CN101407557B - Preparation and use of Dendrobium nobile polysaccharide extract - Google Patents
Preparation and use of Dendrobium nobile polysaccharide extract Download PDFInfo
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Abstract
The invention provides a preparation method of dendrobium nobile polysaccharide extracts, which is realized by steps of degreasing, extracting, alcohol precipitating, protein removing, monose and oligosaccharide removing and purifying gel columns and the like. The polysaccharide content in the polysaccharide extract is more than 93 percent. The polysaccharide extract has remarkable oxidation prevention activity, can be combined with medicament excipients and carriers permitted by preparation agents, and can be applied in preparing medicaments or medicament combinations for treating and preventing cardiovascular diseases. The preparation method of the dendrobium nobile polysaccharide extracts is reasonable in design and convenient in operation.
Description
Technical field
The present invention relates to a kind of Chinese medical extract, be specifically related to a kind of preparation method and application of Dendrobium nobile polysaccharide extract.
Background technology
The stem of noble dendrobium is a rare traditional Chinese medicine commonly used, is the general designation of the fresh or dry stem of the orchid family (Orchidaceae) Dendrobium (Dendrobium Sw.) various plants.Dendrobium is bigger genus in the orchid, about 1100 kinds of the whole world, and China has an appointment 76 kinds.Stem of noble dendrobium beginning is stated from Shennong's Herbal, classified as top grade, effect such as have nourishing Yin and clearing heat, reinforcing stomach reg fluid, moisten the lung and relieve the cough." Chinese pharmacopoeia version in 2005 has been recorded three kinds of dendrobium stem (D.nobileLindl.), Herba Dendrobii (D.officinale Kimura et Migo) and stem of Eyeshaped Dendrobium (D.fimbriatum Hook.).
The modern chemistry pharmacological research shows that dendrobium stem mainly contains polyose, alkaloids, and phenols isoreactivity material, wherein the polyose composition has the inhibition tumour, strengthens or the recovery immunologic function effect such as hypoglycemic grade.Drawbacks such as the research of dendrobium polysaccharide at present exists basic substance indeterminate, and quality is uncontrollable, and separation purifying technique is coarse, it is high to lack active component content, specific chemical components, significant document of drug activity and patent report.And, do not see appearance on the market about the medicine or the pharmaceutical composition of Dendrobium nobile polysaccharide yet.
Summary of the invention
The object of the present invention is to provide a kind of Dendrobium nobile polysaccharide extract; Mainly contain Dendrobium nobile polysaccharide in the described Dendrobium nobile polysaccharide extract; Wherein, by weight percentage, the content of Dendrobium nobile polysaccharide is more than 93%; The content of preferred polysaccharide is 95%-98%, realizes through following steps:
(1) degreasing: get the dendrobium stem medicine materical crude slice, doubly measure organic solvent with 8-15 and soak back backflow 1-3 time, filter, volatilize organic solvent and get the dregs of a decoction;
(2) extract: after the above-mentioned dregs of a decoction were soaked, 50 ℃ of water-baths were extracted, and filter, and the dregs of a decoction add 100 ℃ of extractions of water, filtered, and concentrated filtrate extremely every ml is equivalent to contain crude drug 0.5-2.0g;
(3) alcohol precipitation: in above-mentioned liquid concentrator, add an amount of ethanol, ice bath is placed, and filters, and gets polyoses extract bullion I after the deposition lyophilize;
(4) remove albumen: it is soluble in water in right amount to get above-mentioned polyoses extract bullion I, and adding volume ratio is the chloroform of 5:1: propyl carbinol, stir the back layering; After upper strata repetitive operation 4-8 time, add an amount of ethanol, ice bath is placed; Filter, the deposition lyophilize gets polyoses extract bullion II;
(5) remove monose and oligosaccharides: it is soluble in water in right amount to get above-mentioned polyoses extract bullion II; (end molecular weight: 8000-14000) dialysis was taken out the interior liquid of dialysis tubing and is added an amount of ethanol after 2 days, and ice bath is placed with dialysis membrane; Filter, get polyoses extract bullion III after the deposition lyophilize;
(6) gel column purifying: above-mentioned polyoses extract bullion III is used the gel chromatography column purification, follow the tracks of cut with the sulfuric acid phynol method, after the collection main peak merges, add an amount of ethanol, ice bath is placed, and filters, and the deposition lyophilize gets Dendrobium nobile polysaccharide extract.
