 μl of 1% (w/v) sulfanilamide, a GRIESS reagent, were added to each well of a 96-well plate, and the 96-well plate shaded from light was incubated at room temperature for 10 minutes and then 50 μl of 0.1% (w/v) N-1-naphthylethylenediamine dissolved in 2.5% (v/v) phosphoric acid was added to each well of the 96-well plate and mixed, followed by incubation under dark conditions for 10 minutes. Absorbance was read at 540 nm using a microplate reader (Molecular Devices, CA, USA) within 30 minutes after finishing incubation. NO production was calculated using a nitric oxide standard solution.
[0119] As a result, as illustrated in
Example 5. Confirmation of Inhibitory Effects of Lonicera japonica Extracts on Fat Cell Differentiation
[0120] After seeding 3T3-L1 cells into a 6-well plate at a density of 5×10.sup.5 cells/well, the cells were cultured until reaching full confluence. The pre-existing culture medium for the cells was exchanged with DMEM (differentiation media) containing 1 μM dexamethasone, 0.5 mM IBMX, and 10 μg/ml insulin, and the cells were cultured for 48 hours and then were treated with DMEM (maturation media) containing 10 μg/ml insulin to induce differentiation. Differentiation-induced fat cells produced as a result of the process were treated with samples at various concentrations or a positive control group, and inhibitory effects on fat cell differentiation were analyzed using an Oil red O staining method, TG, and a TC assay.
[0121] As a result, as illustrated in
Example 6. Glucose Uptake Assay Depending Upon Administration of Lonicera japonica Extracts
[0122] Undifferentiated L6 rat myoblast cells were differentiated into myotube cells using 2% horse serum. As another method, HepG2 cells were seeded into each well of a 96-well back/clear bottom plate and incubated, and then the pre-existing medium was exchanged with a glucose free medium to provide a glucose starvation condition to the cells, followed by incubation for 12 hours. Thereafter, a medium of the cell culture was exchanged with a glucose free medium containing various samples and 2-NBDG, a fluorescent reagent, at a concentration of 100 μg/ml and then incubated for 6 to 12 hours. After incubation, the cell culture was washed two times with DPBS and then subjected to measurement of fluorescence intensity at 485/535 nm (excitation/emission=485/535 nm) using a fluorescence microplate reader. When performing measurement, apigenin, a compound that inhibits glucose uptake, was used as a control.
[0123] As a result, as illustrated in
Example 7. Insulin Secretion Assay Depending Upon Administration of Lonicera japonica Extracts
[0124] RIN-m5F insulinoma cells were cultured in a RPMI 1640 medium (WELGENE Inc., Korea) containing 10% FBS, 0.6% penicillin streptomycin (PS), and 300 mg/l L-glutamine in a CO.sub.2 incubator set to 37° C. with 5% CO.sub.2. RIN-m5F cells were aliquoted to each well of a 12-well plate at 3×10.sup.5 cells/well and incubated for 3 days, and then the cells were treated with the combination of 0.75 mM metformin and each of the Lonicera japonica extracts (GEH, GEH 30, or GEH 100). After culturing for 2 days, the pre-existing medium was discarded from the cells, and the cell culture was washed two times with modified Krebs-Ringer Bicarbonate Buffer (KRBB-HEPES, 134 mmol/1 NaCl, 4.8 mmol/1 KCl, 1 mmol/1 CaCl.sub.2, 1.2 mmol/1 MgSO.sub.4, 1.2 mmol/1 KH.sub.2PO.sub.4, 5 mmol/1 NaHCO.sub.3, 10 mmol/1 HEPES, 1 mg/ml BSA, pH 7.4) and incubated in a KRBB-HEPES buffer containing 20 mM glucose for 1 hour. A portion of cell culture supernatant was subjected to centrifugation at 4° C. for 10 minutes, and after centrifugation, a supernatant was collected and stored at −20° C. for further use. The amount of secreted insulin was measured using a rat insulin ELISA kit (Mercodia, Sweden), and an insulin secretion amount per gram of proteins was calculated by measuring the concentration of cellular proteins in each well.
[0125] As a result, as illustrated in
Example 8. Insulin Resistance Assay Depending Upon Administration of Lonicera japonica Extracts
[0126] Undifferentiated L6 rat myoblast cells were seeded into each well of a 96-well back/clear bottom plate and differentiated into myotube cells by adding 2% horse serum and then subjected to measurement of fluorescence intensity. The pre-existing medium of the differentiated L6 cells was exchanged with a glucose free medium to provide a glucose starvation condition to the cells, followed by incubation for 2 hours. After the incubation period, the cells under the glucose starvation condition were treated with samples at various concentrations. Thereafter, a medium of the cell culture was exchanged with a glucose free medium containing 5 mM glucosamine and incubated for 6 to 12 hours to induce insulin resistance. After removing a supernatant from the cell culture, the cell culture was treated with a glucose-free medium containing 100 μg/ml 2-NBDG and subsequently incubated for 6 hours, and then the cell culture was washed two times with DPBS and subjected to measurement of fluorescence intensity at 485/535 nm (excitation/emission=485/535 nm) using a fluorescence microplate reader.
[0127] As a result, as illustrated in
Example 9. Confirmation of Changes in Expression Levels of Related Proteins Depending Upon Administration of Lonicera japonica Extracts
9-1. DPP-4 and PPAR-γ Protein Expression
[0128] 3T3-L1 preadipocytes were cultured in DMEM (WELGENE Inc., Korea) containing 10% FBS and 1% penicillin streptomycin (PS) in a CO.sub.2 incubator set to 37° C. with 5% CO.sub.2. The cells were aliquoted to each well of a 6-well plate for cell culture at 8×10.sup.4 cells/well. To induce cell differentiation, the cells were cultured until reaching 50 to 60% confluence and subsequently, the pre-existing medium was exchanged with a differentiation-inducing DMEM medium containing 0.5 mM IBMX, 1 μM dexamethasone, 10 μg/ml insulin and 10% FBS, and then the cells were cultured for 3 days. After 3 days, the medium of the cell culture was exchanged with a DMEM medium containing 10 μg/ml insulin and 10% FBS and the cell culture was cultured while exchanging the medium every 2 days. At 5 days after differentiation, the cell culture was treated with samples and incubated for 24 hours. The cells in the 6-well plate were washed two times with PBS and subjected to lysis using a RIPA buffer (50 mM Tris-HCl pH 7.4, 1% NP-40, 0.25% sodium deoxycholate, 150 mM NaCl, 1 mM EDTA, 1 mM PMSF, 1 mM NaF, 1 mM sodium, 1 μg/ml aprotinin, leupeptin, pepstatin), and then the lysate was subjected to centrifugation at 12,000 rpm for 20 minutes to obtain a supernatant containing proteins. After performing quantification according to the BCA (Thermo Scientific, USA) method, electrophoresis was carried out on a 10% polyacrylamide gel. After electrophoresis, proteins on the gel were transferred to a PVDF membrane at 200 mA for 90 minutes, and the membrane was treated with a blocking buffer containing 5% skim milk or 5% BSA to reduce background signals due to non-specific proteins and incubated with primary antibodies at 4° C. overnight, and then the membrane was washed three times with TBS-T, in which each washing was performed for 10 minutes. Thereafter, the membrane was treated with secondary antibodies at room temperature for 1 hour and then washed three times with TBS-T, in which each washing was performed for 10 minutes, and the membrane was treated with an ECL (NEURONEX, Korea) solution and subsequently subjected to measurement of protein expression levels using LAS-3000 (FUJIFILM, Japan).
