Abstract
A process for obtaining a compound from buckwheat and its use as a
pharmaceutical treatment are disclosed. Methods of treatment using
extracts of buckwheat are also disclosed.
Claims
1. A product obtained by extracting buckwheat with about 10-30% ethanol.
2. The product of claim 1, wherein about 20% ethanol is used for
said extracting.
3. The product of claim 1, wherein said buckwheat is tartary buckwheat.
4. The product of claim 1, wherein said buckwheat is buckwheat
bran.
5. The product of claim 1, wherein said product is obtained by
centrifugation of said about 10-30% ethanol after said about 10-30%
ethanol has been placed in contact with said buckwheat.
6. The product of claim 1, wherein said extraction further comprises
concentration of said product by a process selected from the group
consisting of evaporation and drying.
7. A pharmaceutical composition for lowering blood glucose comprising
a extract of buckwheat bran obtained by extraction with about 10%
to 30% ethanol.
8. A nutritional supplement for lowering blood glucose comprising
an extract of buckwheat bran obtained by extraction with about 10%
to 30% ethanol.
9. A method for treating diabetic symptoms in an individual comprising
the administration of an effective dose of an extract of buckwheat
to said individual, wherein said extract was obtained by extraction
of buckwheat with about 10% to 30% ethanol.
10. The method of claim 9, wherein said ethanol is about 20% ethanol.
11. The method of claim 9, wherein said diabetic symptoms are selected
from the group consisting of hyperglycemia, glucose intolerance
and hyperlipidemia.
12. The method of claim 11, wherein said hyperlipidemia is selected
from the group consisting of hypercholesterolemia and hypertriglyceridemia.
13. The method of claim 9, wherein said treatment manifests as
an effect selected from the group consisting of lower fasting blood
glucose, lower non-fasting blood glucose, higher levels of superoxide
dismutase activity, higher catalase activity levels, lowering peak
glucose levels and increasing the rate of falling blood glucose
levels.
14. A method for isolating an anti-hyperglycemic agent from buckwheat,
comprising: (a) drying seed from said buckwheat; (b) isolating bran
from said seed; (c) extracting said agent from said bran with about
10% to 30% ethanol; and (d) processing said ethanol to isolate said
anti-hyperglycemic agent.
15. The method of claim 14, wherein said buckwheat is tartary buckwheat.
16. The method of claim 14, wherein said drying of said seed takes
place at a temperature of about 10 degrees Celsius.
17. The method of claim 14, wherein said alcohol is about 10% to
30% ethanol (w/v).
18. The method of claim 17, wherein said ethanol has a concentration
of about 20% (w/v).
19. The method of claim 14, wherein said processing comprises:
(a) centrifuging said ethanol to obtain a supernatant liquid; (b)
evaporating said supernatant liquid to obtain a residue; and (c)
drying said residue.
20. The method of claim 19, wherein said centrifuging is performed
at speeds of about 1000 to about 3000 RPM for about 5 to about 30
minutes.
21. The method of claim 19, wherein said method further comprises
a filtering step after centrifugation.
22. The method of claim 21, wherein said filtering step is performed
with an about 100 to about 300 mesh sieve filter.
Description
FIELD OF INVENTION
[0001] The present invention is related to the extract of tartary
buckwheat bran, method of extraction and the use of the extract
as anti-diabetic agent.
DESCRIPTION OF THE RELATED ART
[0002] Common and tartary buckwheat have been grown in many countries
around the world as a source of food. The flour and bran of both
types of buckwheat are proven to contain useful nutrients, such
as protein, lipid, starch, dietary fibre and vitamins B1, B2 and
B6.
[0003] Buckwheat products are known for their resistant starch
(Skrabanja, Laerke, & Kreft, 1998; Skrabanja, Liljeberg, Kreft,
& Bjorck, 2001) and as an important source of antioxidative
substances (Kreft, Bonafaccia, & Zigo, 1994; Kreft, Skrabanja,
Ikeda, Ikeda, & Bonafaccia, 1996), trace element, and dietary
fibre (Steadman, Burgoon, Lewis, Edwardson, & Obendorf 2001).
Buckwheat protein products have been associated preventive nutrition.
They are associated with retardation of mammary carcinogenesis by
lowering serum estradiol, and with suppression of colon carcinogenesis
by reducing cell proliferation (Kayashita, Shimaoka, Nakajoh, Kishida,
& Kato, 1999; Liu et al., 2001). There are, however, only a
few reports on the technological quality of buckwheat. Buckwheat
is also known as effective in modulating blood sugar and blood lipids
levels. However, the efficiency thereof is not very satisfactory.
[0004] It is therefore an object of the present invention to provide
compound and improved method of production of compounds for the
treatment of hyperglycemia.
SUMMARY OF INVENTION
[0005] In accordance with the object of the present invention,
there is provided in one aspect an active component in buckwheat
for the treatment of hyperglycemia. In the preferred embodiment,
the active component is obtained by extraction of buckwheat bran
using about 5-90% (w/v) ethanol. In another preferred embodiment,
the active component is obtained particularly in tartary buckwheat.
In yet another preferred embodiment, the ethanol concentration is
about 10-30% (w/v). In the most preferred embodiment, the ethanol
concentration is about 20% (w/v).
[0006] According to another aspect of the invention, there is provided
a novel anti-diabetic formulation comprising an effective amount
of the extract obtained from tartary buckwheat bran, optionally
together with additives, pharmaceutically accepted carriers, diluents
or excipients. The concentration of the extract in the formulation
may be 1 to 100% by wt.
[0007] Another aspect of the present invention is a method of extracting
a biologically active component from buckwheat comprising extraction
of buckwheat bran using about 10-90% (w/v) ethanol. In the preferred
embodiment, the active component of the present method is obtained
particularly from tartary buckwheat. In another preferred embodiment,
the ethanol concentration is about 10-30% (w/v). In the most preferred
embodiment, the ethanol concentration is about 20% (w/v).
