CN101709093A - Method for preparing blumea riparia water-soluble polysaccharides - Google Patents

Method for preparing blumea riparia water-soluble polysaccharides Download PDF

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CN101709093A
CN101709093A CN200910114640A CN200910114640A CN101709093A CN 101709093 A CN101709093 A CN 101709093A CN 200910114640 A CN200910114640 A CN 200910114640A CN 200910114640 A CN200910114640 A CN 200910114640A CN 101709093 A CN101709093 A CN 101709093A
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soluble polysaccharides
molecular weight
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blumea riparia
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CN101709093B (en
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林翠梧
廖敏富
黄丽
许子竞
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Guangxi University
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Abstract

The invention discloses a method for preparing blumea riparia water-soluble polysaccharides. One method of the invention comprises the steps of extraction, film separation, protein removal, desalination, decoloration, refining and refining. The second method of the invention comprises the steps of extraction, film separation, protein removal, silica gel column chromatographic separation, decoloration, dialysis and refining. The method has the advantages of simple process flow, energy conservation, high product purity, stable quality and the like. The production of the invention particularly has significant hemostatic activity in blood coagulation recalcification tests and isolated uterine tests of mice.

Description

A kind of preparation method of blumea riparia water-soluble polysaccharides
Technical field
The present invention relates to medical technical field, specifically is a kind of preparation method of blumea riparia water-soluble polysaccharides.
Background technology
Herba Blumeae Balsamiferae is a composite family Herba Blumeae Balsamiferae platymiscium, record in " Chinese medicine sea ", and the Herba Blumeae Balsamiferae meridian distribution of property and flavor: light, sweet flat, go into liver, kidney, bladder three warps; Effect cures mainly: the sweet liver of fading in of promoting blood circulation and hemostasis-this product, and nourishing the liver is invigorated blood circulation, matter is puckery, and astringing to arrest bleeding has the merit that the stasis of blood is not stayed in invigorate blood circulation not blood trouble, hemostasis, can be used for various hemorrhages; Mention also in " Xinhua book on Chinese herbal medicine outline " that it is invigorated blood circulation, hemostatic function, can be used for menstrual period in advance, gynecological and hemorrhage symptoms such as massive postpartum vaginal bleeding.
Herba Blumeae Balsamiferae is all taken with the decocting decoction among the people as the existing long history of Guangxi medication among the people, is used for the treatment of women's dysfunctional uterine hemorrhage, and diseases such as postpartum hemorrhage have unique curative effect.Chinese Traditional Medicines with the Herba Blumeae Balsamiferae exploitation mainly are the FUXUEKANG particles that Nanning Gui Xi pharmaceutical factory produces at present, medicines such as FUXUEKANG capsule.Therefore, Herba Blumeae Balsamiferae is a herbal medicine among the people that has value of exploiting and utilizing.The experts and scholars of domestic each ambit have launched number of research projects to contained chemical ingredients of this plant and drug effect.Stigmasterol, epifriedelinol, suberone, brown eleostearic acid ethyl ester, Ethyl Stearate, coffic acid, β-Gu Zaichun, tricin, tricin 7-O-β-D-glucopyranoside, apigenin, apigenin 7-O-β-D-glucopyranoside, Reseda odorata, luteolin 7-O-β-compounds such as D-glucopyranoside have therefrom been found.But the still rare both at home and abroad at present relevant research report of the concrete chemical ingredients of Herba Blumeae Balsamiferae aspect pharmacologically active.Particularly also very limited to the correlative study of the contained polysaccharose substance of Herba Blumeae Balsamiferae plant.
Various studies show that, glucide have various biological function, as having unique effects at aspect such as anticancer, antitumor, antiviral, anti-ageing, hypoglycemic.Because the biological activity of polysaccharide is very extensive and cytotoxic effect is little, aspect the multiple diseases such as cancer therapy, treating diabetes and anti-virus infection suitable notable therapeutic effect is being arranged.People are to polysaccharide, and particularly herbal polysaccharide has carried out deep research and application, and its biological significance has been subjected to extensive concern, become one of the world of medicine's hot fields.