[0129] As a result, as illustrated in
9-2. p-AMPK and Sirt1 Protein Expression
[0130] RAW 264.7 cells, a macrophage cell line, were obtained from the Korean Cell Line Bank (KCLB, Seoul, Korea), and DMEM containing 10% FBS, 2 mM L-glutamine, 100 U/ml penicillin, and 100 μg/ml streptomycin was used as a medium for culturing the RAW 264.7 cells. The cells were cultured in a CO.sub.2 incubator set to 37° C. with 5% CO.sub.2 and 95% O.sub.2. Lonicera japonica extracts (100% water and 30% ethanol extracts) used in the experiments of the present invention were provided from the College of Pharmacy, Dongguk University. Experiments were performed for a total of 4 groups, including a normal group (N), a metformin-administered group (M), a group administered with a Lonicera japonica extract (30% ethanol extract) (GEH), and a group administered with metformin and a Lonicera japonica extract (30% ethanol extract) (M+GEH).
[0131] DMEM containing 10% FBS, 2 mM L-glutamine, 100 U/ml penicillin, and 100 μg/ml streptomycin was used as a medium for culturing the RAW 264.7 cells, and the cells were cultured under conditions of 37° C., 5% CO.sub.2, and 90% humidity. The cultured cells were maintained while exchanging the culture medium once every 2 to 3 days. When the cells were fully differentiated, the cell culture was washed with phosphate buffered saline (PBS) and then the cells were detached from a culture dish using a trypsin-EDTA solution. The separated cells were subjected to centrifugation to collect the same, and then the collected cells were mixed with a fresh medium and subcultured.
[0132] To prepare a cell lysate, cells treated with the composition according to the present invention were washed with a 10 mM phosphate buffer (pH 7.4) solution containing 150 mM NaCl (in PBS) and subjected to lysis with a PBS solution containing 0.1% SDS and 10 mM β-mercaptoethanol. After cell harvesting, a cell lysate was loaded onto an 8% SDS-polyacrylamide gel and subjected to electrophoresis. The protein bands existing on the gel were transferred to a nitrocellulose membrane (Schleicher and Schull, Dassel, Germany) using a semi-dry blotter (MilliBlot-SDE system, Millipore, Bedford, Mass., USA). The membrane was washed one time with a 10 mM Tris-buffered saline buffer (TBS, pH 7.2) containing 0.1% Tween-20 (TBS-T) and then soaked in a Tris-buffered saline buffer (TBS, pH 7.2) containing 3% skim milk and incubated at room temperature for 1 hour for blocking reaction. The membrane was incubated with anti-Sift1 antibodies, anti-p-AMPK antibodies, anti-AMPK antibodies (Cell Signaling Technology, DV, USA) or anti-beta actin antibodies. After incubation for 2 hours, the membrane was incubated with horseradish peroxidase-conjugated goat anti-Rabbit IgG antibodies (Santa Cruz Biotechnology, CA, USA) (diluted 1:1000) as a secondary antibody. Thereafter, the membrane was treated with an Enhanced Chemiluminescence (ECL) solution (Amersham Corp., Newark, N.J., USA) and subsequently analyzed using an image reader (LAS-3000, Fuji Photo Film, Tokyo, Japan). The intensities of the protein bands were measured using densitometry, and protein quantification was analyzed based on beta-actin.
[0133] As a result, as illustrated in
Example 10. Confirmation of Changes in Expression Levels of Related Genes Depending Upon Administration of Lonicera japonica Extracts
[0134] 10-1. Expression of Genes Associated with Anti-Diabetic Effect
[0135] To confirm whether combined use of metformin and a Lonicera japonica extract affects the expression of genes associated with an anti-diabetic effect, the gene expression levels of AMPK-α, PPAR-α, and PPAR-γ of RAW 264.7 cells administered with metformin alone (M) and RAW 264.7 cells administered with metformin and a Lonicera japonica extract (30% ethanol or 100% water) were compared using real-time PCR. RAW 264.7 cells were harvested according to the same method as described in Example 9-2. Experiments were performed for a total of 4 groups, including a normal group (N), a metformin-administered group (M), a group administered with metformin and a Lonicera japonica extract (30% ethanol) (M+GEH) and a group administered with metformin and a Lonicera japonica extract (water extract) (M+GEHW).
[0136] Total RNA was separated and purified using TRIsure (Bioline, USA) according to a protocol. 1 μg of total RNAs was subjected to a reverse transcription reaction using a cDNA synthesis kit (Sprint™RT Complete Oligo-(dT)18, Clontech, Mountain View, Calif., USA) according to a protocol for synthesizing first strand cDNA. The produced RT-PCR sample was subjected to real-time PCR reaction, in which the final reaction volume was adjusted to 20 μl and Light Cycler-Fast Start DNA Master SYBR Green (Roche Applied Science, Indianapolis, Ind., USA) and a Light Cycler instrument (Roche Applied Science) were used.
[0137] DNA sequences of primers used in Example 10-1 are as follows.
TABLE-US-00002 TABLE 2 Genus Specific Annealing Primers Direction Sequence temp. Beta-actin F 5′-GCAAGTGCTTCTAGGCGGAC-3′ 52° C. (SEQ ID NO. 1) R 5′-AAGAAAGGGTGTAAAACGCAGC-3′ (SEQ ID NO. 2) AMPK alpha 1 F 5′-AAGCCGACCCAATGACATCA-3′ 49° C. (SEQ ID NO. 3) R 5′-CTTCCTTCGTACACGCAAAT-3′ (SEQ ID NO. 4) PPAR-alpha F 5′-GCCTGTCTGTCGGGATGT-3′ 50° C. (SEQ ID NO. 5) R 5′-GGCTTCGTGGATTCTCTTG-3′ (SEQ ID NO. 6) PPAR-gamma F 5′-GCCCTTTGGTGACTTTATGGA-3′ 51° C. (SEQ ID NO. 7) R 5′-GCAGCAGGTTGTCTTGGATG-3′ (SEQ ID NO. 8)
[0138] PCR amplification was performed according to PCR steps, consisting of a pre-incubation step at 95° C. for 10 minutes and 35 (for beta-actin) or 45 (for C/EBPa) cycles of amplification (denaturation at 95° C. for 10 seconds, annealing at 52° C. for 10 seconds, and extension at 72° C. for 15 seconds). Total RNA was separated and purified using TRIsure (Bioline, USA) according to a protocol. 1 μg of total RNAs was subjected to a reverse transcription reaction using a cDNA synthesis kit (Sprint™RT Complete Oligo-(dT)18, Clontech, Mountain View, Calif., USA) according to a protocol for synthesizing first strand cDNA. The produced RT-PCR sample was subjected to real-time PCR reaction, in which the final reaction volume was adjusted to 20 μl and Light Cycler-Fast Start DNA Master SYBR Green (Roche Applied Science, Indianapolis, Ind., USA) and a Light Cycler instrument (Roche Applied Science) were used.
