CN105838752A - Method for simultaneously preparing ginkgolide B and quercetin by tremella aurantialba - Google Patents
Method for simultaneously preparing ginkgolide B and quercetin by tremella aurantialba Download PDFInfo
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Abstract
The invention discloses a method for simultaneously preparing ginkgolide B and quercetin by tremella aurantialba. The method includes: sequentially performing test tube expanding culture, liquid shake culture, seed tank expanding culture, solid primary fermentation culture, liquid secondary fermentation culture, extraction and separation to obtain a fermentation liquor containing the ginkgolide B and mycelia containing the quercetin; respectively extracting the fermentation liquor containing the ginkgolide B and the mycelia containing the quercetin to obtain the ginkgolide B and quercetin crystal. By addition of ginkgo biloba extract into a solid matrix made from husked ginkgos and rice and by taking the tremella aurantialba as a strain, conversion of ginkgolide and ginkgetin is realized through solid primary fermentation; by secondary fermentation, the quercetin and the ginkgolide B are separated, industrial large-scale production can be realized, and simultaneous production of the ginkgolide B and the quercetin is realized as well; technical simplicity is achieved, ginkgolide B purity of products is larger than 90%, quercetin purity of the products is larger than 95%, and high purity is realized.
Description
Technical field
The present invention relates to technical field of bioengineering, be specifically related to one and utilize Tremella aurantialba Bandoni et Zang to prepare ginkalide B and Mongolian oak simultaneously
The method of Pi Su.
Background technology
At present, research proves that bilobalide is one of active component main in Folium Ginkgo, is the special effective blood of class
Platelet activation factor (Platelet activating factor) receptor antagonist.Platelet activating factor (PAF) is by blood
A kind of endogenous phosphide that platelet and inflammation tissue secretion produce, is the maximally effective platelet aggregation induction having now been found that
Agent, closely related with the Emergence and Development of numerous disease.Bilobalide, as paf receptor specific antagonists, has medicine widely
Reason effect.Research find ginkalide B to central nervous system and the protected effect of ischemic injuries, shock, antiallergic, antibacterial
Rejection in antiinflammatory action, and anti-organ transplantation.The most also find that ginkalide B can reduce hepatic portal vein pressure, improves
System vascular toleration, illustrates that it has certain curative effect to liver cirrhosis.Bilobalide has therapeutical effect for injury of kidney.These are made
With all relevant as paf receptor antagonists with ginkalide B, and it be presently believed to be effect the strongest, most have clinical should
With native platelets activation factor (PAF) receptor antagonist of prospect.
Quercetin and derivant thereof are that plant kingdom is widely distributed, have the flavone compound of various biological activity.
In recent years, domestic and international medical personal is increasing to the research of Quercetin, finds that it has many pharmacologically actives, such as antioxidation
And scavenging activated oxygen effect, anti-fibrosis effect, antitumor action, can reduce blood pressure, Ischemic myocardium reperfusion injury,
Antiviral, analgesia and antidiarrheal etc., and Quercetin is to human non-toxic, harmless, without carcinogenic, without lethal, without the advantages such as teratogenesis, state
Once tried out in the treatment of multiple disease outward, achieved good effect.Quercetin is present in the many flower of plant, leaf, fruit,
Many presented in glycoside, such as rutin, quercitrin, hyperin etc., these glycosides generally prepare Quercetin through acid hydrolysis.Few use
Biological method prepares Quercetin.
Scholar is had to propose herb fermenting pharmaceutical technology in recent years.So-called herb fermenting pharmaceutical technology is to inherit Chinese medicine
Concoct on the basis of learning fermentation method, drawn Microecology achievement, formed in conjunction with the fermentation technique of modern biological project
High-tech herbal pharmaceutical new technique, be in terms of Chinese medicine (natural drug) pharmacy find medicine new curative effect.Traditional Chinese medicine
Mostly fermentation is to carry out under conditions of natural, and present herb fermenting pharmaceutical technology is to fully absorb Tiny ecosystem in modern age
Learn, bionic achievement in research and gradually form.