Organic solvent in the step (1) is selected a kind of in sherwood oil, ETHYLE ACETATE, ethanol or the high concentration ethanol aqueous solution for use.
The dregs of a decoction described in the step (2) are soaked, and amount of water is that 4-10 doubly measures, and preferred 8-10 doubly measures.
In step (3)-(6), described adding ethanol, wherein the alcoholic acid volumn concentration is 50%-80%, preferred content is 70%-80%.
In step (3)-(6), described ice bath storage period is more than 12 hours, and preferred ice bath storage period is 24 hours.
Another object of the present invention is to provide the application of described Dendrobium nobile polysaccharide extract in preparation treatment and preventing cardiovascular disease medicine.
Drug prepared also contains preparation allowable pharmaceutical excipients or carrier.
Usefulness of the present invention is the quality controllable of the activeconstituents Dendrobium nobile polysaccharide that extracts, and content is high, specific chemical components, and drug activity is remarkable.The separation purifying technique of preparation method of extract of the present invention is reasonable in design, and is easy and simple to handle.The appearance of medicine provided by the invention or pharmaceutical composition is for Dendrobium nobile polysaccharide provides medicinal use widely.
Embodiment
To combine embodiment to further specify flesh and blood of the present invention and beneficial effect below, this embodiment only is used to the present invention is described but not limitation of the present invention.
The preparation of embodiment one Dendrobium nobile polysaccharide extract
(1) degreasing: get the dendrobium stem medicine materical crude slice,, filter, volatilize organic solvent and get the dregs of a decoction with refluxing 2 times after 8 times of amount alcohol immersion; (2) extract: after the above-mentioned dregs of a decoction added 10 times of amount immersions of water, 50 ℃ of water-baths were extracted, and filter, and the dregs of a decoction add 10 times of water gagings, and 100 ℃ are extracted 3 times, and each 1 hour, filter, concentrated filtrate extremely every ml is equivalent to contain crude drug 1.0g; (3) alcohol precipitation: in above-mentioned liquid concentrator, adding an amount of ethanol to ethanol content is 80%, and ice bath was placed 12 hours, filters, and gets polyoses extract bullion I after the deposition lyophilize; (4) remove albumen: it is soluble in water in right amount to get above-mentioned polyoses extract bullion I, adds an amount of chloroform and propyl carbinol, stirs the back layering; After the upper strata repetitive operation 4 times, adding an amount of ethanol to ethanol content is 80%, and ice bath was placed 12 hours; Filter, the deposition lyophilize gets polyoses extract bullion II; (5) remove monose and oligosaccharides: it is soluble in water in right amount to get above-mentioned polyoses extract bullion II; (end molecular weight: 8000-14000) dialysis is after 2 days with dialysis membrane; It is 70% that the interior liquid of taking-up dialysis tubing adds an amount of ethanol to ethanol content; Ice bath was placed 12 hours, filtered, and got polyoses extract bullion III after the deposition lyophilize; (6) gel column purifying: above-mentioned polyoses extract bullion III is used the gel chromatography column purification, follow the tracks of cut, after the collection main peak merges with the sulfuric acid phynol method; Adding an amount of ethanol to ethanol content is 70%, and ice bath is placed, and filters; The deposition lyophilize gets white Dendrobium nobile polysaccharide extract.It is 93% that phenol sulfuric acid process mensuration polysaccharide gets content, and the bradford method is measured albumen and is respectively 0.8%.