[0139] As a result, as illustrated in
[0140] In addition, as illustrated in
[0141] In addition, as illustrated in
10-2. Expression of Genes Associated with Side Effects of Metformin
[0142] To identify the effect of co-administration of metformin and a Lonicera japonica extract on expression of genes, which are associated with side effects caused by metformin, the gene expression levels of XBP-1, TNF-α, and IL-6 of RAW 264.7 cells administered with metformin alone (M) and RAW 264.7 cells administered with metformin and a Lonicera japonica extract (30% ethanol or 100% water) were compared using real-time PCR. RAW 264.7 cells were harvested according to the same method as described in Example 9-2. Experiments were performed for a total of 4 groups, including a normal group (N), a metformin-administered group (M), a group administered with metformin and a Lonicera japonica extract (30% ethanol) (M+GEH) and a group administered with metformin and a Lonicera japonica extract (water extract) (M+GEHW).
[0143] To identify the gene expression levels of XBP-1, TNF-α, and IL-6, real-time PCR was performed according to the same method as described in Example 10-1 except primers.
[0144] DNA sequences of primers used in Example 10-2 are as follows.
TABLE-US-00003 TABLE 3 Genus Specific Annealing Primers Direction Sequence temp. beta-actin F 5′-GCAAGTGCTTCTAGGCGGAC-3′ 52° C. (SEQ ID NO. 1) R 5′-AAGAAAGGGTGTAAAACGCAGC-3′ (SEQ ID NO. 2) XBP-1 F 5′-TGGCCGGGTCTGCTGAGTCCG-3′ 51° C. (SEQ ID NO. 9) R 5′-GTCCATGGGAAGATGTTCTGG-3′ (SEQ ID NO. 10) TNF-alpha F 5′-GAACTGGCAGAAGAGGCACT-3′ 52° C. (SEQ ID NO. 11) R 5′-AGGGTCTGGGCCATAGAACT-3′ (SEQ ID NO. 12) IL-6 F 5′-AGTTGCCTTCTTGGGACTGA-3′ 49° C. (SEQ ID NO. 13) R 5′-CAGAATTGCCATTGCACAAC-3′ (SEQ ID NO. 14)
[0145] As a result, as illustrated in
[0146] In addition, as illustrated in
[0147] In addition, as illustrated in
Example 11. Intraperitoneal Insulin Tolerance Test (IPITT) According to Administration of Lonicera japonica Extracts
[0148] To identify the effect of co-administration of metformin and a Lonicera japonica extract on diabetes mellitus, 4-week-old OLETF and LETO rats (Otsuka Pharmaceutical, Japan) were purchased and subjected to an 8-week adaptation period, and thereafter the rats were administered with 100 mg/kg of metformin alone or co-administered with 200 mg/kg of a Lonicera japonica extract and 100 mg/kg of metformin. Dietary intakes, body weights, states, and the like were checked weekly, and at 24 weeks, an IPITT was performed using blood collected from the tail veins. After 12 weeks, the rats were sacrificed under anesthesia with an intraperitoneal (IP) injection of Zoletil/Rompun, and fat, each organ sample, and serum were separated. One week prior to the end of the experiments, OLETF/LETO rats were fasted for 15 hours and then administered with 1 U/kg of insulin by intraperitoneal (IP) injection, and then measurement of blood sugar levels was performed using an Accu-Chek blood glucose meter (Roche, USA) on blood samples, which had been collected from the tail vein of each individual by bleeding a small amount of blood at 0, 30, 60, 90, and 120 minutes. The obtained values for blood sugar levels were analyzed using an area under curve (AUC), and the like.
[0149] As a result, as illustrated in
Example 12. Measurement of Pharmacokinetic Changes of Metformin by Co-Administration of Metformin and Lonicera japonica Extract
12-1. Pharmacokinetic Changes of Metformin According to Period of Co-Administration
[0150] A cannula was inserted into an artery of a rat under anesthesia. After awakening from the anesthesia, the rats were orally administered with 100 mg/kg of metformin (a group administered with metformin alone) or with 100 mg/kg of metformin and 200 mg/kg of a Lonicera japonica extract (a group co-administered with metformin and a Lonicera japonica extract). The drugs were administered once, for 7 days, or for 4 weeks according to experimental conditions. After administration, blood was drawn at regular intervals and urine was collected for 24 hours, and at 24 hours, gastrointestinal samples were taken to determine the amount of metformin remaining in the gastrointestinal tract. In addition, a blood concentration profile, urine, and the amount of metformin remaining in the gastrointestinal tract were calculated by quantification using LC/MSMS.