[0008] According to a further aspect of the present invention,
an extract from buckwheat bran obtained by the method described
above is used for the preparation of a medicament or nutritional
supplement for reducing blood glucose concentration.
[0009] According to yet a further aspect of the present invention,
there is provided a method of reducing blood glucose concentration
in humans by administering an effective dose of an extract from
buckwheat bran obtained by the method described above.
[0010] An additional aspect of the invention comprises a method
for obtaining an anti-hyperglycemia agent, comprising the steps
of: [0011] (a) drying fresh seeds of tartary buckwheat at ambient
temperature, preferably around 10 degree Celsius; [0012] (b) separating
the bran from dried seeds by grinding; [0013] (c) extracting the
bran with ten fold of about 10-30% ethanol (w/v) for a period ranging
from about 24-120 hrs. at a temperature in a range of about 10-30
degree C., shaking or stirring occasionally during extraction and
transferring the liquid extract to a centrifuge bottle; and [0014]
(d) centrifuging at a speed in a range of about 1000-3000 rpm/min
for about 5-30 min to obtain supernatant liquid, then filtering
through about 100-300 mesh sieve filter, followed by evaporating
the filtered liquid to obtain a residue at reduced pressure with
temperature of about 60-80 degree C., and drying the residue with
vacuum-freezing drier to obtain dried residue.
[0015] Additional aspects of the invention include methods of treating
hyperglycemia in an individual comprising the administration of
a formulation comprising extract from tartary buckwheat bran to
said individual in a dosage of about 0.1 to 5 g/kg body weight per
day. In a preferred embodiment, a method of treatment for an adult
mammal comprises the administration of a formulation comprising
extract from tartary buckwheat bran to said mammal at a dosage of
about 5 to 250 mg/kg body weight per day. In an additional preferred
embodiment, the dosage of a formulation comprising extract from
tartary buckwheat bran used to treat an individual varies according
to the severity of the condition being treated and the pharmacological
activity of the formulation being used.
[0016] In some embodiments of the present invention, a product
obtained by extracting buckwheat with about 10-30% ethanol is provided.
The amount of ethanol can be, for example, at about 20%. The buckwheat
can be, for example, tartary buckwheat or buckwheat bran. The extraction
may occur by concentration of the product by evaporation or by drying.
In some embodiments, the product can be obtained by centrifugation
after the ethanol has been placed in contact with the buckwheat.
The product can also be used for the preparation of a medicament
for lowering blood glucose.
[0017] In additional embodiments of the present invention, a pharmaceutical
composition for lowering blood glucose having a extract of buckwheat
bran obtained by extraction with about 10% to 30% ethanol is provided.
[0018] In further embodiments of the present invention, a nutritional
supplement for lowering blood glucose having an extract of buckwheat
bran obtained by extraction with about 10% to 30% ethanol is provided.
[0019] In additional embodiments of the present invention, a method
for treating diabetic symptoms in an individual by the administration
of an effective dose of an extract of buckwheat to the individual
is provided, where the extract is obtained by extraction of buckwheat
with about 10% to 30% ethanol. The ethanol can be at a level of
about 20%. The diabetic symptoms may be, for example, hyperglycemia,
glucose intolerance, or hyperlipidemia. The hyperlipidemia can be
hypercholesterolemia or hypertriglyceridemia. The treatment may
manifest, for example, as lower fasting blood glucose, lower non-fasting
blood glucose, higher levels of superoxide dismutase activity, higher
catalase activity levels, lowering peak glucose levels and increasing
the rate of falling blood glucose levels.
[0020] In yet additional embodiments of the present invention,
a method for isolating an anti-hyperglycemic agent from buckwheat
is provided, by drying seed from the buckwheat, isolating the bran
from the seed, extracting the agent from the bran with about 10%
to 30% ethanol, and processing the ethanol to isolate the anti-hyperglycemic
agent. The buckwheat can be, for example, tartary buckwheat. The
drying of the seed can take place, for example, at a temperature
of about 10 degrees Celsius. The alcohol can be, for example, about
10% to 30% ethanol (w/v). The ethanol can have a concentration of
about 20 % (w/v). The processing can involve centrifuging the ethanol
to obtain a supematant liquid, evaporating the supematant liquid
to obtain a residue, and drying the residue. The centrifugation
can be performed at speeds of, for example, about 1000 to about
3000 RPM for about 5 to about 30 minutes. The method may also include
a filtering step after centrifugation. The filtering step can be
performed, for example, with an about 100 to about 300 mesh sieve
filter.
DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENT
[0021] The experiments to identify a biologically active component
for reducing blood sugar levels were performed initially using various
groups of compounds. These groups included flavonoids and other
solvent-extracted fractions obtained from buckwheat.
[0022] The experiments were performed in two stages. In the first
stage, the effectiveness of (1) a 20% ethanol extract of tartary
buckwheat; (2)a 60% ethanol extract of tartary buckwheat; and (3)
flavonoid(s) purified from tartary buckwheat were tested on alloxan
diabetic mice and STZ (streptozocin) diabetic rats. The negative
and positive controls used for comparison were water (negative control
group) and metformin (positive control group) respectively. In the
second stage, the effectiveness of 20% ethanol extract at different
doses was further tested on STZ diabetic rats, in comparison with
water (negative control group) and metformin (positive control group).
[0023] As stated earlier, the extract is obtained from tartary
buckwheat bran. The said extract is used to prepare the anti-diabetic
formulation. The formulation may be prepared according to any method
known in the art. The formulation may be intended for oral, parenternal
or other uses. The formulation for oral use may be in the form of
granules, particles, powders, tablets, capsules, liquid syrup, etc.
In order to prepare such formulation, any pharmaceutically acceptable
organic or inorganic, solid or liquid carrier, excipient, diluent
may be used. The formulation may also contain sweetening agent,
flavoring agent, colouring and preserving agents in order to provide
pharmaceutically elegant and palatable preparations. Tablets containing
the active ingredients, are prepared using the extract from tartary
buckwheat bran in combination with non-toxic pharmaceutically acceptable
carriers or additives.