The preparation of embodiment two Dendrobium nobile polysaccharide extracts
(1) degreasing: get the dendrobium stem medicine materical crude slice,, filter, volatilize organic solvent and get the dregs of a decoction with refluxing 2 times after 10 times of amount 80% alcohol immersion; (2) extract: after the above-mentioned dregs of a decoction added 8 times of amount immersions of water, 50 ℃ of water-baths were extracted 2 times, and each 1 hour, filter, the dregs of a decoction add 8 times of water gagings, and 100 ℃ of water-baths are extracted 2 times, and each 1 hour, filter, concentrated filtrate extremely every ml is equivalent to contain crude drug 1.5g; (3) alcohol precipitation: in above-mentioned liquid concentrator, adding an amount of ethanol to ethanol content is 80%, and ice bath was placed 24 hours, filters, and gets polyoses extract bullion I after the deposition lyophilize; (4) remove albumen: it is soluble in water in right amount to get above-mentioned polyoses extract bullion I, adds an amount of chloroform and propyl carbinol, stirs the back layering; After the upper strata repetitive operation 8 times, adding an amount of ethanol to ethanol content is 80%, and ice bath was placed 24 hours; Filter, the deposition lyophilize gets polyoses extract bullion II; (5) remove monose and oligosaccharides: it is soluble in water in right amount to get above-mentioned polyoses extract bullion II; (end molecular weight: 8000-14000) dialysis is after 2 days with dialysis membrane; It is 80% that the interior liquid of taking-up dialysis tubing adds an amount of ethanol to ethanol content; Ice bath was placed 24 hours, filtered, and got polyoses extract bullion III after the deposition lyophilize; (6) gel column purifying: above-mentioned polyoses extract bullion III is used the gel chromatography column purification, follow the tracks of cut, after the collection main peak merges with the sulfuric acid phynol method; Adding an amount of ethanol to ethanol content is 80%, and ice bath was placed 24 hours, filters; The deposition lyophilize gets white polysaccharide CP50 elaboration.It is 94% that phenol sulfuric acid process mensuration polysaccharide gets content, and the bradford method is measured albumen and is respectively 0.6%.
The preparation of embodiment three Dendrobium nobile polysaccharide extracts
(1) degreasing: take by weighing stem of noble dendrobium medicinal material 4kg (dry product, block medicine materical crude slice), add 8 times of amounts of 80% ethanol and soak 3 hours (W/V), 85 ℃ were refluxed 2 times 5 hours.Filter, the dregs of a decoction are divided, and volatilize ethanol; (2) extract: the above-mentioned dregs of a decoction are waved to there not being the alcohol flavor, add 4 times of amount zero(ppm) water (W/V), soak 12 hours, and 50 ℃ of water-baths were extracted 2 times 2 hours.Four layers of gauze B suction filtration, the dregs of a decoction continue to add 4 times of amount zero(ppm) water (W/V), 100 ℃ of boiling water extraction 2 hours, 2 times.Four layers of gauze B filter, and collect filtrating, merge, and are concentrated into 3000ml in 60 ℃ of rotary evaporations; (3) alcohol precipitation: add about 9000ml absolute ethyl alcohol to above-mentioned liquid concentrator, be adjusted to 80% ethanol content with vinometer, ice bath was placed 24 hours, flocks occurred, and with four layers of gauze B suction filtration, the deposition lyophilize gets polyoses extract bullion I; (4) remove albumen: take by weighing above-mentioned polyoses extract bullion I5.0g, be dissolved in the 500ml zero(ppm) water, add CHCl
3100ml, propyl carbinol 20ml, electronic stirring 30 minutes, separating funnel left standstill 10 minutes, and isolated for disposal subnatant, upper strata liquid repeat deproteinated operation 6 times.Afterwards, upper strata liquid adds absolute ethyl alcohol to 80%, and ice bath was placed 24 hours, and is centrifugal, and the deposition lyophilize gets polyoses extract bullion II; (5) remove monose and oligosaccharides: get above-mentioned polyoses extract bullion II and be dissolved in right amount in the 300ml zero(ppm) water, (end molecular weight: 8000~14000) dialysis, dialysis tubing external application magnetic agitation at the uniform velocity stirs, and changes water 1 time in per 2 hours, dialyses 2 days with dialysis membrane.Liquid takes out and adds absolute ethyl alcohol to 80% in the dialysis tubing, and ice bath 24 hours is centrifugal, gets gray precipitate, and lyophilize gets polyoses extract bullion III; (6) gel column purifying: above-mentioned polyoses extract bullion III with Deae sepharose FF gel chromatography column purification, is followed the tracks of cut with the sulfuric acid phynol method, after the collection main peak merges; Add an amount of ethanol to 80%, ice bath is placed, and filters; The deposition lyophilize gets white polysaccharide CP50 elaboration.It is 96% that phenol sulfuric acid process mensuration polysaccharide gets content, and the bradford method is measured albumen and is respectively 0.5%.