Summary of the invention
The invention provides a kind of preparation method who from the Herba Blumeae Balsamiferae plant, extracts blumea riparia water-soluble polysaccharides.So that the concrete chemical ingredients of clear and definite Herba Blumeae Balsamiferae performance anastalsis in diseases such as treatment women dysfunctional uterine hemorrhage, postpartum hemorrhage, for further research and the drug development utilization of Herba Blumeae Balsamiferae plant provides reference frame.
The present invention is as follows for the technical scheme that solves the problems of the technologies described above:
One of preparation method of blumea riparia water-soluble polysaccharides comprises the steps:
(1) extracts: each deionized water or the distilled water that adds 15 times of weight of the dried medicinal material of Herba Blumeae Balsamiferae is decocted, totally 2 times, each 3 hours, filter merging filtrate.
(2) membrane sepn: the filtrate of extracting is carried out micro-filtration and ultra-filtration and separation with hollow tubular ceramic microfiltration membrane and the organic ultra-filtration membrane of hollow tubular, obtain molecular weight ranges 10 3To 10 4Between parting liquid, this parting liquid is evaporated to about 0.1g/mL for 60 ℃ with Rotary Evaporators.
(3) deproteinated: under ice bath and agitation condition, adding weight concentration is 20% trichloroacetic acid solution, makes the weight concentration of trichoroacetic acid(TCA) in the polysaccharide soln system reach 5%, centrifugal removal vegetable-protein precipitation after the standing over night.
(4) desalination: the supernatant liquor after centrifugal is neutralized to pH with the NaOH solution of 1mol/L and equals 7; Be evaporated to about 0.2~0.5g/mL, be cooled to that to add dehydrated alcohol concentration of ethanol to the solution after the room temperature be 75~80%, in 5 ℃ of refrigerators, leave standstill and make salt precipitation, centrifugation remove sedimentary trichoroacetic acid(TCA) to receive salt; After the supernatant liquor evaporated under reduced pressure removed ethanol, with 100mL deionized water or dissolved in distilled water.
(5) decolouring: with the polysaccharide soln behind above-mentioned desalination and the removal ethanol, separate with the decolouring of DEAE Anion exchange column chromatography,, collect sugary soln with deionized water wash-out polysaccharide, be evaporated to sugared content 0.5g/mL, get the pale brown look cotton-shaped Crude polysaccharides of preliminary purification through lyophilize.
(6) refining: that the Crude polysaccharides of (5) is dissolved in the 10mL deionized water, behind 0.45 μ m micropore filtering film filtration under diminished pressure, cross Sephadex G-10 gel chromatography separation and remove remaining salt and other small molecular weight impurities, utilize Sephadex G-50 gel chromatography to carry out purifying again, with the ultrapure water is moving phase, quantitatively receive through automatic part receptor, UV spectrum detects, merge unimodal part solution, this solution decompression is concentrated into sugared content 0.5~1.0g/mL, through lyophilize, obtain the purified blumea riparia water-soluble polysaccharides.
The preparation method's of blumea riparia water-soluble polysaccharides two comprises the steps:
(1) extracts: each deionized water or the distilled water that adds 10 times of weight of the dried medicinal material of Herba Blumeae Balsamiferae is decocted, totally 3 times, each 2 hours, filter merging filtrate.
(2) membrane sepn: the filtrate of extracting is carried out micro-filtration and ultra-filtration and separation with hollow tubular ceramic microfiltration membrane and the organic ultra-filtration membrane of hollow tubular, obtain molecular weight ranges 10 3To 10 4Between parting liquid, this parting liquid is evaporated to about 0.2g/mL.
(3) deproteinated: under condition of ice bath, adding concentration while stirring is 20% trichloroacetic acid solution, makes the concentration of trichoroacetic acid(TCA) reach 5%, centrifugal removal vegetable-protein precipitation after the standing over night in 5 ℃ of refrigerators; Supernatant liquor is neutralized to pH with the NaOH solution of 1mol/L and equals 7, and the concentrating under reduced pressure after-filtration is removed sedimentary salinity.