[0024] Another aspect of the invention features methods for evaluating
the ability of buckwheat extracts to treat disease conditions. After
extraction of material from buckwheat, components of the material
are separated from one another by any one or more of a variety of
techniques, essentially creating two or more fractions of extract
material. Methods of separating the protein, mineral and carbohydrate
materials that can be present in such extracts are known to those
with skill in the art. Examples of such methods include precipitation,
centrifugation, filtration, PAGE, SDS-PAGE, high performance liquid
chromatography, size exclusion chromatography, ion exchange chromatography,
affinity chromatography and immunoassay. In these method examples,
component molecules of extracts are separated from one another based
on any one or more of numerous physical and chemical properties,
including, but not limited to, molecular size, charge, affinity
for other molecules, including hydrophobicity, solublity, molecular
shape and molecular structure. Once separated from the initial extract,
fractions of extracts can be tested for their ability to affect
biochemical properties of clinical samples and disease symptoms.
The examples below provide some exemplary methods for testing the
properties of extracts and fractions of extracts. It would be evident
to one with skill in the art that any number of different tests
and assays could be used to evaluate the properties of extracts
and fractions of extracts.
[0025] In the following animal study experiments, performed at
the Institute of Materia Medica of The Chinese Academy of Medical
Science, the glucose as well as the reagents were administered orally
into the mice and rats.
EXAMPLE 1
Determination of Effectiveness of Tartary Buckwheat Extracts
1.1 Preparing Tartary Buckwheat Extracts
1.1.1 20% Ethanol Extracts
[0026] The bran was provided by Shanxi GAP cultivation site. Food
Grade Ethanol was purchased from CSA Distilleries. Deionized water
was provided from in house water system.
[0027] Buckwheat concentrates were produced by soaking the bran
of tartary buckwheat in ten fold volume of 20% ethanol for 72 hours.
The extract was stirred occasionally within the set period (one
time per day). The supernatant was collected and filtered through
a 200 mesh sieve. Ethanol was removed when concentrated at 60.degree.
C., 600 mmHg. The sample was concentrated until 95% of volume was
evaporated. The concentrate was then dried by freeze-drying at -57.degree.
C. under vacuum. The moisture content for the dried sample was 9-10%.
[0028] The powder so obtained was then used for the formulation
of a preparation with the required concentration using conventional
pharmaceutically accepted additives suitable for oral or parenternal
administration to diabetic rats.
1.1.2 60% Ethanol Extracts
[0029] The bran was provided by Shanxi GAP cultivation site. Food
Grade Ethanol was purchased from CSA Distilleries. Deionized water
was provided from in house water system.
[0030] Buckwheat concentrates were produced by soaking the bran
of tartary buckwheat in ten fold volume of 60% ethanol, reflux for
1 hour, 2 times repeated. The supernatant was collected and filtered
through a 200 mesh sieve. Ethanol was removed when concentrated
at 60.degree. C., 600 mmHg. The sample was concentrated until 90%
of volume was evaporated. The concentrate was then dried by spray-dried
at inlet temperature of 140-150.degree. C. and outlet temperature
of 90-100.degree. C. The moisture content for the dried sample was
3-5%, total flavonoids content was 25%, the yield was 10.4%.
1.1.3 Purified Flavonoids
[0031] A purified flavonoids A was purchased from Institute of
Comprehensive Utilization of Agricultural Products, Shanxi Academy
of Agricultural Science. The purity of this sample was 70%, and
the moisture content was 3-5%.
[0032] A purified flavonoids B was prepared by our team. Tartary
buckwheat bran concentrates were produced by soaking the bran of
tartary buckwheat in ten fold volume of 60% ethanol, reflux for
1 hour, 2 times repeated. The supernatant was collected and filtered
through a 200 mesh sieve. Ethanol was removed when concentrated
at 60.degree. C., 600 mmHg. The sample was concentrated until 90%
of volume was evaporated. Let precipitate at 4.degree. C. overnight,
centrifuged at 3500 rpm for 20 minutes, collected the precipitate,
then dried in vacuum oven at 60.degree. C., 600 mmHg. The moisture
content for the dried sample was 3-5%, total flavonoids content
was 65%, yield 2.8%.
[0033] The powder so obtained is then used for the formulation
of the required concentration using conventional pharmaceutically
accepted additives suitable for oral or parenternal administration
to diabetic rats.
1.1.4 Determination of Total Flavonoids Content
[0034] Flavonoids are plant polyphenols and were found in the buckwheat
bran. Their hydrogen-donating antioxidant activity and their ability
to complex divalent transition metal cations are known. Spectrometry
method of measuring absorbance at 430 nm was employed for the determination
of flavonoid content.
[0035] 0.25-2.5 g sample was extracted by reflux in 125 ml 60%
ethanol for 1 hour. The solution was filtered by vacuum. The residue
was extracted again by reflux in 125 ml 60% ethanol for 1 hour and
the solution was filtered. The filtrates were combined and the volume
was fixed to 250 ml. The sample solution was freeze-dried and extract
powder was obtained. The dried sample was dissolved in methanol
to test.
[0036] 1 ml of extract methanolic solution was used. 1 ml of methanolic
AlCl3.quadrature. 6H2O was added. The sample was left for 10 minutes
for reaction. Absorbance was measured at 430 nm.
[0037] 0, 0.01, 0.02, 0.04, 0.06 mg/ml of Rutin standard was used.
The test was conducted to obtain the absorbance (A). The standard
solution concentration was used as x-axis while the absorbance (A)
was used as y-axis. The regression formula was determined
[0038] The flavonoids content in samples was calculated through
the regression formula.
1.2 Determination of Effect of the Extracts on the Alloxan Diabetic
Mice
1.2.1 Animals
[0039] Male ICR mice, weighing 22 to 26 g, were purchased from
VTLF Experiment Animal Technology Center Company Ltd., Beijing P.