[0151] As a result, as illustrated in Table 4 and
TABLE-US-00004 TABLE 4 Lonicera japonica, Lonicera japonica, Single administration 7 days administration 4 weeks administration Metformin + Lonicera Metformin + Lonicera Metformin + Lonicera Metformin japonica Metformin japonica Metformin japonica Parameter (n = 11) (n = 13) (n = 8) (n = 8) (n = 6) (n = 7) Body weight 295 ± 47.7 275 ± 49.4 291 ± 11.3 295 ± 9.30 345 ± 32.7 356 ± 12.7 (g) AUC.sub.0-720 min 1739 ± 456 1940 ± 417 1983 ± 546 1770 ± 389 1984 ± 277 1653 ± 318 (μg min/ml) AUC.sub.0-∞ (μg 1980 ± 552 2001 ± 433 2062 ± 508 1840 ± 397 2140 ± 334 1895 ± 275 min/ml) Terminal half- 171 ± 73.5 128 ± 55.1 114 ± 40.5 139 ± 40.1 129 ± 49.1 155 ± 34.9 life (min) CL/F (ml/min/ 54.3 ± 15.4 52.5 ± 13.2 51.0 ± 11.9 56.9 ± 13.9 47.6 ± 7.00 53.8 ± 8.48 kg) C.sub.max (μg/ml) 7.65 ± 3.10 6.03 ± 1.47 8.60 ± 2.30 7.54 ± 0.879 8.00 ± 1.20 6.12 ± 1.21 T.sub.max (min).sup.a 90 (30-120) 90 (30-240) 90 (60-180) 75 (30-120) 120 (60-180) 120 (60-240) CL.sub.R (ml/min/kg) 40.3 ± 13.8 43.5 ± 8.71 40.5 ± 11.6 44.2 ± 12.1 37.9 ± 3.60 40.1 ± 6.54 Ae.sub.0-24 h (% of 74.0 ± 10.9 78.5 ± 8.52 79.5 ± 11.4 77.6 ± 6.80 80.1 ± 5.30 75.2 ± 13.3 dose) GI.sub.24 h (% of 5.72 ± 2.05 6.36 ± 2.04 4.10 ± 2.40 6.70 ± 3.30 8.80 ± 1.30 6.84 ± 4.20 dose) AUC.sub.0-720 min/ 90.2 ± 16.2 97.0 ± 1.83 95.7 ± 6.10 96.1 ± 2.40 93.1 ± 6.50 88.4 ± 17.3 AUC.sub.0-∞ (%) .sup.aMedian (ranges)
[0152] Whether metformin uptake was changed depending upon combined use of metformin and a Lonicera japonica extract was observed in cell products obtained from OCT transporter expressing cells. Verapamil was used as an inhibitor of OCT1 and 2, while 30 μM and 100 μM verapamil were applied for inhibiting OCT1 and OCT2, respectively, and 10 μM metformin was used as a substrate for OCT1 and 2.
[0153] As a result, as illustrated in
[0154] Taken together, it was confirmed that co-administration of a Lonicera japonica extract and metformin, an anti-diabetic drug, has no effect on absorption and action of metformin drug itself.
Example 13. Cytotoxicity Experiments for Scutellaria baicalensis Extracts
[0155] Cytotoxicity, using the same method as described in Example 1, was measured according to extraction methods (water extract: HG, 30% ethanol extract: HG30, 100% ethanol extract: HG100), whether metformin was co-administered, and concentration changes of Scutellaria baicalensis extracts (20, 50, 100, 200 μg/ml).
[0156] As a result, as illustrated in
Example 14. Measurement of Changes in Intracellular ROS Activity by Administration of Scutellaria baicalensis Extracts
[0157] Using the same method as described in Example 2, changes in intracellular ROS activity by administration of Scutellaria baicalensis extracts were measured.
[0158] As a result, as illustrated in
Example 15. Measurement of DPPH Free Radical Scavenging Activity by Administration of Scutellaria baicalensis Extracts
[0159] Using the same method as described in Example 3, depending upon 3 extraction methods (water, 30% ethanol, and 100% ethanol extractions), the DPPH free radical scavenging capacity of a Scutellaria baicalensis extract was measured and IC.sub.50 values were calculated.
[0160] As a result, BHT, a control group, showed a value of 113.85 μg/ml. In addition, when a Scutellaria baicalensis water extract, a Scutellaria baicalensis 30% ethanol extract, and a Scutellaria baicalensis 100% ethanol extract were administered, as illustrated in the following Table 5, IC.sub.50 values were 123.44 μg/ml, 244.36 μg/ml, and 249.47 μg/ml, respectively, demonstrating that these extracts have an excellent free radical scavenging capacity. The most significant effect was observed in a Scutellaria baicalensis water extract (Water extract).
TABLE-US-00005 TABLE 5 IC.sub.50 Scutellaria baicalensis Water extract 123.44 μg/μl 30% EtoH 244.36 μg/μl 100% EtoH 249.47 μg/μl
Example 16. Measurement of Capacity of Scutellaria baicalensis Extracts for Inhibiting Nitrogen Monoxide Generation
[0161] Using the same method as described in Example 4, the capacity of a Scutellaria baicalensis extract for inhibiting nitrogen monoxide generation was measured.
[0162] As a result, as illustrated in
Example 17. Confirmation of Inhibitory Effects of Scutellaria baicalensis Extracts on Fat Cell Differentiation
[0163] Using the same method as described in Example 5, inhibitory effects of Scutellaria baicalensis extracts on fat cell differentiation were analyzed.
[0164] As a result, as illustrated in
Example 18. Glucose Uptake Assay Depending Upon Administration of Scutellaria Baicalensis Extracts
[0165] Using the same method as described in Example 6, the capacity of glucose uptake depending upon administration of a Scutellaria baicalensi extract was measured.
[0166] As a result, as illustrated in
Example 19. Confirmation of Changes in Expression Levels of Related Proteins Depending Upon Administration of Scutellaria baicalensis Extracts
[0167] 3T3-L1 preadipocytes were cultured in DMEM (WELGENE Inc., Korea) containing 10% FBS and 1% penicillin streptomycin (PS) in a CO.sub.2 incubator set to 37° C. with 5% CO.sub.2. The cells were aliquoted to each well of a 6-well plate for cell culture at 8×10.sup.4 cells/well. To induce cell differentiation, the cells were cultured until reaching 50 to 60% confluence and subsequently, the pre-existing medium were exchanged with a differentiation-inducing DMEM medium containing 0.5 mM IBMX, 1 μM dexamethasone, 10 μg/ml insulin and 10% FBS, and then the cells were cultured for 3 days. After 3 days, the medium of the cell culture was exchanged with a DMEM medium containing 10 μg/ml insulin and 10% FBS and the cell culture was cultured while exchanging the medium every 2 days. At 5 days after differentiation, the cell culture was treated with samples and incubated for 24 hours. The cells in the 6-well plate were washed two times with PBS and subjected to lysis using a RIPA buffer (50 mM Tris-HCl pH 7.4, 1% NP-40, 0.25% sodium deoxycholate, 150 mM NaCl, 1 mM EDTA, 1 mM PMSF, 1 mM NaF, 1 mM sodium, 1 μg/ml aprotinin, leupeptin, pepstatin), and then the lysate was subjected to centrifugation at 12,000 rpm for 20 minutes to obtain a supernatant containing proteins. After performing quantification according to the BCA (Thermo Scientific, USA) method, electrophoresis was carried out on a 10% polyacrylamide gel. After electrophoresis, proteins on the gel were transferred to a PVDF membrane at 200 mA for 90 minutes, and the membrane was treated with a blocking buffer containing 5% skim milk or 5% BSA to reduce background signals due to non-specific proteins and incubated with primary antibodies at 4° C. overnight, and then the membrane was washed three times with TBS-T, in which each washing was performed for 10 minutes. Thereafter, the membrane was treated with secondary antibodies at room temperature for 1 hour and then washed three times with TBS-T, in which each washing was performed for 10 minutes, and the membrane was treated with an ECL (NEURONEX, Korea) solution and subsequently subjected to measurement of protein expression levels using LAS-3000 (FUJIFILM, Japan).