Commonly used in prior art ginkalide B and Quercetin are utilized respectively simple process for separation and purification obtain
Substantial amounts of ginkalide B and Quercetin, separation efficiency is low, it is impossible to is applicable to industrialization large-scale production, and individually purifies
Separation method is more backward, and production cost is higher.
Inventor, through further investigation and industrialized production test repeatedly, finds out industrially scalable and produces in Semen Ginkgo simultaneously
Ester B and Quercetin technology, no matter the present invention from the mode of production and the product of production of product, is different from conventional patent and literary composition
The content of chapter report, a kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to produce ginkalide B and Quercetin.
Summary of the invention
, problem to be solved
For the above-mentioned problems in the prior art, the present invention provides one to utilize Tremella aurantialba Bandoni et Zang to prepare ginkalide B and Mongolian oak simultaneously
The method of Pi Su, it adds Folium Ginkgo extract with peeling Semen Ginkgo and rice for solid matrix, passes through solid with Tremella aurantialba Bandoni et Zang for strain
Primary fermentation, converts bilobalide and ginkgetin, by after fermentation, makes Quercetin and ginkalide B be separated, can realize work
Industry large-scale production, it is possible to simultaneously produce ginkalide B and Quercetin;Technique is simple, and in obtained product, Semen Ginkgo
Lactone B purity is more than 90%, and Quercetin purity is more than 95%, and the purity produced is higher.
, technical scheme
In order to solve the problems referred to above, the technical solution adopted in the present invention is as follows:
A kind of described method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin, described preparation method is with rice, peeling
Semen Ginkgo and Folium Ginkgo extract are primary raw material, with Tremella aurantialba Bandoni et Zang as starting strain, sequentially pass through test tube amplification culture, liquid shaking bottle training
Support and seed tank amplification culture, the cultivation of solid primary fermentation, liquid post-fermentation and culture and extraction separating step prepare containing in Semen Ginkgo
The fermentation liquid of ester B and the mycelium containing Quercetin;The described fermentation liquid containing ginkalide B and the mycelium containing Quercetin
Preparing ginkalide B and Quercetin crystal respectively through extracting again, wherein ginkalide B purity reaches 90%, and Quercetin purity reaches
To 95%.
Preferably, described preparation method comprises the steps:
A1 test tube amplification culture: cultivate in slant strains is inoculated in potato dextrose medium in Tremella aurantialba Bandoni et Zang, prepares gold
Ear test tube slant strain;
A2 liquid submerged culture: the Tremella aurantialba Bandoni et Zang test tube slant strain obtained by step A1 is inoculated into equipped with liquid submerged culture base
In shaking flask, cultivate, prepare golden fungus liquid shaking flask strain;
A3 seed tank amplification culture: the golden fungus liquid shaking flask strain obtained by step A2 is inoculated in seed tank culture base and carries out
Cultivate, make Tremella aurantialba Bandoni et Zang seed tank strain;
A4 solid primary fermentation is cultivated: is inoculated in solid medium by the Tremella aurantialba Bandoni et Zang seed tank strain obtained by step A3, and mixes
Uniformly, carry out fermentation culture, prepare Tremella aurantialba Bandoni et Zang solid fermentation thing;
A5 liquid post-fermentation and culture: the Tremella aurantialba Bandoni et Zang solid primary fermentation thing obtained by step A4 is transferred to liquid fermentation tank culture medium
In, carry out liquid after fermentation, prepare the fermentation liquid containing ginkalide B and the tremella filament containing Quercetin;
A6 extracts separation: by the tremella filament containing Quercetin obtained by step A5 and the fermentation liquid containing ginkalide B
Respectively through extraction, obtain Quercetin and ginkalide B crystal.