R. China. The animals were made diabetic by a single intravenous
injection of 70 mg/kg alloxan into the tail vein. After a period
of 4 days, the treated mice were fasted for 2 hours, then the blood
sample was taken from the treated mice intravenously. The blood
glucose concentration was determined using Glucose Oxidase Peroxidase
method. The mice with the blood glucose concentration above 200
mg/dl were marked diabetic mice and were used for further experiments.
A total of 27 mice were marked as diabetic mice.
1.2.2 Reagents
[0040] (1) 60% ethanolic extracts of tartary buckwheat bran as
prepared in 1.1.2: 10.4% yield, 25% flavonoid
[0041] (2) 20% ethanolic extracts of tartary buckwheat bran as
prepared in 1.1.1: 7.5% yield, 0.3% flavonoid
[0042] (3) Purified flavonoid B from tatary buckwheat bran as prepared
in 1.1.3: 2.8% yield, 65% flavonoid
1.2.3 Methods
[0043] The mice were divided into 5 groups, each group having 9
mice. The difference in the average blood glucose concentration
among the 5 groups was less than 10 mg/dl
[0044] Group 1 served as the negative control and received water,
group 2 received metformin (200 mg/kg) as the positive control,
groups 3 and 4 received reagents (1) and (2), respectively, at the
dose of 5 g/kg (p.o.) (p.o. means oral administration), once every.
Group 5 received reagent (3) at the dose of 5 g/kg (p.o.).
[0045] At day 7 and 14, measurements of blood glucose concentration
were taken after fasting for 2.5 and 5 hours. The change of glucose
concentration by percentage was compared against the control group.
Blood triglyceride and cholesterol concentrations were tested at
day 14 (enzymatic method). Glucose tolerance test (2.0 g/kg, p.o.)
was conducted at day 19. First, the mice were fasted for half an
hour before the administration of control and test substances. Two
and half hours later, the mice received glucose at the dose of 2
g/kg, po. Blood samples were taken at 0, 30, 60, 120 minutes after
administration of the glucose. Blood glucose concentration (mg/dl)
of the mice were determined and the related measurements of Area
Under the Curve (AUC) were estimated. The serum superoxide dismutase
(SOD) level of blood samples taken at 0 minute was tested. Glucose
tolerance test was conducted again at day 22. The mice were fasted
for 1 hour before administration. One and half hour after administration,
the mice received glucose at the dose of 2 g/kg, po Blood samples
were taken at 0, 30 60, 120 minutes. For ease of description, the
negative control group that received water is indicated simply as
the "Control" while the positive control group is indicated
as the "Metformin" group in the following tables.
[0046] 1.2.4 Results TABLE-US-00001 TABLE 1 The effects of tartary
buckwheat bran extract on the blood glucose level of alloxan diabetic
mice Blood glucose concentration Blood glucose concentration at
day 7 (mg/dl) at day 14 (mg/dl) 2.5 hr after 2.5 hr after 5 hr after
administering 5 hr after administering administering (blood administering
(blood (blood glucose (blood glucose glucose glucose Dose change
by change by change by change by Group (mg/kg) percentage) percentage)
percentage) percentage) Control -- 357.9 .+-. 61.7 270.5 .+-. 63.7
357.1 .+-. 74.1 281.5 .+-. 24.6 Metformin 200 216.8 .+-. 78.2**
182.8 .+-. 88.1* 281.5 .+-. 60.9* 221.7 .+-. 65.9 (.dwnarw.39.4)
(.dwnarw.32.4) (.dwnarw.21.2) (.dwnarw.21.3) 60% 5000 323.8 .+-.
73.4 236.1 .+-. 74.0 394.2 .+-. 84.8 319.9 .+-. 91.6 ethanol (.dwnarw.9.5)
(.dwnarw.12.7) (.uparw.10.4) (.uparw.13.6) extract 20% 5000 325.7
.+-. 72.9 227.7 .+-. 75.6 374.3 .+-. 63.0 325.4 .+-. 71.4 ethanol
(.dwnarw.9.0) (.dwnarw.15.8) (.uparw.4.8) (.uparw.15.5) extract
Purified 5000 335.6 .+-. 113.6 233.1 .+-. 83.2 387.1 .+-. 144.1
321.4 .+-. 125.5 flavonoid B (.dwnarw.6.2) (.dwnarw.13.8) (.uparw.8.4)
(.uparw.14.1) Asterisks * indicate differences (*p < 0.05, **p
< 0.01, ***p < 0.005) between control group and reagent-treated
mice. Numbers in bracket indicate the change of blood glucose concentration
by percentage (%).
[0047] TABLE-US-00002 TABLE 2 The effects of tartary buckwheat
bran extract on the blood lipid level of alloxan diabetic mice at
day 14 Dose Blood cholesterol Blood triglyceride Group (mg/kg) (mg/dl)
(mg/dl) Control -- 173.4 .+-. 24.6 155.7 .+-. 33.9 Metformin 200
159.8 .+-. 48.7 132.8 .+-. 34.2 60% ethanol extract 5000 190.0 .+-.
26.0 180.8 .+-. 29.5 20% ethanol extract 5000 172.4 .+-. 16.5 133.9
.+-. 20.6 Purified flavonoid B 5000 172.4 .+-. 20.0 160.3 .+-. 27.2
[0048] TABLE-US-00003 TABLE 3 The effects of tartary buckwheat
bran extract on the serum SOD level of alloxan diabetic mice at
day 19 Serum SOD Group Dose (mg/kg) (u/mg) SOD change (%) Control
-- 70.0 .+-. 43.1 0 Metformin 200 78.3 .+-. 26.5 .uparw.11.9 60%
ethanol 5000 115.0 .+-. 23.1* .uparw.64.4 extract 20% ethanol 5000
94.8 .+-. 48.0 .uparw.35.5 extract Purified flavonoid B 5000 85.5
.+-. 33.8 .uparw.22.2 *indicates difference (p < 0.05) compared
with the control group.