[0168] As a result, as illustrated in
Example 20. Confirmation of Changes in Expression Levels of Related Genes Depending Upon Administration of Scutellaria baicalensis Extracts
[0169] 20-1. Preparation of Cells and Scutellaria baicalensis Extracts
[0170] RAW 264.7 cells, a macrophage cell line, were obtained from the Korean Cell Line Bank (KCLB, Seoul, Korea), and DMEM containing 10% FBS, 2 mM L-glutamine, 100 U/ml penicillin, and 100 μg/ml streptomycin was used as a medium for culturing the RAW 264.7 cells. The cells were cultured in a CO.sub.2 incubator set to 37° C. with 5% CO.sub.2 and 95% O.sub.2. Scutellaria baicalensis extracts (100% water and 30% ethanol extracts) used in the experiments of the present invention were provided from the College of Pharmacy, Dongguk University. Experiments were performed for a total of 4 groups, including a normal group (N), a metformin-administered group (M), a group administered with metformin and a Scutellaria baicalensis extract (30% ethanol extract) (M+HGE), a group administered with metformin and a Scutellaria baicalensis extract (water extract) (M+HGW).
[0171] DMEM containing 10% FBS, 2 mM L-glutamine, 100 U/ml penicillin, and 100 μg/ml streptomycin was used as a medium for culturing the RAW 264.7 cells, and the cells were cultured under conditions of 37° C., 5% CO.sub.2, and 90% humidity. The cultured cells were maintained while exchanging the culture medium once every 2 to 3 days. When the cells were fully differentiated, the cell culture was washed with phosphate buffered saline (PBS) and then the cells were detached from a culture dish using a trypsin-EDTA solution. The separated cells were subjected to centrifugation to collect the same, and then the collected cells were mixed with a fresh medium and subcultured.
20-2. Expression of Genes Associated with Anti-Diabetic Effect
[0172] To confirm whether combined use of metformin and a Scutellaria baicalensis extract affects the expression of genes associated with an anti-diabetic effect, the gene expression levels of AMPK-α and PPAR-α of RAW 264.7 cells administered with metformin alone (M) and RAW 264.7 cells administered with metformin and a Scutellaria baicalensis extract (30% ethanol or 100% water) were compared using real-time PCR.
[0173] Total RNA was separated and purified using TRIsure (Bioline, USA) according to a protocol. 1 μg of total RNAs was subjected to a reverse transcription reaction using a cDNA synthesis kit (Sprint™RT Complete Oligo-(dT)18, Clontech, Mountain View, Calif., USA) according to a protocol for synthesizing first strand cDNA. The produced RT-PCR sample was subjected to real-time PCR, in which the final reaction volume was adjusted to 20 μl and Light Cycler-Fast Start DNA Master SYBR Green (Roche Applied Science, Indianapolis, Ind., USA) and a Light Cycler instrument (Roche Applied Science) were used.
[0174] DNA sequences of primers used in Example 20-2 are as follows.
TABLE-US-00006 TABLE 6 Genus Specific Annealing Primers Direction Sequence temp. Beta-actin F 5′-GCAAGTGCTTCTAGGCGGAC-3′ 52° C. (SEQ ID NO. 1) R 5′-AAGAAAGGGTGTAAAACGCAGC-3′ (SEQ ID NO. 2) AMPK alpha 1 F 5′-AAGCCGACCCAATGACATCA-3′ 49° C. (SEQ ID NO. 3) R 5′-CTTCCTTCGTACACGCAAAT-3′ (SEQ ID NO. 4) PPAR-alpha F 5′-GCCTGTCTGTCGGGATGT-3′ 50° C. (SEQ ID NO. 5) R 5′-GGCTTCGTGGATTCTCTTG-3′ (SEQ ID NO. 6)
[0175] PCR amplification was performed according to PCR steps, consisting of a pre-incubation step at 95° C. for 10 minutes and 35 (for beta-actin) or 45 (for C/EBPa) cycles of amplification (denaturation at 95° C. for 10 seconds, annealing at 52° C. for 10 seconds, and extension at 72° C. for 15 seconds). Total RNA was separated and purified using TRIsure (Bioline, USA) according to a protocol. 1 μg of total RNAs was subjected to a reverse transcription reaction using a cDNA synthesis kit (Sprint™RT Complete Oligo-(dT)18, Clontech, Mountain View, Calif., USA) according to a protocol for synthesizing first strand cDNA. The produced RT-PCR sample was subjected to real-time PCR, in which the final reaction volume was adjusted to 20 μl and Light Cycler-Fast Start DNA Master SYBR Green (Roche Applied Science, Indianapolis, Ind., USA) and a Light Cycler instrument (Roche Applied Science) were used.
[0176] As a result, as illustrated in
[0177] In addition, as illustrated in
20-3. Expression of Genes Associated with Side Effects of Metformin
[0178] To identify the effect of co-administration of metformin and a Scutellaria baicalensis extract on expression of genes, which are associated with side effects caused by metformin, the gene expression levels of XBP-1, TNF-α, and IL-6 of RAW 264.7 cells administered with metformin alone (M) and RAW 264.7 cells administered with metformin and a Scutellaria baicalensis extract (30% ethanol or 100% water) were compared using real-time PCR.
[0179] To identify the gene expression levels of XBP-1, TNF-α, and IL-6, real-time PCR was performed according to the same method as described in Example 3 except primers.
[0180] DNA sequences of primers used in Example 20-3 are as follows.
TABLE-US-00007 TABLE 7 Genus Specific Annealing Primers Direction Sequence temp. beta-actin F 5′-GCAAGTGCTTCTAGGCGGAC-3′ 52° C. (SEQ ID NO. 1) R 5′-AAGAAAGGGTGTAAAACGCAGC-3′ (SEQ ID NO. 2) XBP-1 F 5′-TGGCCGGGTCTGCTGAGTCCG-3′ 51° C. (SEQ ID NO. 9) R 5′-GTCCATGGGAAGATGTTCTGG-3′ (SEQ ID NO. 10) TNF-alpha F 5′-GAACTGGCAGAAGAGGCACT-3′ 52° C. (SEQ ID NO. 11) R 5′-AGGGTCTGGGCCATAGAACT-3′ (SEQ ID NO. 12) IL-6 F 5′-AGTTGCCTTCTTGGGACTGA-3′ 49° C. (SEQ ID NO. 13) R 5′-CAGAATTGCCATTGCACAAC-3′ (SEQ ID NO. 14)
[0181] As a result, as illustrated in
[0182] In addition, as illustrated in
[0183] In addition, as illustrated in
Example 21. Intraperitoneal Insulin Tolerance Test (IPITT) According to Administration of Scutellaria baicalensis Extracts
[0184] Using the same method as described in Example 11, an IPITT was performed to identify the effect of administration of Scutellaria baicalensis extracts on insulin tolerance.