Preferably, described preparation method is specific as follows:
B1 test tube amplification culture: slant strains in Tremella aurantialba Bandoni et Zang test tube is cut into 3 × 3 mm fritter strains, inoculates a fritter oblique to test tube
In the culture medium of face, cultivating 4~15 days for 20~35 DEG C, prepare test tube slant strain, 4 DEG C, this test tube slant saves backup;
B2 liquid submerged culture: the test tube slant strain obtained by step B1 is cut into 3 × 3 mm fritter strains, picking 3~10
Block is inoculated in the 250mL triangular flask equipped with 20~150mL liquid submerged culture bases, triangular flask rotating speed be 50~200 turns/
Point, under conditions of temperature 20~35 DEG C, 18-86h cultivated by shaking table, makes liquid shaking bottle strain;
B3 seed tank amplification culture: the liquid shaking bottle strain obtained by step B2 is inoculated in seed tank amplification culture base, and
Described liquid shaking bottle strain and seed tank amplification culture base are the inoculum concentration inoculation of 1~20% by volume, are 20~35 in temperature
DEG C, speed of agitator is 50~160 revs/min, the volume being passed through gas per minute and seed tank amplification culture base volume ratio for for
Under the conditions of the ventilation of 0.2~1.8:1, cultivate 18~96h, make Tremella aurantialba Bandoni et Zang seed tank strain;
B4 solid primary fermentation is cultivated: access the Tremella aurantialba Bandoni et Zang seed tank strain obtained by step B3 equipped with solid primary fermentation culture medium
In culture bag, and described Tremella aurantialba Bandoni et Zang seed tank strain is 2~10% with the culture bag equipped with solid primary fermentation culture medium by volume
Inoculum concentration is inoculated, and in temperature 20~35 DEG C, humidity 80% primary fermentation 20~40 days, wherein every 3~6 days, turns over bag once, prepares
Solid primary fermentation thing;
B5 liquid post-fermentation and culture: the solid primary fermentation thing obtained by step B4 is crushed to 20 mesh, joins liquid fermentation tank
In culture medium, described liquid fermentation tank culture volume is 5~10 with the weight ratio of solid primary fermentation thing, is 20~43 in temperature
DEG C, speed of agitator is 50~160 revs/min, at the volume being passed through gas per minute with liquid fermentation tank culture volume ratio is
Fermentation 24~72h under the conditions of the ventilation of 0.2-1.8:1, obtained fermented liquid is under the conditions of 2000~6000 revs/min
The centrifugal fermentation liquid prepared containing ginkalide B and the mycelium containing Quercetin;
B6 extracts separation: by the tremella filament containing Quercetin obtained by step A5 and the fermentation liquid containing ginkalide B
Respectively through extraction, obtain Quercetin and ginkalide B crystal.
Preferably, liquid submerged culture base described in step B2 is sterilizing 90~360 min under the conditions of 100~130 DEG C
Prepare, and containing wheat bran 5~20g, the raw material of rice 5~20g in every liter of liquid submerged culture base.
Preferably, the base of seed tank amplification culture described in step B3 is sterilizing 90~360 under the conditions of 100~130 DEG C
Min prepares, and containing wheat bran 5~20g, the raw material of rice 5~20g in every liter of liquid submerged culture base.
Preferably, the culture medium of solid primary fermentation described in step B4 is sterilizing 90~360 under the conditions of 100~130 DEG C
Min prepares, and containing peeling Semen Ginkgo 200~400g, Folium Ginkgo extract 30~50g in each kilogram of solid primary fermentation culture medium
Raw material with rice 750~570g.
Preferably, the raw material in described solid primary fermentation culture medium is mixed with water in the ratio of 1:0.6~1.5.