(4) silica gel column chromatography separates: with the about 0.5g/mL of polysaccharide concentrated solution behind the deproteinated., evenly admix 200 order silica gel evaporated under reduced pressure after, sample is crossed silicagel column on the dry method, presses different ratios blended solution system gradient elution with methyl alcohol and ethyl acetate.Collection contains the sugar moieties elutriant, and evaporated under reduced pressure is also filtered with the water dissolution of about 50mL after having removed methyl alcohol and ethyl acetate, gets the pale brown look Crude polysaccharides of preliminary purification through lyophilize.
(5) decolouring: the deionized water that Crude polysaccharides is dissolved in 5 times of weight.Separate with the decolouring of DEAE Anion exchange column chromatography, with deionized water wash-out polysaccharide.Collect sugary soln, be evaporated to about 0.1g/mL.
(6) dialysis: with the polysaccharide concentrated solution molecular weight cut-off of decolouring is 10 3The dialysis tubing flowing water dialysis 48h of Da, deionized water dialysis 24h removes and desalts and small molecular weight impurity.Solution to 0.5 in the concentrating under reduced pressure dialysis tubing~1.0g/mL.
(7) refining: with the polysaccharide concentrated solution with 0.45 μ m micropore filtering film filtration under diminished pressure after, utilize Sephadex G-50 gel chromatography to be further purified again, with the ultrapure water is moving phase, quantitatively receive through automatic part receptor, UV spectrum detects, merge unimodal part solution, the concentrating under reduced pressure postlyophilization obtains the purified blumea riparia water-soluble polysaccharides.
One of above-mentioned preparation method and preparation method two in, described step (2) membrane sepn: used membrane separation plant is that the outstanding film engineering of Hefei generation limited liability company produces, and the molecular weight cut-off of ceramic microfiltration membrane is 10 5Da, the molecular weight cut-off of organic ultra-filtration membrane is respectively 10 4Da and 10 3Da.
One of above-mentioned preparation method and preparation method two in, described concentrating under reduced pressure all utilizes Rotary Evaporators to concentrate not being higher than under 60 ℃ of conditions reduction vaporization.
Being characterized as of the blumea riparia water-soluble polysaccharides of one of above-mentioned preparation method and preparation method's two preparations: (a) Herba Blumeae Balsamiferae polysaccharide outward appearance is a white cotton shape solid, be the simple component of molecular weight distribution homogeneous, its number-average molecular weight and weight-average molecular weight are respectively 2654 and 2716; (b) blumea riparia water-soluble polysaccharides is made up of seminose and fructose.
The blumea riparia water-soluble polysaccharides of one of above-mentioned preparation method and preparation method's two preparations has hemostatic function, can be used for treating diseases such as women's dysfunctional uterine hemorrhage, postpartum hemorrhage.
Advantage of the present invention is:
1. the present invention is used in combination method separation and purification water-soluble polysaccharides such as membrane sepn, silica gel column chromatography and gel column chromatography, has advantages such as technical process is simple, energy efficient.
2. product purity is higher, steady quality; Particularly in multiple calcium experiment of blood coagulation and the experiment of small white mouse isolated uterine, possesses significant styptic activity effect.
Description of drawings
Fig. 1 is the GPC gel permeation chromatography figure of blumea riparia water-soluble polysaccharides of the present invention.
Fig. 2 is the uv-spectrogram of blumea riparia water-soluble polysaccharides of the present invention.
Fig. 3 is the infared spectrum of blumea riparia water-soluble polysaccharides of the present invention.
Fig. 4 is the high performance liquid chromatography of blumea riparia water-soluble polysaccharides of the present invention.
Fig. 5 is the high performance liquid chromatography of standard monose.
Embodiment
Composition analysis to blumea riparia water-soluble polysaccharides of the present invention:
1. blumea riparia water-soluble polysaccharides molecular weight distribution test
Blumea riparia water-soluble polysaccharides is adopted gel permeation chromatography (GPC) analysis, as. shown in Figure 1, single symmetrical peak type shows that this polysaccharide is the simple component of molecular weight distribution homogeneous, is standard specimen with the polysaccharide of known molecular amount, and sets up the GPC calibration curve.The number-average molecular weight and the weight-average molecular weight of trying to achieve this polysaccharide according to the standard correction curve are respectively 2654 and 2716.