[0049] TABLE-US-00004 TABLE 4 The effects of tartary buckwheat
bran extract on the glucose tolerance and AUC of alloxan diabetic
mice at day 19 Blood glucose (mg/dl) AUC Group 0 min 30 min 60 min
120 min (mg/dl h) Control 396.5 .+-. 87.9 513.9 .+-. 88.2 457.6
.+-. 106.2 355.9 .+-. 137.3 877.2 .+-. 206.4 Metformin 346.8 .+-.
68.3 544.4 .+-. 45.3 512.0 .+-. 76.9 408.4 .+-. 71.3 947.1 .+-.
118.1 60% 408.3 .+-. 75.2 554.9 .+-. 53.8 494.1 .+-. 65.8 440.7
.+-. 92.0 970.4 .+-. 131.6 ethanol extract 20% 362.0 .+-. 72.7 530.4
.+-. 58.7 462.4 .+-. 54.3 377.6 .+-. 83.8 891.3 .+-. 114.8 ethanol
extract Purified 408.0 .+-. 129.8 517.2 .+-. 81.7 466.2 .+-. 75.4
394.7 .+-. 94.9 907.7 .+-. 167.5 flavonoid B
[0050] TABLE-US-00005 TABLE 5 The effects of tartary buckwheat
bran extract on the glucose tolerance and AUC of alloxan diabetic
mice at day 22 Blood glucose (mg/dl) AUC Group 0 min 30 min 60 min
120 min (mg/dl h) Control 430.5 .+-. 66.1 520.1 .+-. 52.7 478.9
.+-. 53.7 387.2 .+-. 72.8 920.4 .+-. 113.4 Metformin 377.6 .+-.
87.6 474.5 .+-. 74.4 450.7 .+-. 80.1 358.6 .+-. 88.3 849.0 .+-.
158.3 60% 381.5 .+-. 60.1 464.6 .+-. 38.7* 438.9 .+-. 40.6 372.3
.+-. 56.2 843.0 .+-. 86.1 ethanol extract 20% 362.1 .+-. 54.4* 428.1
.+-. 40.8*** 391.3 .+-. 47.8** 319.4 .+-. 73.6 757.7 .+-. 101.8**
ethanol extract Purified 435.5 .+-. 103.2 444.2 .+-. 66.1* 408.2
.+-. 54.6* 339.4 .+-. 63.2 806.8 .+-. 125.0 flavonoid B *indicates
differences (p < 0.05, **p < 0.01, ***p < 0.005) compared
with the control group.
1.2.5 Conclusion
[0051] Neither the administration of a 20% ethanol tartary buckwheat
extract nor of a 60% tartart buckwheat extract, continuously for
7 and 14 days at the dose of 5 g/kg, were effective in lowering
blood glucose concentration in alloxan diabetic mice. However, metformin
used in the positive control group showed significant glucose-lowering
effect. After 7 and 14 days of continuing administration, the blood
glucose concentration in alloxan diabetic mice treated by metformin
was lowered by 34% (2.5 h, P<0.005), 32.4% (5 h, P<0.05),
21.2% (2.5 h, P<0.05), and 21.3% (5 h).
[0052] The administration of 20% and 60% ethanol extracts of tartary
buckwheat, continuously for 14 days at the dose of 5 g/kg, did not
affect the blood lipid level in alloxan diabetic mice.
[0053] Alloxan diabetic mice were treated separately with either
a 20% ethanol extract of tartary buckwheat, a 60% ethanol extract
of tartary buckwheat or purified flavonoids, continuously for 19
days at the dose of 5 g/kg. The treatments were effective in increasing
the amounts of SOD in serum samples from the mice by 64.4% (P<0.05),
35.5%, and 22.2%, respectively.
[0054] These three treatments, however, were not effective in improving
the glucose tolerance of alloxan diabetic mice when administered
continuously for 19 days at the dose of 5 g/kg. This may be because
glucose tolerance was tested 2.5 hours after administration and
the effect of the doses of the treatments had begun diminishing.
The glucose tolerance was tested again at day 22. The blood samples
were taken 1.5 hour after administration. Results from blood taken
at 0 min, 30 min and 60 min. showed that the 20% ethanol extract
was effective at in lowering blood glucose and AUC at day 22. The
60% ethanol extract was also effective in lowering blood glucose
as measured in blood samples taken at 30 and 60 minutes.
1.3 Determination of Effect of the Extracts on the Streptozocin
(STZ) Diabetic Rats
1.3.1 Reagents
[0055] (1) Purified flavonoid A from tartary buckwheat as prepared
in 1.1.3: 70% flavonoid
[0056] (2) Purified flavonoid B from tartary buckwheat as prepared
in 1.1.3: 70% flavonoid
[0057] (3) 20% ethanolic extracts of tartary buckwheat bran as
prepared in 1.1.1: 7.5% yield, 0.3% flavonoid
[0058] (4) 60% ethanolic extracts of tartary buckwheat bran as
prepared in 1.1.2: 10.4% yield, 25% flavonoid
1.3.2 Animals
[0059] Male rats (Sprague-Dwaley, male), weighing 120 to 140 g,
were purchased from VTLF Experiment Animal Technology Center Company
Ltd., Beijing P. R. China The animals were made diabetic by a single
intraperitoneal injection of streptozocin (freshly prepared in 0.1
M citrate buffer (pH 4.5) at the dose of of 58 mg/kg). After a period
of 4 days, the treated rats were fasted for 2.5 hours, then blood
samples were taken from the treated rats intravenously. Blood glucose
concentrations were determined using the Glucose Oxidase Peroxidase
method. The rats with blood glucose concentrations above 190 mg/dl
were marked as diabetic rats and used for further experiments.
1.3.3 Methods
[0060] The rats were divided into 6 groups of 10 rats per group.