Embodiment four neonatal rat myocardial cell H
2O
2Damage model
Use the pure DMSO melt into concentration of top grade to be 50mg/mL Dendrobium nobile polysaccharide extract, jolting, centrifugal.Store down at-20 ℃, subsequent use.At first carry out cell cultures.The quantity of safeguarding cell can supply to screen used to guarantee it, but cell count can not be too many, otherwise can influence the growth of cell, regularly change liquid and go down to posterity it.H
9C
2Be attached cell, change liquid and only need inhale the nutrient solution supernatant, wash one time, add fresh medium again and get final product with PBS.Go down to posterity to inhale and remove the nutrient solution supernatant, wash one time with PBS, use trysinization, add nutrient solution again and stop digestion, centrifugal going down to posterity get final product (nutrient solution is that DMEM (high sugared)+10%FBS (G)+1% non-essential amino acid+0.1% pair resists).Reach one regularly Deng cell quantity, just can plant plate, for dosing is prepared.In culturing bottle, blow and beat cell dispersion, transfer to mixed solution in the centrifuge tube, draw a little and on hematimeter, expect blue method of exclusion counting with platform, centrifugal 10 minutes remaining (900rpm) inhales and removes supernatant.Add an amount of nutrient solution again, piping and druming disperses the cell mixing gently, draws an amount of nutrient solution and joins in the cell groove, makes cell density be about 1 * 10
4Individual/0.15mL.Cell suspension is added on the 96 porocyte culture plates uniformly every hole 0.15mL with the octal road volley of rifle fire.After planting plate, be put in the constant temperature cell culture incubator and cultivate after 24 hours, it is carried out H
2O
2The manufacturing of damage model.Get plate, draw supernatant, wash one time, remove supernatant with PBS.Dosing is with H is arranged
2O
2Nutrient solution dilutes medicine, makes that the component drug final concentration is 50 μ g/mL, and the positive drug final concentration is 50 μ mol/mL, H
2O
2Final concentration be 200 μ mol/mL.With 96 orifice plates put into incubator (37 ℃, 5%CO
2, 21%O
2), get plate after 24 hours, mtt assay is surveyed cell activity.With the positive medicine of the VC of 50 μ mol/mL.Treatment rate=(each dosing group A value-DMSO group A value)/(DMSO group A value-blank control group A value) * 100%, the result sees table 1.
Table 1 neonatal rat myocardial cell H
2O
2Damage model
Embodiment five neonatal rat myocardial cell anoxic reoxygenation models
Use the pure DMSO melt into concentration of top grade to be 50mg/mL Dendrobium nobile polysaccharide extract, jolting, centrifugal.Store down at-20 ℃, subsequent use.At first carry out cell cultures.The quantity of safeguarding cell can supply to screen used to guarantee it, but cell count can not be too many, otherwise can influence the growth of cell, regularly change liquid and go down to posterity it.H
9C
2Be attached cell, change liquid and only need inhale the nutrient solution supernatant, wash one time, add fresh medium again and get final product with PBS.Go down to posterity to inhale and remove the nutrient solution supernatant, wash one time with PBS, use trysinization, add nutrient solution again and stop digestion, centrifugal going down to posterity get final product (nutrient solution is that DMEM (high sugared)+10%FBS (G)+1% non-essential amino acid+0.1% pair resists).Reach one regularly Deng cell quantity, just can plant plate, for dosing is prepared.In culturing bottle, blow and beat cell dispersion, transfer to mixed solution in the centrifuge tube, draw a little and on hematimeter, expect blue method of exclusion counting with platform, centrifugal 10 minutes remaining (900rpm) inhales and removes supernatant.Add an amount of nutrient solution again, piping and druming disperses the cell mixing gently, draws an amount of nutrient solution and joins in the cell groove, makes cell density be about 1 * 10