2. UV spectrum detects
Blumea riparia water-soluble polysaccharides is carried out UV spectrum to be detected: get the about 1mg of Herba Blumeae Balsamiferae polysaccharide, add suitable quantity of water and dissolve, in wavelength 200~600nm scope, scan, with deionized water as blank.Do not have absorption through UV scanning 280nm place, as shown in Figure 2, determine not contain polypeptide, protein.
3. infrared spectra detects
Blumea riparia water-soluble polysaccharides is carried out infrared spectra to be detected: get the about 2mg of purifying exsiccant blumea riparia water-soluble polysaccharides sample, add an amount of KBr and be ground to carefully, compressing tablet is measured infrared spectra.As shown in Figure 3, collection of illustrative plates shows that blumea riparia water-soluble polysaccharides is at 4000~500cm -1The charateristic avsorption band that has β-furans glucide in the scope.
4. monose compositional analysis
Blumea riparia water-soluble polysaccharides is carried out the monose compositional analysis: blumea riparia water-soluble polysaccharides utilizes efficient liquid phase chromatographic analysis as shown in Figure 4 after the sulfuric acid complete hydrolysis.By contrasting, as shown in Figure 5, confirm that blumea riparia water-soluble polysaccharides is made of fructose and seminose with monose mark product such as D-glucose, D-seminose, D-fructose, L-rhamnosyls.
Below in conjunction with real two embodiment of the present invention the present invention is elaborated.But need to prove that embodiment does not constitute the restriction to the claimed scope of the present invention.
Embodiment 1
Blumea riparia water-soluble polysaccharides preparation method one, operation steps are as follows successively:
1. extract: the each deionized water that adds 15 times of weight of the dried medicinal material of 3.0kg Herba Blumeae Balsamiferae is decocted 2 times, each 3 hours, filter merging filtrate.
2. membrane sepn: utilize membrane separation plant to carry out rough segmentation, it is 10 that the filtrate that step 1 is extracted is crossed molecular weight cut-off 5The ceramic membrane of Da, molecular weight is less than 10 5The filtrate of Da is 10 by molecular weight cut-off 4The organic membrane of Da, it is 10 that filtrate is continued by molecular weight cut-off 3The organic membrane of Da obtains molecular weight ranges 10 3To 10 4Between trapped fluid, be evaporated to 500mL.
(3) deproteinated: under ice bath and agitation condition, add weight concentration and be 20% the about 170mL of trichloroacetic acid solution, make that the trichoroacetic acid(TCA) weight concentration is the sedimentary vegetable-protein of centrifugal removal after 5%, 5 ℃ of refrigerator standing over night in the solution system.
4. desalination: the supernatant liquor behind the deproteinated is neutralized to the pH value with the NaOH solution of 1mol/L and equals 7, concentrate polysaccharide soln to sugared content 0.5g/mL, be cooled to and add dehydrated alcohol to the alcohol concn of solution after the room temperature and be about 75~80%, make trichoroacetic acid(TCA) sodium salt precipitation, leave standstill 12h in 5 ℃ of refrigerators, centrifugally remove sedimentary salt.After the supernatant liquor evaporated under reduced pressure removed ethanol, with 100mL deionized water or dissolved in distilled water.
5. decolouring: the polysaccharide soln behind above-mentioned desalination and the removal ethanol is decoloured with the DEAE Anion exchange column chromatography.With deionized water wash-out polysaccharide component.Be evaporated to the about 0.5g/mL of sugared content.Get the light yellow cotton-shaped Crude polysaccharides of 4g preliminary purification through lyophilize.
6. refining: will decolouring completely, Crude polysaccharides is dissolved in about 10mL deionized water, behind the micropore filtering film filtration under diminished pressure with 0.45 μ m, cross the SephadexG-10 gel column chromatography, separate and remove remaining salt and other small molecular weight impurities, utilize Sephadex G-50 gel chromatography to carry out purifying again, with the ultrapure water is moving phase, quantitatively receives through automatic part receptor, and UV spectrum detects.Merge unimodal part solution, lyophilize gets the purified blumea riparia water-soluble polysaccharides of 2.70g.