The difference in the average blood glucose concentrations among
the 6 groups was less than 10 mg/dl. Group 1 served as the negative
control and received water. Group 2 received metformin (200 mg/kg)
as the positive control. The remaining four groups received reagents
(1) to (4) as listed in Section 1.3.1 above. Reagents (1) and (2)
were administered at a dose of 4 g/kg, while (3) and (4) were administered
at a dose of 5 g/kg. The treatments were administered once every
day.
[0061] At day 7, the rats in groups 1, 2 and 3 were fasted and
blood samples were taken at 2.5 hours and 5 hours after fasting
began. Blood glucose concentrations (mg/dl) in these samples were
then determined.
[0062] At day 14, glucose tolerance tests were conducted. The rats
were fasted for 1 hour before receiving the reagents at dosages
of 2.0 g/kg (p.o.). Blood samples were taken at 0, 30, 60, and 120
min after receiving the reagents. Blood glucose concentrations (mg/dl)
were determined and the related AUC were calculated.
[0063] At day 19, blood samples were taken, and blood glucose concentrations
without fasting, the activities of SOD and catalase (CAT) levels
were determined.
[0064] At day 21, glucose tolerance tests were conducted. The rats
were fasted for 1 hour, then received their respective reagents
at the dose of 5 g/kg (p.o.). 2.5 hours after administration of
reagent the rats received glucose at a dose of 2 g/kg (p.o.). Blood
samples were taken at 0, 30, and 120 minutes after glucose administration.
Blood glucose concentrations (mg/dl) were determined and the related
AUC were calculated.
[0065] 1.3.4 Results TABLE-US-00006 TABLE 6 The effects of tartary
buckwheat bran extract on the fasting blood glucose concentration
in STZ diabetic rat after oral administration for 7 days Fasting
blood glucose concentration (mg/dl) Sample dose (g/kg) 2.5 hr. 5.0
hr. Control -- 312.3 .+-. 53.5 282.6 .+-. 34.4 Metformin 0.2 261.1
.+-. 45.7* 185.6 .+-. 78.8** (.dwnarw.16.4) (.dwnarw.34.3) Purified
4.0 2.4.9 .+-. 37.7 244.6 .+-. 77.8 flavonoid A (.dwnarw.5.6) (.dwnarw.13.5)
Purified 4.0 311.2 .+-. 18.6 272.6 .+-. 26.0 flavonoid B (.dwnarw.0.4)
(.dwnarw.3.5) 20% ethanol 5.0 277.0 .+-. 35.3 247.5 .+-. 27.4* extract
(.dwnarw.11.3) (.dwnarw.12.4) 60% ethanol 5.0 311.8 .+-. 41.2 258.6
.+-. 15.7 extract (.dwnarw.0.2) (.dwnarw.8.5) Asterisks * indicate
differences (*p < 0.05, **p < 0.01) compared with the control
group. Numbers in the brackets indicate the change of blood glucose
concentration by percentage (%).
[0066] At day 7, the fasting blood glucose concentration in STZ
diabetic rats that received reagent (3) at a dose of 5 g/kg was
significantly reduced by 12.4%. Those rats that received reagents
(1) and (2) (at 4 g/kg) and (4) (at 5 g/kg) did not show any significant
effects. TABLE-US-00007 TABLE 7 The effects of tartary buckwheat
bran extracts on blood glucose concentration and AUC in STZ-diabetic
rat after oral administration for 14 days dosage blood glucose concentration
(mg/dl) AUC Sample (g/kg) 0 min 30 min 60 120 min (mg/dl hr) Control
-- 398.4 .+-. 75.0 473.0 .+-. 104.5 438.9 .+-. 75.5 355.1 .+-. 62.0
842.8 .+-. 150.1 Metformin 0.2 341.8 .+-. 44.8 356.2 .+-. 93.3*
320.9 .+-. 64.6* 296.6 .+-. 72.6 652.5 .+-. 133.8* (.dwnarw.22.6)
Purified 4.0 370.1 .+-. 55.5 421.5 .+-. 68.0 378.9 .+-. 83.9 339.9
.+-. 82.6 757.3 .+-. 139.5 flavonoid A (.dwnarw.10.1) Purified 4.0
364.1 .+-. 25.2 440.5 .+-. 39.4 406.6 .+-. 31.0 367.9 .+-. 26.7
800.2 .+-. 53.8 flavonoid B (.dwnarw.5.1) 20% 5.0 354.5 .+-. 31.7
382.3 .+-. 40.4* 359.0 .+-. 51.5* 337.1 .+-. 37.8 717.6 .+-. 75.8*
ethanol (.dwnarw.14.9) extract 60% 5.0 364.7 .+-. 37.0 400.4 .+-.
36.1 378.9 .+-. 42.1 328.7 .+-. 36.0 739.6 .+-. 69.5 ethanol (.dwnarw.12.2)
extract Asterisks * indicate differences (*p < 0.05) compared
with control group. Numbers in brackets indicate the reduction of
AUC by percentage (%)
[0067] Table 7 shows the effects of tartary buckwheat bran extracts
(as prepared according to the method described in section 1.1).
At day 14, glucose tolerance test was conducted. Results showed
that the 20% ethanol extract was effective in lowering the blood
glucose concentration at 30 min and 60 min and its AUC was lower
than the control group by 14.9%. TABLE-US-00008 TABLE 8 The effects
of tartary buckwheat bran extract on blood glucose concentrations
without fasting, serum SOD activity and catalase (CAT) activity
in STZ-diabetic rat after oral administration for 19 days Non-fasting
blood Dosage glucose Serum SOD activity CAT activity Group (g/kg)
concentration mg/dl) (NU/ml) (U/gHb) Control -- 361.5 .+-. 58.2
121.6 .+-. 32.8 68.4 .+-. 22.4 Metforimin 0.2 340.5 .+-. 40.7 164.8
.+-. 16.9** 64.6 .+-. 12.5 (.dwnarw.5.8) (.uparw.35.3) (.dwnarw.5.5)
Purified 4.0 324.0 .+-. 91.4 112.2 .+-. 24.4 79.8 .+-. 15.3 flavonoid
A (.dwnarw.10.4) (.dwnarw.7.8) (.uparw.16.7) Purified 4.0 304.3
.+-. 69.7 86.9 .+-. 8.0** 73.2 .+-. 23.6 flavonoid B (.dwnarw.15.8)
(.dwnarw.28.6) (.uparw.7.0) 20% ethanol extract 5.0 264.1 .+-. 55.6**
132.5 .+-. 17.7 98.3 .+-. 16.3** (.dwnarw.26.9) (.uparw.9.0) (.uparw.43.7)
60% ethanol extract 5.0 298.4 .+-. 36.5* 158.7 .+-. 18.2** 86.0
.+-. 17.1 (.dwnarw.17.4) (.uparw.30.5) (.uparw.25.7) Asterisks *
indicate differences (*p < 0.05, **p < 0.01) compared the
control group. Number in the brackets indicate the change by percentage.