Preferably, liquid fermentation medium described in step B5 is sterilizing 30~60 min system under the conditions of 100~130 DEG C
Obtain, and every liter of liquid fermentation medium contains 5~40g glucoses, 0.5~4g peptone and 0.01~0.1gK2HPO4 。
Preferably, from the tremella filament containing Quercetin, Quercetin crystal is produced described in step A6 or step B6
Method comprises the steps:
Obtained tremella filament is dried by C1, is then crushed to 20 mesh, the 60 of 5~20 times of volumes of addition mycelium weight
~the ethanol of 100%, repeatedly extract 3~5 times, obtain extracting solution one;
Extracting solution one obtained by step C1 is merged by C2, is then evaporated to the 1/30 of original volume, adds residual volume 5 times
Water, under the conditions of 4 DEG C crystallize 3~18 hours, then sucking filtration is dried, and i.e. obtains Quercetin crystal, and Quercetin purity is more than
95%。
Preferably, from the fermentation liquid containing ginkalide B, ginkalide B crystalline substance is produced described in step A6 or step B6
The method of body comprises the steps:
D1 is by the fermentation liquid concentrating under reduced pressure of obtained ginkalide B and is dried and to obtain product;
D2 adds 60~100% alcohol reflux 3~5 times of 5~20 times of weight in step D1 products therefrom, obtains extraction
Liquid two;
Extracting solution two obtained by step D2 is merged by D3, is then evaporated to the 1/40 of original volume, ties under the conditions of-20 DEG C
Brilliant 3~18 hours;
Product after step D3 is crystallized by D4 carries out sucking filtration, and sucking filtration gained filtering residue ethyl acetate is redissolved, then by ethyl acetate
Decompression is concentrated to dryness mutually, then redissolves with dehydrated alcohol, and adds the water of 3~10 times of volumes, precipitation, sucking filtration, and gained filtering residue is dried
Being ginkalide B, its purity is more than 90%.
, beneficial effect
Compared to prior art, the invention have the benefit that
(1) present invention is on the basis of drawing herb fermenting pharmaceutical technology, respective in conjunction with modern solid-state fermentation and liquid fermentation
Advantage, uses solid-state primary fermentation to convert Semen Ginkgo active component flavone and bilobalide, overcomes substrate (silver during liquid fermentation
The active component of Folium Pruni) inhibitory action to Tremella aurantialba Bandoni et Zang mycelial growth, utilize submerged fermentation technology simultaneously, Tremella aurantialba Bandoni et Zang is by ginkalide B
It is secreted into extracellular and flavone is changed into Quercetin and is accumulated in intracellular, ginkalide B is separated with Quercetin;
(2) a kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin of the present invention, is not simple utilization
Process for separation and purification obtains substantial amounts of ginkalide B and Quercetin, but adds silver with peeling Semen Ginkgo and rice for solid matrix
Folium Pruni extract, with Tremella aurantialba Bandoni et Zang for strain by solid primary fermentation, converts bilobalide and ginkgetin, by after fermentation, makes Mongolian oak
Pi Su and ginkalide B are separated, and can realize industrialization large-scale production, it is possible to produce ginkalide B and Cortex querci dentatae simultaneously
Element;
(3) a kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin of the present invention, technique is simple, and institute
In the product obtained, ginkalide B purity is more than 90%, and Quercetin purity is more than 95%, and the purity produced is higher.
Accompanying drawing explanation
Fig. 1 is the preparation stream of a kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin of the present invention
Journey schematic diagram.
Detailed description of the invention
Below in conjunction with specific embodiment, the present invention is further described below.