Embodiment 2
Blumea riparia water-soluble polysaccharides preparation method two, operation steps are as follows successively:
1. extract: the each distilled water that adds 10 times of weight of the dried medicinal material of 3.0kg Herba Blumeae Balsamiferae is decocted 3 times, each 2 hours, filter merging filtrate.
2. membrane sepn: utilize membrane separation plant to carry out rough segmentation, it is 10 that the filtrate that step 1 is extracted is crossed molecular weight cut-off 5The ceramic membrane of Da, molecular weight is less than 10 5The filtrate of Da is 10 by molecular weight cut-off 4The organic membrane of Da, it is 10 that filtrate is continued by molecular weight cut-off 3The organic membrane of Da obtains molecular weight ranges 10 3To 10 4Between trapped fluid, be evaporated to 500mL.
3. deproteinated: under condition of ice bath, adding weight concentration while stirring is the about 170mL of 20% trichloroacetic acid solution, makes the weight concentration of trichoroacetic acid(TCA) reach 5%, the sedimentary vegetable-protein of centrifugal removal after the refrigerator standing over night.Supernatant liquor is concentrated into the about 0.2 gram g/mL after-filtration of 50mL and removes sedimentary salinity with the NaOH solution neutralization of 1mol/L.
4. silica gel column chromatography separates: with the about 0.5g/mL of Deproteinated polysaccharide concentrated solution, evenly admix 100g silica gel (200 order) evaporated under reduced pressure, sample is crossed silicagel column on the dry method, with methyl alcohol and the ethyl acetate mixed system gradient elution by 1: 4,2: 3,3: 2 and 4: 1 different ratioss.Collection merges methyl alcohol, ethyl acetate is the sugary soln of 4: 1 moving phase wash-out, with about 50mL water dissolution and filtration, gets the pale brown look Crude polysaccharides of 6g preliminary purification through lyophilize after evaporated under reduced pressure methyl alcohol and the ethyl acetate.
5. decolouring: Crude polysaccharides is dissolved in the 30mL deionized water, decolours with the DEAE Anion exchange column chromatography.With deionized water eluting water soluble polysaccharide.Collect sugary soln and be evaporated to 80mL.
6. dialysis: is 10 with the polysaccharide concentrated solution of decolouring with the dialysis tubing molecular weight cut-off 3Da flowing water dialysis 48h, deionized water dialysis 24h, desalination and small molecular weight impurity.Solution decompression in the dialysis tubing is concentrated into 10mL.
7. refining: as with utilizing Sephadex G-50 gel chromatography to be further purified again behind the micropore filtering film filtration under diminished pressure of polysaccharide concentrated solution with 0.45 μ m, to be moving phase with the ultrapure water, quantitatively to receive that UV spectrum detects through automatic part receptor.Merge unimodal part solution, concentrate postlyophilization, obtain the purified blumea riparia water-soluble polysaccharides of 3.15g.