4Individual/0.15mL.Cell suspension is added on the 96 porocyte culture plates uniformly every hole 0.15mL with the octal road volley of rifle fire.After planting plate, be put in the constant temperature cell culture incubator and cultivate after 24 hours, it is carried out the manufacturing of anoxia model.Get some sugar-free Hank ' s, logical N
210 minutes, get plate, draw supernatant, use sugar-free Hank ' s to wash one time, remove supernatant.Dosing uses sugar-free Hank ' s that medicine is diluted, and makes that the component drug final concentration is 50 μ g/mL, and the positive drug final concentration is 50 μ mol/mL.96 orifice plates are put into closed environment, vacuumize, logical N
2, make its inner hypoxia that guarantees, put into three gas incubators (37 ℃, 5%CO
2, 5%O
2).Anoxic 6 hours.After 6 hours, get plate, supernatant 10 μ L are got in every hole, survey LDH.Upper plate draws unnecessary supernatant after taking out supernatant 10 μ L, add nutrient solution (low sugar DMEM+FBS), and dosing is supplied again, and making every hole contain amount of liquid is 100 μ L, and makes that the component drug final concentration is 50 μ g/mL, and the positive drug final concentration is 50 μ mol/mL.Put into constant incubator (37 ℃, 5%CO2).Hatched 4 hours.After 4 hours, get plate, supernatant 10 μ L are got in every hole, survey LDH.Get a cell groove, R1 and R2 in the LDH test kit are mixed with 2:1, mixed solution is joined in 96 orifice plates of need measuring with the octal road volley of rifle fire, every hole 300 μ L are hatched under 37 ℃.Set a series of time points, measure the LDH value at the 340nm place.With the positive medicine of the VC of 50 μ mol/mL.Press treatment rate=(DMSO group A value-each dosing group A value)/DMSO group A value * 100%, the results are shown in Table 2.
Table 2 neonatal rat myocardial cell anoxic reoxygenation model experiment result
The preparation of embodiment six pills
Get Dendrobium nobile polysaccharide extract 0.5g and 10.5g polyoxyethylene glycol-6000 mixes, heating and melting moves in the dripping pill drip irrigation after changing material, and in ℃ whiteruss of medicine liquid droplet to 6~8, oil removing makes 300 of dripping pills.
The preparation of embodiment seven lyophilized injectable powders
Get Lignum Dalbergiae Odoriferae oil 1.5g, join in the saturated hydroxypropyl of 13ml, stirring and dissolving filters, and the filtrating cryodrying gets the inclusion compound powder of Lignum Dalbergiae Odoriferae oil and hydroxypropyl.Except that above-mentioned Lignum Dalbergiae Odoriferae oil closes the inclusion compound powder of hydroxypropyl, get Dendrobium nobile polysaccharide extract 0.5g, N.F,USP MANNITOL 5.5g, Calcium Disodium Edetate 0.9g and zero(ppm) water 2ml again, behind the said components mixing, lyophilize, 350 of packing promptly get.
The preparation of embodiment eight tablets
Get that Dendrobium nobile polysaccharide extract is an amount of to mix with Microcrystalline Cellulose, add 3% polyvidone ethanolic soln system softwood, cross 18 mesh sieve system particles, 60 ℃ of dryings 1 hour, whole, the adding talcum powder is an amount of, mixing, compressing tablet promptly gets.
The preparation of embodiment nine capsules
Get Dendrobium nobile polysaccharide extract and peanut oil and stir in the filling in stainless steel in the ratio of 2:18 is water-soluble, add an amount of gelatin and glycerine simultaneously and mix, emit and use the colloidal mill defibrination again, the mixed solution that grinds stirs, and processes soup; Under 40-50 ℃ of temperature, stir glycerine and zero(ppm) water miscible; Again with the glycerin liquid temperature to 80-90 ℃, get gelatin and add wherein to mix and stir, become glue until off-bottom; Glue was left standstill 4 hours, process offset plate with laminator and supply the pill operation to use; Above-mentioned soup of processing and offset plate are sent into the pellet press pill, did cylinder typing in 4 hours at 22-25 ℃ of temperature katabatic wind then, again dry 16-20 hour of 25-30 ℃ of temperature katabatic wind; The qualified capsule and pill of pick; Clean with 95% ethanol,, promptly get dry 4 hours of 25-30 ℃ of katabatic wind.