Embodiment 1
As it is shown in figure 1, a kind of method utilizing Tremella aurantialba Bandoni et Zang to prepare ginkalide B and Quercetin specifically includes following steps simultaneously:
(1) test tube amplification culture: slant strains in Tremella aurantialba Bandoni et Zang test tube is cut into 3 × 3 mm fritter strains, inoculates a fritter to test tube
In slant medium, cultivating 15 days for 20 DEG C, prepare test tube slant strain, 4 DEG C, this test tube slant saves backup;
(2) liquid submerged culture: the test tube slant strain obtained by step (1) is cut into 3 × 3 mm fritter strains, picking 10 pieces
Being inoculated in the 250mL triangular flask equipped with 150mL liquid submerged culture base, triangular flask is 50 revs/min at rotating speed, temperature 35 DEG C
Under the conditions of, 18h cultivated by shaking table, makes liquid shaking bottle strain;Described liquid submerged culture base is sterilizing 360 under the conditions of 130 DEG C
Min prepares, and containing wheat bran 5g, the raw material of rice 20g in every liter of liquid submerged culture base;
(3) seed tank amplification culture: the liquid shaking bottle strain obtained by step (2) is inoculated in seed tank amplification culture base,
And described liquid shaking bottle strain and the inoculum concentration inoculation that seed tank amplification culture base is 1% by volume, it is 35 DEG C in temperature, stirs
Mixing rotating speed is 160 revs/min, in the volume being passed through gas per minute and leading to that seed tank amplification culture base volume ratio is 0.2:1
Under the conditions of tolerance, cultivate 96h, make Tremella aurantialba Bandoni et Zang seed tank strain;Described seed tank amplification culture base is sterilizing under the conditions of 130 DEG C
360 min prepare, and containing wheat bran 5g, the raw material of rice 20g in every liter of liquid submerged culture base;
(4) solid primary fermentation is cultivated: access the Tremella aurantialba Bandoni et Zang seed tank strain obtained by step (3) equipped with solid primary fermentation culture medium
Culture bag in, and described Tremella aurantialba Bandoni et Zang seed tank strain be 10% by volume equipped with the culture bag of solid primary fermentation culture medium
Inoculum concentration is inoculated, and at temperature 20 DEG C, humidity 80% primary fermentation 40 days, wherein every 6 days, turns over bag once, prepares solid primary fermentation
Thing;Described solid primary fermentation culture medium is that sterilizing 360 min prepares under the conditions of 130 DEG C, and each kilogram of solid primary fermentation training
Support in base containing peeling Semen Ginkgo 200g, Folium Ginkgo extract 50g and the raw material of rice 750g;In described solid primary fermentation culture medium
Raw material mix with water in the ratio of 1:0.6;
(5) liquid post-fermentation and culture: the solid primary fermentation thing obtained by step (4) is crushed to 20 mesh, joins liquid fermentation
In tank culture medium, described liquid fermentation tank culture volume is 10 with the weight ratio of solid primary fermentation thing, is 20 DEG C in temperature, stirs
Mixing rotating speed is 50 revs/min, at the volume being passed through gas per minute with liquid fermentation tank culture volume than the ventilation for 0.2:1
Under the conditions of ferment 72h, obtained fermented liquid is centrifugal under the conditions of 2000 revs/min prepares the fermentation containing ginkalide B
Liquid and the mycelium containing Quercetin;Described liquid fermentation medium is that sterilizing 60 min prepares under the conditions of 130 DEG C, and every liter
Liquid fermentation medium contains 5g glucose, 4g peptone and 0.01gK2HPO4;
(6) separation is extracted: by the tremella filament containing Quercetin obtained by step (5) and the fermentation containing ginkalide B
Liquid, respectively through extraction, obtains Quercetin and ginkalide B crystal.
It should be noted that and from the tremella filament containing Quercetin, produce Quercetin crystal described in step (6)
Method comprises the steps:
Obtained tremella filament is dried by A1, is then crushed to 20 mesh, the 100% of 20 times of volumes of addition mycelium weight
Ethanol, repeatedly extract 3 times, obtain extracting solution one;
Extracting solution one obtained by step A1 is merged by A2, is then evaporated to the 1/30 of original volume, adds residual volume 5 times
Water, under the conditions of 4 DEG C crystallize 3 hours, then sucking filtration is dried, and i.e. obtains Quercetin crystal, and quercetin content is 95%.
In the present embodiment, from the fermentation liquid containing ginkalide B, ginkalide B crystal is produced described in step (6)
Method comprise the steps:
B1 is by the fermentation liquid concentrating under reduced pressure of obtained ginkalide B and is dried and to obtain product;
B2 adds 60% alcohol reflux 5 times of 20 times of weight in step B1 products therefrom, obtains extracting solution two;
Extracting solution two obtained by step B2 is merged by B3, is then evaporated to the 1/40 of original volume, ties under the conditions of-20 DEG C
Brilliant 18 hours;
Product after step B3 is crystallized by B4 carries out sucking filtration, and sucking filtration gained filtering residue ethyl acetate is redissolved, then by ethyl acetate
Decompression is concentrated to dryness mutually, then redissolves with dehydrated alcohol, and adds the water of 3 times of volumes, precipitation, sucking filtration, and gained filtering residue is dried and is
Ginkalide B, its content is 90%.