[0068] At day 19, rats treated with reagent (3) (at 5 g/kg) showed
a significant effect by lowering blood glucose concentrations by
26.9% and increasing the activity of CAT by 43.7% in comparison
to the control group. Rats treated with reagent (4) (at 5 g/kg)
also showed a significant effect by lowering blood glucose concentrations
by 17.4% and increasing the activity of serum SOD by 30.5%. Reagents
(1) and (2) were not effective on non-fasting blood glucose concentrations
and CAT activities and reagent (2) (at 4 g/kg) actually reduced
the activity of serum SOD by 28.6%, in comparison to the control
group. TABLE-US-00009 TABLE 9 The effects of tartary buckwheat bran
extracts on oral glucose tolerance in STZ diabetic rat after oral
administration for 21 days dosage blood glucose concentration(mg/dl)
AUC Sample (g/kg) 0 min 30 min 120 min (mg/dl hr) Control -- 363.4
.+-. 61.1 463.9 .+-. 56.6 338.3 .+-. 55.8 808.5 .+-. 101.9 Metformin
0.2 309.8 .+-. 68.5 358.0 .+-. 77.3** 279.8 .+-. 51.6* 645.4 .+-.
122.0** (.dwnarw.20.2) 20% 5.0 322.8 .+-. 59.4 379.6 .+-. 64.9**
327.4 .+-. 32.6 705.9 .+-. 95.2* ethanol (.dwnarw.12.7) extracts
Asterisks * indicate differences (*p < 0.05, **P < 0.01) compared
with the control group. Numbers in brackets indicate the change
of AUC by percentage (%).
[0069] At day 21, glucose tolerance tests were conducted. The 20%
ethanol extracts lowered blood glucose concentrations by 64.9% and
reduced AUC values by 12.7% at 30 min, in comparison to the control
group. TABLE-US-00010 TABLE 10 The effects of tartary buckwheat
bran extracts on weight in STZ diabetic rat after oral administration
for 9, 14 and 21 days dosage weight(g) Sample (g/kg) At day 9 At
day 14 At day 21 Control -- 216.2 .+-. 20.3 217.3 .+-. 25.4 191.5
.+-. 31.6 Metformin 0.2 203.3 .+-. 22.3 200.4 .+-. 29.4 185.3 .+-.
27.3 Purified 4.0 203.6 .+-. 36.3 199.7 .+-. 42.8 N/A flavonoid
A Purified 4.0 198.5 .+-. 36.7 210.5 .+-. 33.7 N/A flavonoid B 20%
ethanol 5.0 224.3 .+-. 13.1 237.5 .+-. 18.5 225.1 .+-. 33.8* extracts
60% ethanol 5.0 220.1 .+-. 24.1 234.0 .+-. 32.7 N/A extracts Asterisks
* indicate differences (*p < 0.05) compared with the control
group.
[0070] Before administration, there was no obvious difference among
the rats of different groups. After administration for 21 days,
the average weight of rats receiving 20% ethanol extract was significantly
heavier than the control group.
1.3.5 Conclusion
[0071] When administered at the dose of 5 g/kg continuously for
7 days, the 20% ethanol extract of tartary buckwheat was effective
in lowering the fasting blood glucose concentration 5 hours after
administration. After 14 and 21 days of continuous administration,
the glucose tolerance of STZ diabetic rats was also significantly
improved. After 19 days of continuous administration, the non-fasting
blood glucose concentrations of STZ diabetic rats was lowered and
the serum CAT activities were enhanced. The average weight of the
rats receiving 20% ethanol extract at 5 g/kg was heavier than the
control group after treatment. Their overall condition was also
better than the control group. The above results demonstrate that
20% ethanol extract of tartary buckwheat was effective for the amelioration
of diabetic symptoms of STZ diabetic rats.
[0072] At the dose of 5 g/kg, the 60% ethanol extract of tartary
buckwheat was effective in lowering the non-fasting blood glucose
of STZ diabetic rats after 19 days of continuous administration.
It was also effective in enhancing the serum SOD and the CAT activities.
However, it was not effective in improving fasting blood glucose
levels or glucose tolerance.
[0073] Flavonoid A (4 g/kg) and B (4 g/kg) purified from tartary
buckwheat do not affect fasting blood glucose and non-fasting blood
glucose concentrations, CAT activities or glucose tolerance. Flavonoid
B (4 g/kg) produced a negative effect by reducing serum SOD activity.
[0074] Flavonoid A and B were administered at 4 g/kg instead of
5 g/kg as used in other groups. This was due to flavonoid A becoming
too condensed for administration when used at a concentration of
5 g/kg.
[0075] In conclusion, the 20% ethanol extracts of tartary buckwheat
were the most effective reagents among those tested for the amelioration
of hyperglycemic and diabetic symptoms.
EXAMPLE 2
Further Analysis of 20% Ethanol Extract of Tartary Buckwheat on
STZ Diabetic Rats
[0076] In this sets of experiments, a range of doses of the 20%
ethanol extract of tartary buckwheat administered for a variety
of lengths of time were tested for effectiveness in the treatment
of STZ diabetic rats.