Claims (6)

1. one of preparation method of a blumea riparia water-soluble polysaccharides is characterized in that comprising the steps:
(1) extracts: each deionized water or the distilled water that adds 15 times of weight of the dried medicinal material of Herba Blumeae Balsamiferae is decocted, totally 2 times, each 3 hours, filter merging filtrate;
(2) membrane sepn: the filtrate of extracting is carried out micro-filtration and ultra-filtration and separation with hollow tubular ceramic microfiltration membrane and the organic ultra-filtration membrane of hollow tubular, obtain molecular weight ranges 10 3To 10 4Between parting liquid, this parting liquid is evaporated to about 0.1g/mL for 60 ℃ with Rotary Evaporators;
(3) deproteinated: under ice bath and agitation condition, the adding weight concentration is 20% trichloroacetic acid solution, makes the weight concentration of trichoroacetic acid(TCA) in the polysaccharide soln system reach 5%, centrifugal removal vegetable-protein precipitation after the standing over night;
(4) desalination: the supernatant liquor after centrifugal is neutralized to pH with the NaOH solution of 1mol/L and equals 7; Be evaporated to about 0.2~0.5g/mL, be cooled to that to add dehydrated alcohol concentration of ethanol to the solution after the room temperature be 75~80%, in 5 ℃ of refrigerators, leave standstill and make salt precipitation, centrifugation remove sedimentary trichoroacetic acid(TCA) to receive salt; After the supernatant liquor evaporated under reduced pressure removed ethanol, with 100mL deionized water or dissolved in distilled water;
(5) decolouring: with the polysaccharide soln behind above-mentioned desalination and the removal ethanol, separate with the decolouring of DEAE Anion exchange column chromatography,, collect sugary soln with deionized water wash-out polysaccharide, be evaporated to sugared content 0.5g/mL, get the pale brown look cotton-shaped Crude polysaccharides of preliminary purification through lyophilize;
(6) refining: that the Crude polysaccharides of (5) is dissolved in the 10mL deionized water, behind 0.45 μ m micropore filtering film filtration under diminished pressure, cross Sephadex G-10 gel chromatography separation and remove remaining salt and other small molecular weight impurities, utilize Sephadex G-50 gel chromatography to carry out purifying again, with the ultrapure water is moving phase, quantitatively receive through automatic part receptor, UV spectrum detects, merge unimodal part solution, this solution decompression is concentrated into sugared content 0.5~1.0g/mL, through lyophilize, obtain the purified blumea riparia water-soluble polysaccharides.
2. the preparation method's of a blumea riparia water-soluble polysaccharides two, it is characterized in that comprising the steps:
(1) extracts: each deionized water or the distilled water that adds 10 times of weight of the dried medicinal material of Herba Blumeae Balsamiferae is decocted, totally 3 times, each 2 hours, filter merging filtrate;
(2) membrane sepn: the filtrate of extracting is carried out micro-filtration and ultra-filtration and separation with hollow tubular ceramic microfiltration membrane and the organic ultra-filtration membrane of hollow tubular, obtain molecular weight ranges 10 3To 10 4Between parting liquid, this parting liquid is evaporated to about 0.2g/mL;
(3) deproteinated: under condition of ice bath, adding concentration while stirring is 20% trichloroacetic acid solution, makes the concentration of trichoroacetic acid(TCA) reach 5%, centrifugal removal vegetable-protein precipitation after the standing over night in 5 ℃ of refrigerators; Supernatant liquor is neutralized to pH with the NaOH solution of 1mol/L and equals 7, and the concentrating under reduced pressure after-filtration is removed sedimentary salinity;
(4) silica gel column chromatography separates: with the about 0.5g/mL of polysaccharide concentrated solution behind the deproteinated., evenly admix 200 purpose silica gel evaporated under reduced pressure after, sample is crossed silicagel column on the dry method, presses different ratios blended solution system gradient elution with methyl alcohol and ethyl acetate.Collection contains the sugar moieties elutriant, and evaporated under reduced pressure is also filtered with the water dissolution of about 50mL after having removed methyl alcohol and ethyl acetate, gets the pale brown look Crude polysaccharides of preliminary purification through lyophilize;
(5) decolouring: the deionized water that Crude polysaccharides is dissolved in 5 times of weight.Separate with the decolouring of DEAE Anion exchange column chromatography, with deionized water wash-out polysaccharide.Collect sugary soln, be evaporated to about 0.1g/mL;
(6) dialysis: with the polysaccharide concentrated solution molecular weight cut-off of decolouring is 10 3The dialysis tubing flowing water dialysis 48h of Da, deionized water dialysis 24h removes and desalts and small molecular weight impurity.Solution to 0.5 in the concentrating under reduced pressure dialysis tubing~1.0g/mL;
(7) refining: with the polysaccharide concentrated solution with 0.45 μ m micropore filtering film filtration under diminished pressure after, utilize Sephadex G-50 gel chromatography to be further purified again, with the ultrapure water is moving phase, quantitatively receive through automatic part receptor, UV spectrum detects, merge unimodal part solution, the concentrating under reduced pressure postlyophilization obtains the purified blumea riparia water-soluble polysaccharides.