The preparation of embodiment ten injections
Get Dendrobium nobile polysaccharide extract in right amount with 40 ℃ of water for injection dissolvings, add an amount of pharmaceutical carrier isotonic agent, the pH value of regulator solution is 7.0-8.0, adds to the full amount of water for injection; Remove thermal source with the ultra-fine filter ultrafiltration, after the mensuration pH value, use membrane filtration, after the packing; Autoclaving, check, packing promptly get.
Claims (6)
1. the preparation method of a Dendrobium nobile polysaccharide extract contains Dendrobium nobile polysaccharide in the described Dendrobium nobile polysaccharide extract, and by weight percentage, the content of Dendrobium nobile polysaccharide is 93%-98%, realizes through following steps:
(1) degreasing: get the dendrobium stem medicine materical crude slice, doubly measure organic solvent with 8-15 and soak back backflow 1-3 time, filter, volatilize organic solvent and get the dregs of a decoction;
(2) extract: after getting the above-mentioned dregs of a decoction and soaking, 50 ℃ of water-baths are extracted, and filter, and the dregs of a decoction add 100 ℃ of extractions of water, and wherein amount of water is that the 4-10 of the dregs of a decoction doubly measures, and filter, and concentrated filtrate is equivalent to contain crude drug 0.5-2.0g to every ml;
(3) alcohol precipitation: in above-mentioned liquid concentrator, add ethanol, ice bath is placed, and filters, and gets polyoses extract bullion I after the deposition lyophilize;
(4) remove albumen: it is soluble in water to get above-mentioned polyoses extract bullion I, adds volume ratio and be 5: 1 chloroform: propyl carbinol, stir the back layering, and after upper strata repetitive operation 4-8 time, add ethanol, ice bath is placed, and filters, and the deposition lyophilize gets polyoses extract bullion II;
(5) remove monose and oligosaccharides: it is soluble in water to get above-mentioned polyoses extract bullion II; After dialysing 2 days by the dialysis membrane of molecular weight: 8000-14000, take out the interior liquid of dialysis tubing and add ethanol, ice bath is placed; Filter, get polyoses extract bullion III after the deposition lyophilize;
(6) gel column purifying: above-mentioned polyoses extract bullion III is used the gel chromatography column purification, follow the tracks of cut with the sulfuric acid phynol method, after the merging of collection main peak, add ethanol, ice bath is placed, and filters, and precipitates lyophilize, gets white Dendrobium nobile polysaccharide extract;
The alcoholic acid volumn concentration is 50%-80% in said step (3)-(6).
2. the preparation method of a kind of Dendrobium nobile polysaccharide extract according to claim 1 is characterized in that: the used organic solvent of step (1) is selected a kind of in sherwood oil, ETHYLE ACETATE, ethanol or the high concentration ethanol aqueous solution for use.
3. the preparation method of a kind of Dendrobium nobile polysaccharide extract according to claim 1, it is characterized in that: the described dregs of a decoction of step (2) are soaked, and wherein amount of water is that the 8-10 of the dregs of a decoction doubly measures.
4. the preparation method of a kind of Dendrobium nobile polysaccharide extract according to claim 1, it is characterized in that: the adding ethanol described in step (3)-(6), wherein the alcoholic acid volumn concentration is 70%-80%.
5. the preparation method of a kind of Dendrobium nobile polysaccharide extract according to claim 1 is characterized in that: be more than 12 hours the ice bath storage period described in step (3)-(6).
6. the Dendrobium nobile polysaccharide extract that preparation method according to claim 1 obtains is preparing treatment and prevention because of myocardial cell H
2O
2Application in the cardiovascular disease medicine that damage or myocardial cell's anoxic cause.
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| 林萍等.石斛属植物药理活性研究进展.《中草药》.2003,第34卷(第11期),附19-22页. * |
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| CN101407557A (en) | 2009-04-15 |
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