2.1 Reagent
[0077] 20% ethanol extract of tartary buckwheat as prepared in
1.1.1: 7.5% yield; 0.3% flavonoid.
2.2 Animals
[0078] The mice were divided according to the blood glucose concentration
under fasting conditions. The difference between the average blood
glucose concentrations of the 4 groups of rats was less than 10
mg/dl.
2.3 Methods
[0079] The STZ diabetic rats were divided into 4 groups, each group
having 10 rats. Group 1 served as the negative control and received
water, group 2 received metformin (200 mg/kg) as the positive control,
group 3 received 20% ethanol extract of the bran of tartary buckwheat
seeds at the dose of 2.5 g/kg (p.o.), group 4 received 20% ethanol
extract of the bran of tartary buckwheat seeds at the dosage of
5 g/kg (p.o.), once every day for 12 days in a row.
[0080] At day 7, fasting blood glucose concentration was tested
after 2.5 and 5 hours of fasting. The change of glucose concentration
by percentage was compared against the control group.
[0081] At day 12, oral glucose tolerance tests (2.0 g/kg) were
conducted. The rats were fasted for 1 hour before administration
of reagents at dosages of 2.5 or 5 g/kg (p.o.). 1 hour later, the
rats received glucose at the dose of 2 g/kg (p.o.). Blood samples
were taken at 0, 30 and 120 min respectively. Blood glucose concentrations
(mg/dl) were determined and the related AUC values were calculated.
[0082] 2.4 Results TABLE-US-00011 TABLE 11 The effects of 20% ethanol
extract of tartary buckwheat on the fasting blood glucose concentration
in STZ diabetic rats after oral administration for 7 days fasting
blood glucose dosage concentration (mg/dl) Group (g/kg) 2.5 hr.
5 hr. Control -- 404.6 .+-. 40.2 372.7 .+-. 59.3 metformin 0.2 357.2
.+-. 51.5 288.9 .+-. 68.8* (11.7) (22.5) 20% Extract 2.5 340.8 .+-.
44.5** 310.6 .+-. 37.3* (15.8) (16.7) 20% Extract 5.0 329.0 .+-.
43.0** 311.3 .+-. 21.5* (18.7) (16.5) Asterisks * indicate differences
(*p < 0.05, **p < 0.01) compared with the control group, numbers
in brackets indicate the reduction of blood glucose concentration
by percentage (%).
[0083] After oral administration for 7 days, the rats in group
1, 2, 3 and 4 were fasted for 2.5 and 5 hours, blood samples were
taken, and blood glucose concentrations (mg/dl) of these rats were
determined. The 20% extract was effective in lowering blood glucose
concentration by 15.8%, 18.7%, 16.7%, and 16.5% (Table 11). TABLE-US-00012
TABLE 12 The effects of tartary buckwheat bran extract on oral glucose
tolerance in STZ diabetic rats after 12 days oral administration
Fasting blood glucose dosage concentration (mg/dl) AUC Group (g/kg)
0 min 30 min 120 min (mg/dl hr) Control -- 448.6 .+-. 52.2 475.2
.+-. 52.6 408.3 .+-. 41.9 934.0 .+-. 80.8 metformin 0.2 398.4 .+-.
36.6 458.4 .+-. 59.7 323.9 .+-. 51.2* 800.9 .+-. 103.2* (14.2) 20%
extract 2.5 399.0 .+-. 56.4 455.6 .+-. 69.6 359.5 .+-. 63.8 825.0
.+-. 124.8 (11.7) 20% extract 5.0 434.2 .+-. 27.6 456.3 .+-. 32.4*
357.9 .+-. 53.9 833.3 .+-. 17.5** (10.8) Asterisks * indicate differences
(*p < 0.05, **P < 0.01) compared with the control group. Numbers
in brackets indicate the reduction of AUC by percentage (%).
[0084] After oral administration for 12 days, glucose tolerance
tests on rats given extracts or control substances were conducted.
The 20% ethanol extract at the dose of 5 g/kg showed a statistically
significant (p<0.05) anti-diabetic effect at 30 min by lowering
the blood glucose concentrations and AUC (10.8%) values in comparison
to the control group (water) of rat (Table 12).
2.5 Conclusion
[0085] The 20% ethanol extract of tartary buckwheat was effective
in lowering the fasting blood glucose of STZ diabetic rats 2.5 and
5 hours after single dose administration when administered over
the previous consecutive 7 days at the doses of 2.5 g/kg and 5 g/kg.
After administration for 12 days at the doses of 2.5 g/kg and 5
g/kg, the glucose tolerances of the STZ diabetic rats were also
improved with different degrees. The effects of differing amounts
of the extract on blood glucose concentrations were basically the
same.
CONCLUSION
[0086] Based on the pharmacology results, the results above show
that 20% ethanol extract of tartary buckwheat has effect on hyperglycemia
or diabetes in animal models. The data indicate that in a preferred
embodiment, a dose equivalent to 18.2 g human daily dosage is effective
for treatment of hyperglycemia or diabetes in humans.
[0087] While the present invention has been described with respect
to the effectiveness of tartary buckwheat extracts on lowering glucose
concentrations in mice/rats, it should be understood by those skilled
in the art that various changes may be made and equivalents may
be substituted without departing from the true spirit and scope
of the invention. For instance, the ethanol used can be replaced
with other alcohols, such as propanol, isopropanol, n-butanol, etc.
In addition, many modifications may be made to adapt a particular
situation, material, composition of matter, process, process step
or steps, to the objective, spirit and scope of the present invention.
All such modifications are intended to be within the scope of the
claims appended hereto. As used in the present specification and
claims, the terms "comprise," "comprises," and
"comprising" mean "including, but not necessarily
limited to". For example, a method, apparatus, molecule or
other item which contains A, B, and C may be accurately said to
comprise A and B. Likewise, a method, apparatus, molecule or other
item which "comprises A and B" may include any number
of additional steps, components, atoms or other items as well.
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