[0185] As a result, as illustrated in
Example 22. Measurement of Pharmacokinetic Changes of Metformin by Co-Administration of Metformin and Scutellaria baicalensis Extract
22-1. Pharmacokinetic Changes of Metformin According to Period of Co-Administration
[0186] Using the same method as described in Example 12-1, pharmacokinetic changes of metformin according to the period of co-administration were measured.
[0187] As a result, as illustrated in Table 8 and
TABLE-US-00008 TABLE 8 Scutellaria baicalensis, Scutellaria baicalensis, Single administration 7 days administration 4 weeks administration Metformin + Metformin + Metformin + Scutellaria Scutellaria Scutellaria Metformin baicalensis Metformin baicalensis Metformin baicalensis Parameter (n = 11) (n = 8) (n = 8) (n = 8) (n = 10) (n = 9) Body 253 ± 21.6 264 ± 31.1 274 ± 6.94 277 ± 15.8 351 ± 27.5 286 ± 169 weight (g) AUC.sub.0-720 min 1834 ± 198 1695 ± 315 2065 ± 460 1922 ± 311 1865 ± 312 1745 ± 519 (μg min/ml) AUC.sub.0-∞ (μg 1940 ± 209 1790 ± 316 2131 ± 457 1985 ± 313 1940 ± 296 1875 ± 492 min/ml) Terminal 256 ± 141 210 ± 75.7 165 ± 71.4 152 ± 59.1 187 ± 102 288 ± 180 half- life (min) CL/F (ml/min/ 52.1 ± 6.01 57.4 ± 9.81 48.7 ± 9.86 51.4 ± 7.65 52.6 ± 8.17 55.8 ± 12.5 kg) C.sub.max (μg/ 8.60 ± 1.13 .sup. 6.93 ± 0.926.sup.a 9.21 ± 1.44 .sup. 7.54 ± 0.879.sup.a 7.14 ± 1.05 6.76 ± 0.189 ml) T.sub.max (min).sup.a 60 (30-120) 60 (30-120) 60 (30-120) 90 (30-180) 90 (30-180) 90 (60-180) CL.sub.R (ml/min/ 35.03 ± 6.33 35.9 ± 4.02 34.2 ± 9.80 38.1 ± 4.31 38.6 ± 9.09 117 ± 143 kg) Ae.sub.0-24 h (% 80.5 ± 12.1 71.02 ± 11.1 77.3 ± 18.6 83.03 ± 8.11 81.8 ± 15.4 75.8 ± 17.5 of dose) GI.sub.24 h (% of 12.9 ± 2.70 10.8 ± 4.49 6.52 ± 3.31 5.09 ± 1.64 9.21 ± 4.88 10.7 ± 3.31 dose) AUC.sub.0-720 min/ 94.6 ± 3.36 94.7 ± 4.34 96.8 ± 2.35 96.8 ± 1.27 95.9 ± 2.08 92.6 ± 4.12 AUC.sub.0-∞ (%) .sup.aP < 0.05 compared with metformin .sup.bMedian (ranges)
22-2. Changes in Metformin Uptake by Inhibition of OCT 1 and OCT 2
[0188] Using the same method as described in Example 12-2, changes in metformin uptake by inhibition of OCT 1 and 2 were measured.
[0189] As a result, as illustrated in
[0190] Taken together, it was confirmed that co-administration of a Scutellaria baicalensis extract and metformin, an anti-diabetic drug, has no effect on absorption and action of metformin drug itself.
Example 23. Cytotoxicity Experiments for Houttuynia cordata Extracts
[0191] Cytotoxicity, using the same method as described in Example 1, was measured according to extraction methods (water extract: OSC, 30% ethanol extract: OSC30, 100% ethanol extract: OSC100), whether metformin was co-administered, and concentration changes of Houttuynia cordata extracts (20, 50, 100, 200 μg/ml).
[0192] As a result, as illustrated in
Example 24. Measurement of Changes in Intracellular ROS Activity by Administration of Houttuvnia cordata Extracts
[0193] Using the same method as described in Example 2, changes in intracellular ROS activity by administration of Houttuynia cordata extracts were measured.
[0194] As a result, as illustrated in
Example 25. Measurement of DPPH Free Radical Scavenging Activity by Administration of Houttuynia cordata Extracts
[0195] Using the same method as described in Example 3, depending upon 3 extraction methods (water, 30% ethanol, and 100% ethanol extractions), the DPPH free radical scavenging capacity of a Houttuynia cordata extract was measured and IC.sub.50 values were calculated.
[0196] As a result, BHT, a control group, showed a value of 113.85 μg/ml. In addition, when a Houttuynia cordata water extract, a Houttuynia cordata 30% ethanol extract, and a Houttuynia cordata 100% ethanol extract were administered, as illustrated in the following Table 9, IC.sub.50 values were 239.80 μg/ml, 246.10 μg/ml, and 293.11 μg/ml, respectively, demonstrating that these extracts have an excellent free radical scavenging capacity. The most significant effect was observed in a Houttuynia cordata water extract (Water extract).
TABLE-US-00009 TABLE 9 IC.sub.50 Houttuynia cordata Water extract 239.80 μg/μl 30% EtoH 246.10 μg/μl 100% EtoH 293.11 μg/μl
Example 26. Measurement of Capacity of Houttuynia cordata Extracts for Inhibiting Nitrogen Monoxide Generation
[0197] Using the same method as described in Example 4, the capacity of a Houttuynia cordata extract for inhibiting nitrogen monoxide generation was measured.
[0198] As a result, as illustrated in
Example 27. Confirmation of Inhibitory Effects of Houttuynia cordata Extracts on Fat Cell Differentiation
[0199] Using the same method as described in Example 5, inhibitory effects of Houttuynia cordata extracts on fat cell differentiation were analyzed.
[0200] As a result, as illustrated in
Example 28. Glucose Uptake Assay According to Administration of Houttuynia cordata Extracts
[0201] Using the same method as described in Example 6, the capacity of glucose uptake depending upon administration of a Houttuynia cordata extract was measured.
[0202] As a result, as illustrated in
Example 29. Insulin Secretion Assay Depending Upon Administration of Houttuynia Cordata Extracts
[0203] Using the same method as described in Example 7, the capacity of insulin secretion depending upon administration of Houttuynia cordata extracts was measured.
[0204] As a result, as illustrated in
Example 30. Insulin Resistance Assay Depending Upon Administration of Houttuvnia Cordata Extracts
[0205] Using the same method as described in Example 8, insulin resistance depending upon administration of Houttuynia cordata extracts was measured.