The mensuration of described quercetin content uses high performance liquid chromatography (Qi Ningli etc.: high performance liquid chromatography-two pole
Pipe array detection measures rutin and the content of Quercetin in Radix Et Rhizoma Fagopyri Tatarici simultaneously. food science and technology, and 2013,38 (10): 301-304):
Intersil ODS-SP C 18 post (150 mm × 4.6 mm, 5 μm), flowing is used (to use phosphorus for methanol-0.5% phosphoric acid solution mutually
Acid dihydride potassium regulation p H to 4.5) (40:60), flow velocity: 1.0 m L/min, column temperature: 35 DEG C, sample size: 10 μ L, detects ripple
Long 255 nm, using Quercetin standard substance as comparison, according to Quercetin and the corresponding peak area of variable concentrations, carry out recurrence and obtain
Quercetin concentration and face, peak relation equation, further according to Quercetin peak area in sample and extension rate and regression equation calculation sample
Middle quercetin content.
The mensuration of described ginkalide B content uses High Performance Liquid Chromatography/Mass Spectrometry: be furnished with high pressure binary pump, water this
996 diode array detector and Agilent 1200 series autosampler, chromatographic column BEH C-18 post (2.5 μm, 3.0 ×
100) high performance liquid chromatography (HPLC) is used for analyzing bilobalide.With first alcohol and water (7:3) as flowing phase, flow velocity is
0.2 mL/ min carries out eluting.Three grades of quadrupole rod mass spectrum 6400 ion trap mass spectrometers of Agilent, as detector, are born at full scan
The mode operation of ion electrospray ionization (ESI) (M/Z500-800).Ion trap mass spectrometer, condition ISO be: ESI,
Negative polarity ionizes;Spray voltage: 4.0 kilovolts;Heated capillary temperature: 275 DEG C;Sheath gas (N2 gas) flow velocity: 30 Arb;Auxiliary/
Purge gas (N2 gas);Flow velocity: 50 Arb.Using ginkalide B standard substance as comparison, according to the ginkalide B of variable concentrations with
Corresponding peak area, carries out recurrence and obtains ginkalide B concentration and face, peak relation equation, further according to face, ginkalide B peak in sample
Amass and ginkalide B content in extension rate and regression equation calculation sample.
Based on above-mentioned, invention, on the basis of drawing herb fermenting pharmaceutical technology, ferments in conjunction with modern solid-state
Advantage respective with liquid fermentation, uses solid-state primary fermentation to convert Semen Ginkgo active component flavone and bilobalide, overcomes liquid
The sweat mesostroma (active component of the Folium Ginkgo) inhibitory action to Tremella aurantialba Bandoni et Zang mycelial growth, utilizes submerged fermentation skill simultaneously
Art, ginkalide B is secreted into extracellular and flavone changes into Quercetin and is accumulated in intracellular by Tremella aurantialba Bandoni et Zang, by ginkalide B and
Quercetin separates;And the process for separation and purification that utilizes that the present invention is not simple obtains substantial amounts of ginkalide B and Quercetin, and
It is to add Folium Ginkgo extract for solid matrix removing the peel Semen Ginkgo and rice, with Tremella aurantialba Bandoni et Zang for strain by solid primary fermentation, converts
Bilobalide and ginkgetin, by after fermentation, make Quercetin and ginkalide B be separated, can realize industrialization extensive
Produce, it is possible to produce ginkalide B and Quercetin simultaneously;There is the simple advantage of technique, and in obtained product, Semen Ginkgo
Lactone B purity is more than 90%, and Quercetin purity is more than 95%, and the purity produced is higher.