3. according to claim 1 or the described a kind of preparation method of claim 2, it is characterized in that described step (2) membrane sepn: the molecular weight cut-off of used ceramic microfiltration membrane is 10 with blumea riparia water-soluble polysaccharides of styptic activity effect 5Da, the molecular weight cut-off of organic ultra-filtration membrane is respectively 10 4Da and 10 3Da.
4. according to claim 1 or the described a kind of preparation method of claim 2, it is characterized in that described concentrating under reduced pressure all utilizes Rotary Evaporators to concentrate not being higher than under 60 ℃ of conditions reduction vaporization with blumea riparia water-soluble polysaccharides of styptic activity effect.
5. according to claim 1 or the described a kind of preparation method of claim 2 with blumea riparia water-soluble polysaccharides of styptic activity effect, it is characterized in that, being characterized as of the blumea riparia water-soluble polysaccharides of this method preparation: (a) Herba Blumeae Balsamiferae polysaccharide outward appearance is a white cotton shape solid, be the simple component of molecular weight distribution homogeneous, its number-average molecular weight and weight-average molecular weight are respectively 2654 and 2716; (b) blumea riparia water-soluble polysaccharides is made up of seminose and fructose.
6. according to claim 1 or the described a kind of preparation method of claim 2 with blumea riparia water-soluble polysaccharides of styptic activity effect, it is characterized in that, the blumea riparia water-soluble polysaccharides of this method preparation has hemostatic function, can be used for treating diseases such as women's dysfunctional uterine hemorrhage, postpartum hemorrhage.
CN2009101146404A 2009-12-17 2009-12-17 Method for preparing blumea riparia water-soluble polysaccharides Expired - Fee Related CN101709093B (en)

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Cited By (5)

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CN102512344A (en) * 2011-12-28 2012-06-27 中国热带农业科学院热带作物品种资源研究所 Blumea balsamifera extract, preparation method and application thereof in oral care and clean product
CN107475215A (en) * 2017-09-06 2017-12-15 成都晟博源生物工程有限公司 A kind of extracting method of phosphorylase B
CN109627352A (en) * 2018-11-26 2019-04-16 吉林化工学院 A kind of decoloration process of corn silk polysaccharide
CN113082068A (en) * 2021-05-13 2021-07-09 广西壮族自治区食品药品检验所 Method for extracting blumea riparia active extract and application of blumea riparia active extract in preparing medicine for treating dysfunctional uterine bleeding
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CN101181329A (en) * 2007-11-28 2008-05-21 广西万寿堂药业有限公司 Total chromocor extract of blumea riparia as well as pharmaceutical composition and preparing method thereof
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Publication number Priority date Publication date Assignee Title
CN102512344A (en) * 2011-12-28 2012-06-27 中国热带农业科学院热带作物品种资源研究所 Blumea balsamifera extract, preparation method and application thereof in oral care and clean product
CN102512344B (en) * 2011-12-28 2013-06-05 中国热带农业科学院热带作物品种资源研究所 Blumea balsamifera extract, preparation method and application thereof in oral care and clean product
CN107475215A (en) * 2017-09-06 2017-12-15 成都晟博源生物工程有限公司 A kind of extracting method of phosphorylase B
CN109627352A (en) * 2018-11-26 2019-04-16 吉林化工学院 A kind of decoloration process of corn silk polysaccharide
CN113082068A (en) * 2021-05-13 2021-07-09 广西壮族自治区食品药品检验所 Method for extracting blumea riparia active extract and application of blumea riparia active extract in preparing medicine for treating dysfunctional uterine bleeding
CN113801798A (en) * 2021-08-02 2021-12-17 广西大学 Arthrospora adenantha A50 strain, exopolysaccharide produced by same and application thereof
CN113801798B (en) * 2021-08-02 2023-07-28 广西大学 Acidocella adephagia strain A50, extracellular polysaccharide produced by same and application thereof

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