[0206] As a result, as illustrated in
Example 31. Confirmation of Changes in Expression Levels of Related Proteins Depending Upon Administration of Houttuvnia cordata Extracts
[0207] 3T3-L1 preadipocytes were cultured in DMEM (WELGENE Inc., Korea) containing 10% FBS and 1% penicillin streptomycin (PS) in a CO.sub.2 incubator set to 37° C. with 5% CO.sub.2. The cells were aliquoted to each well of a 6-well plate for cell culture at 8×10.sup.4 cells/well. To induce cell differentiation, the cells were cultured until reaching 50 to 60% confluence and subsequently, the pre-existing medium was exchanged with a differentiation-inducing DMEM medium containing 0.5 mM IBMX, 1 μM dexamethasone, 10 μg/ml insulin and 10% FBS, and then the cells were cultured for 3 days. After 3 days, the medium of the cell culture was exchanged with a DMEM medium containing 10 μg/ml insulin and 10% FBS and the cell culture was cultured while exchanging the medium every 2 days. At 5 days after differentiation, the cell culture was treated with samples and incubated for 24 hours. The cells in the 6-well plate were washed two times with PBS and subjected to lysis using a RIPA buffer (50 mM Tris-HCl pH 7.4, 1% NP-40, 0.25% sodium deoxycholate, 150 mM NaCl, 1 mM EDTA, 1 mM PMSF, 1 mM NaF, 1 mM sodium, 1 μg/ml aprotinin, leupeptin, pepstatin), and then the lysate was subjected to centrifugation at 12,000 rpm for 20 minutes to obtain a supernatant containing proteins. After performing quantification according to the BCA (Thermo Scientific, USA) method, electrophoresis was carried out on a 10% polyacrylamide gel. After electrophoresis, proteins on the gel were transferred to a PVDF membrane at 200 mA for 90 minutes, and the membrane was treated with a blocking buffer containing 5% skim milk or 5% BSA to reduce background signals due to non-specific proteins and incubated with primary antibodies at 4° C. overnight, and then the membrane was washed three times with TBS-T, in which each washing was performed for 10 minutes. Thereafter, the membrane was treated with secondary antibodies at room temperature for 1 hour and then washed three times with TBS-T, in which each washing was performed for 10 minutes, and the membrane was treated with an ECL (NEURONEX, Korea) solution and subsequently subjected to measurement of protein expression levels using LAS-3000 (FUJIFILM, Japan).
[0208] As a result, as illustrated in
Example 32. Confirmation of Changes in Expression Levels of Related Genes Depending Upon Administration of Houttuynia cordata Extracts
[0209] 32-1. Preparation of Cells and Houttuynia cordata Extracts
[0210] RAW 264.7 cells, a macrophage cell line, were obtained from the Korean Cell Line Bank (KCLB, Seoul, Korea), and DMEM containing 10% FBS, 2 mM L-glutamine, 100 U/ml penicillin, and 100 μg/ml streptomycin was used as a medium for culturing the RAW 264.7 cells. The cells were cultured in a CO.sub.2 incubator set to 37° C. with 5% CO.sub.2 and 95% O.sub.2. Houttuynia cordata extracts (100% water and 30% ethanol extracts) used in the experiments of the present invention were provided from the College of Pharmacy, Dongguk University. Experiments were performed for a total of 4 groups, including a normal group (N), a metformin-administered group (M), a group administered with metformin and a Houttuynia cordata extract (30% ethanol extract) (M+USE), a group administered with metformin and a Houttuynia cordata extract (water extract) (M+USW).
[0211] DMEM containing 10% FBS, 2 mM L-glutamine, 100 U/ml penicillin, and 100 μg/ml streptomycin was used as a medium for culturing the RAW 264.7 cells, and the cells were cultured under conditions of 37° C., 5% CO.sub.2, and 90% humidity. The cultured cells were maintained while exchanging the culture medium once every 2 to 3 days. When the cells were fully differentiated, the cell culture was washed with phosphate buffered saline (PBS) and then the cells were detached from a culture dish using a trypsin-EDTA solution. The separated cells were subjected to centrifugation to collect the same, and then the collected cells were mixed with fresh media and used in subculture.
32-2. Expression of Genes Associated with Anti-Diabetic Effect
[0212] To confirm whether combined use of metformin and a Houttuynia cordata extract affects the expression of genes associated with an anti-diabetic effect, the gene expression levels of AMPK-α, PPAR-α, and PPAR-γ of RAW 264.7 cells administered with metformin alone (M) and RAW 264.7 cells administered with metformin and a Houttuynia cordata extract (30% ethanol or 100% water) were compared using real-time PCR.
[0213] Total RNA was separated and purified using TRIsure (Bioline, USA) according to a protocol. 1 μg of total RNAs was subjected to a reverse transcription reaction using a cDNA synthesis kit (Sprint™RT Complete Oligo-(dT)18, Clontech, Mountain View, Calif., USA) according to a protocol for synthesizing first strand cDNA. The produced RT-PCR sample was subjected to real-time PCR, in which the final reaction volume was adjusted to 20 μl and Light Cycler-Fast Start DNA Master SYBR Green (Roche Applied Science, Indianapolis, Ind., USA) and a Light Cycler instrument (Roche Applied Science) were used.
[0214] DNA sequences of primers used in Example 32-2 are as follows.
TABLE-US-00010 TABLE 10 Genus Specific Annealing Primers Direction Sequence temp. Beta-actin F 5′-GCAAGTGCTTCTAGGCGGAC-3′ 52° C. (SEQ ID NO. 1) R 5′-AAGAAAGGGTGTAAAACGCAGC-3′ (SEQ ID NO. 2) AMPK alpha 1 F 5′-AAGCCGACCCAATGACATCA-3′ 49° C. (SEQ ID NO. 3) R 5′-CTTCCTTCGTACACGCAAAT-3′ (SEQ ID NO. 4) PPAR-alpha F 5′-GCCTGTCTGTCGGGATGT-3′ 50° C. (SEQ ID NO. 5) R 5′-GGCTTCGTGGATTCTCTTG-3′ (SEQ ID NO. 6) PPAR-gamma F 5′-GCCCTTTGGTGACTTTATGGA-3′ 51° C. (SEQ ID NO. 7) R 5′-GCAGCAGGTTGTCTTGGATG-3′ (SEQ ID NO. 8)
[0215] PCR amplification was performed according to PCR steps, consisting of a pre-incubation step at 95° C. for 10 minutes and 35 (for beta-actin) or 45 (for C/EBPa) cycles of amplification (denaturation at 95° C. for 10 seconds, annealing at 52° C. for 10 seconds, and extension at 72° C. for 15 seconds). Total RNA was separated and purified using TRIsure (Bioline, USA) according to a protocol. 1 μg of total RNAs was subjected to a reverse transcription reaction using a cDNA synthesis kit (Sprint™RT Complete Oligo-(dT)18, Clontech, Mountain View, Calif., USA) according to a protocol for synthesizing first strand cDNA. The produced RT-PCR sample was subjected to real-time PCR, in which the final reaction volume was adjusted to 20 μl and Light Cycler-Fast Start DNA Master SYBR Green (Roche Applied Science, Indianapolis, Ind., USA) and a Light Cycler instrument (Roche Applied Science) were used.