Embodiment 2
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin specifically includes following steps:
(1) test tube amplification culture: slant strains in Tremella aurantialba Bandoni et Zang test tube is cut into 3 × 3 mm fritter strains, inoculates a fritter to test tube
In slant medium, cultivating 4 days for 35 DEG C, prepare test tube slant strain, 4 DEG C, this test tube slant saves backup;
(2) liquid submerged culture: the test tube slant strain obtained by step (1) is cut into 3 × 3 mm fritter strains, picking 3 pieces
Being inoculated in the 250mL triangular flask equipped with 20mL liquid submerged culture base, triangular flask is 200 revs/min at rotating speed, temperature 20 DEG C
Under the conditions of, 86h cultivated by shaking table, makes liquid shaking bottle strain;Described liquid submerged culture base is sterilizing 90 under the conditions of 100 DEG C
Min prepares, and containing bran 20g, the raw material of rice 5g in every liter of liquid submerged culture base;
(3) seed tank amplification culture: the liquid shaking bottle strain obtained by step (2) is inoculated in seed tank amplification culture base,
And described liquid shaking bottle strain and the inoculum concentration inoculation that seed tank amplification culture base is 20% by volume, it is 20 DEG C in temperature, stirs
Mixing rotating speed is 50 revs/min, at the volume being passed through gas per minute with seed tank amplification culture base volume ratio for for 0.2~1.8:1
Ventilation under the conditions of, cultivate 18h, make Tremella aurantialba Bandoni et Zang seed tank strain;Described seed tank amplification culture base is under the conditions of 100 DEG C
Sterilizing 90min prepares, and containing wheat bran 20g, the raw material of rice 5g in every liter of liquid submerged culture base;
(4) solid primary fermentation is cultivated: access the Tremella aurantialba Bandoni et Zang seed tank strain obtained by step (3) equipped with solid primary fermentation culture medium
Culture bag in, and described Tremella aurantialba Bandoni et Zang seed tank strain and the culture bag equipped with solid primary fermentation culture medium be 2% connect by volume
Plant amount inoculation, at temperature 35 DEG C, humidity 80% primary fermentation 20 days, wherein every 3 days, turn over bag once, prepare solid primary fermentation thing;
Described solid primary fermentation culture medium is that sterilizing 90min prepares under the conditions of 100 DEG C, and in each kilogram of solid primary fermentation culture medium
Containing peeling Semen Ginkgo 400g, Folium Ginkgo extract 30g and the raw material of rice 570g;Raw material in described solid primary fermentation culture medium
Mix with water in the ratio of 1:1.5;
(5) liquid post-fermentation and culture: the solid primary fermentation thing obtained by step (4) is crushed to 20 mesh, joins liquid fermentation
In tank culture medium, described liquid fermentation tank culture volume is 5 with the weight ratio of solid primary fermentation thing, is 35 DEG C in temperature, stirs
Mixing rotating speed is 160 revs/min, at the volume being passed through gas per minute with liquid fermentation tank culture volume than the ventilation for 1.8:1
Ferment under the conditions of amount 24h, and obtained fermented liquid centrifugal preparing under the conditions of 6000 revs/min contains sending out of ginkalide B
Ferment liquid and the mycelium containing Quercetin;Described liquid fermentation medium is that sterilizing 30min prepares under the conditions of 100 DEG C, and often
Rise liquid fermentation medium and contain 40g glucose, 0.5g peptone and 0.01gK2HPO4;
(6) separation is extracted: by the tremella filament containing Quercetin obtained by step (5) and the fermentation containing ginkalide B
Liquid, respectively through extraction, obtains Quercetin and ginkalide B crystal.
It should be noted that and from the tremella filament containing Quercetin, produce Quercetin crystal described in step (6)
Method comprises the steps:
Obtained tremella filament is dried by A1, is then crushed to 20 mesh, the 60% of 5 times of volumes of addition mycelium weight
Ethanol, repeatedly extracts 5 times, obtains extracting solution one;
Extracting solution one obtained by step A1 is merged by A2, is then evaporated to the 1/30 of original volume, adds residual volume 5 times
Water, under the conditions of 4 DEG C crystallize 18 hours, then sucking filtration is dried, and i.e. obtains Quercetin crystal, and quercetin content is 99.9%.