[0216] As a result, as illustrated in
[0217] In addition, as illustrated in
[0218] In addition, as illustrated in
32-3. Expression of Genes Associated with Side Effects of Metformin
[0219] To identify the effect of co-administration of metformin and a Houttuynia cordata extract on expression of genes, which are associated with side effects caused by metformin, the gene expression levels of XBP-1 of RAW 264.7 cells administered with metformin alone (M) and RAW 264.7 cells administered with metformin and a Houttuynia cordata extract (30% ethanol or 100% water) were compared using real-time PCR. RAW 264.7 cells were harvested according to the same method as described in Example 9-2. Experiments were performed for a total of 4 groups, including a normal group (N), a metformin-administered group (M), a group administered with metformin and a Houttuynia cordata extract (30% ethanol) (M+USE) and a group administered with metformin and a Houttuynia cordata extract (water extract) (M+USW).
[0220] To identify the gene expression level of XBP-1, real-time PCR was performed according to the same method as described in Example 10-1 except primers.
[0221] DNA sequences of primers used in Example 32-3 are as follows.
TABLE-US-00011 TABLE 11 Genus Specific Annealing Primers Direction Sequence temp. beta-actin F 5′-GCAAGTGCTTCTAGGCGGAC-3′ 52° C. (SEQ ID NO. 1) R 5′-AAGAAAGGGTGTAAAACGCAGC-3′ (SEQ ID NO. 2) XBP-1 F 5′-TGGCCGGGTCTGCTGAGTCCG-3′ 51° C. (SEQ ID NO. 9) R 5′-GTCCATGGGAAGATGTTCTGG-3′ (SEQ ID NO. 10)
[0222] As a result, as illustrated in
Example 33. Intraperitoneal Insulin Tolerance Test (IPITT) According to Administration of Houttuynia cordata Extracts
[0223] Using the same method as described in Example 11, an IPITT was performed to identify the effect of administration of Houttuynia cordata extracts on insulin tolerance.
[0224] As a result, as illustrated in
Example 34. Measurement of Pharmacokinetic Changes of Metformin by Co-Administration of Metformin and Houttuynia cordata Extract
34-1. Pharmacokinetic Changes of Metformin According to Period of Co-Administration
[0225] Using the same method as described in Example 12-1, pharmacokinetic changes of metformin according to the period of co-administration were measured.
[0226] As a result, as illustrated in the following Table 12 and
TABLE-US-00012 TABLE 12 Houttuynia cordata, Houttuynia cordata, Single administration 7 days administration 4 weeks administration Metformin + Metformin + Metformin + Houttuynia Houttuynia Houttuynia Metformin cordata Metformin cordata Metformin cordata Parameter (n = 12) (n = 14) (n = 7) (n = 7) (n = 7) (n = 7) Body 276 ± 32.8 274 ± 31.5 284 ± 12.7 289 ± 10.7 354 ± 34.1 338 ± 13.4 weight (g) AUC.sub.0-720 min 1797 ± 297 2101 ± 397.sup.a 1616 ± 176 1633 ± 179 1922 ± 165 1808 ± 200 (μg min/ml) AUC.sub.0-∞ (μg 1865 ± 309 2172 ± 419.sup.a 1657 ± 181 1676 ± 202 1991 ± 156 1880 ± 213 min/ml) Terminal 174 ± 47.8 152 ± 43.5 143 ± 41.8 118 ± 42.8 156 ± 49.5 164 ± 58.7 half- life (min) CL/F (ml/min/ 54.4 ± 9.68 48.1 ± 9.62 61.0 ± 6.79 60.4 ± 7.74 50.5 ± 3.90 53.9 ± 6.73 kg) C.sub.max (μg/ 9.49 ± 1.65 8.42 ± 1.53 8.46 ± 2.49 6.71 ± 0.911 7.45 ± 0.960 8.22 ± 1.11 ml) T.sub.max (min).sup.b 60 (30-60) 90 (30-240).sup.a 60 (30-120) 90 (60-180) 120 (60-180) 90 (90-180) CL.sub.R (ml/min/ 39.1 ± 8.68 36.2 ± 7.92 50.1 ± 6.21 49.1 ± 6.06 45.3 ± 6.02 43.4 ± 6.81 kg) Ae.sub.0-24 h (% 70.7 ± 14.6 75.4 ± 10.2 82.7 ± 11.4 81.4 ± 5.24 89.4 ± 6.21 .sup. 80.5 ± 5.74.sup.a of dose) GI.sub.24 h (% of 9.00 ± 4.22 6.81 ± 3.47 10.3 ± 5.28 7.55 ± 4.08 11.2 ± 2.39 8.43 ± 4.42 dose) AUC.sub.0-720 min/ 96.3 ± 1.22 96.8 ± 1.31 97.5 ± 1.39 97.6 ± 1.90 96.5 ± 2.43 96.2 ± 2.57 AUC.sub.0-∞ (%)
34-2. Changes in Metformin Uptake by Inhibition of OCT 1 and OCT 2
[0227] Using the same method as described in Example 12-2, changes in metformin uptake by inhibition of OCT 1 and 2 were measured.
[0228] As a result, as illustrated in
[0229] Taken together, it was confirmed that co-administration of a Houttuynia cordata extract and metformin, an anti-diabetic drug, has no effect on absorption and action of metformin drug itself.
[0230] The aforementioned description of the present invention is provided by way of example and those skilled in the art will understood that the present invention can be easily changed or modified into other specified forms without change or modification of the technical spirit or essential characteristics of the present invention. Therefore, it should be understood that the aforementioned examples are only provided by way of example and not provided to limit the present invention.
INDUSTRIAL APPLICABILITY
[0231] The present invention relates to a composition for improving anti-diabetic and anti-obesity effects, including an extract extracted from any one selected from the group consisting of Lonicera japonica (Lonicerae Flos), Scutellaria baicalensis (Scutellariae Radix), and Houttuynia cordata (Houttuyniae Herba).
[0232] It was confirmed that combined use of the extract of the present invention and metformin, an anti-diabetic drug, improves therapeutic effects on diabetes mellitus and prediabetes and reduces side effects. Thus, it is expected that the extract can be usefully used as a pharmaceutical composition for improving a therapeutic effect on diabetes mellitus. In addition, it was confirmed that the extract exhibits an inhibitory effect on fat accumulation along with the therapeutic effect on diabetes mellitus. Therefore, it is expected that the extract can prevent or treat obesity along with treating diabetes.