In the present embodiment, from the fermentation liquid containing ginkalide B, ginkalide B crystal is produced described in step (6)
Method comprise the steps:
B1 is by the fermentation liquid concentrating under reduced pressure of obtained ginkalide B and is dried and to obtain product;
B2 adds 60~100% alcohol reflux 3 times of 5 times of weight in step B1 products therefrom, obtains extracting solution two;
Extracting solution two obtained by step B2 is merged by B3, is then evaporated to the 1/40 of original volume, ties under the conditions of-20 DEG C
Brilliant 3 hours;
Product after step B3 is crystallized by B4 carries out sucking filtration, and sucking filtration gained filtering residue ethyl acetate is redissolved, then by ethyl acetate
Decompression is concentrated to dryness mutually, then redissolves with dehydrated alcohol, and adds the water of 10 times of volumes, precipitation, sucking filtration, and gained filtering residue is dried and is
Ginkalide B, its content is 99.8%.
Embodiment 3
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin specifically includes following steps:
(1) test tube amplification culture: slant strains in Tremella aurantialba Bandoni et Zang test tube is cut into 3 × 3 mm fritter strains, inoculates a fritter to test tube
In slant medium, cultivating 10 days for 28 DEG C, prepare test tube slant strain, 4 DEG C, this test tube slant saves backup;
(2) liquid submerged culture: the test tube slant strain obtained by step (1) is cut into 3 × 3 mm fritter strains, picking 7 pieces
Being inoculated in the 250mL triangular flask equipped with 80mL liquid submerged culture base, triangular flask is 120 revs/min at rotating speed, temperature 28 DEG C
Under the conditions of, 57h cultivated by shaking table, makes liquid shaking bottle strain;Described liquid submerged culture base is sterilizing 260 under the conditions of 120 DEG C
Min prepares, and containing wheat bran 13g, the raw material of rice 13g in every liter of liquid submerged culture base;
(3) seed tank amplification culture: the liquid shaking bottle strain obtained by step (2) is inoculated in seed tank amplification culture base,
And described liquid shaking bottle strain and the inoculum concentration inoculation that seed tank amplification culture base is 10% by volume, it is 28 DEG C in temperature, stirs
Mixing rotating speed is 110 revs/min, is the ventilation for 1:1 at the volume being passed through gas per minute and seed tank amplification culture base volume ratio
Under the conditions of amount, cultivate 57h, make Tremella aurantialba Bandoni et Zang seed tank strain;Described seed tank amplification culture base is sterilizing under the conditions of 120 DEG C
260 min prepare, and containing wheat bran 13g, the raw material of rice 13g in every liter of liquid submerged culture base;
(4) solid primary fermentation is cultivated: access the Tremella aurantialba Bandoni et Zang seed tank strain obtained by step (3) equipped with solid primary fermentation culture medium
Culture bag in, and described Tremella aurantialba Bandoni et Zang seed tank strain and the culture bag equipped with solid primary fermentation culture medium be 6% connect by volume
Plant amount inoculation, at temperature 28 DEG C, humidity 80% primary fermentation 30 days, wherein every 4.5 days, turn over bag once, prepare solid primary fermentation
Thing;Described solid primary fermentation culture medium is that sterilizing 260 min prepares under the conditions of 120 DEG C, and each kilogram of solid primary fermentation training
Support in base containing peeling Semen Ginkgo 300g, Folium Ginkgo extract 40g and the raw material of rice 660g;In described solid primary fermentation culture medium
Raw material mix with water in the ratio of 1:1;
(5) liquid post-fermentation and culture: the solid primary fermentation thing obtained by step (4) is crushed to 20 mesh, joins liquid fermentation
In tank culture medium, described liquid fermentation tank culture volume is 8 with the weight ratio of solid primary fermentation thing, is 27 DEG C in temperature, stirs
Mixing rotating speed is 110 revs/min, logical than for 0.2-1.8 of the volume being passed through gas per minute and liquid fermentation tank culture volume
Ferment under the conditions of tolerance 48h, and obtained fermented liquid is centrifugal under the conditions of 4000 revs/min to be prepared containing ginkalide B
Fermentation liquid and the mycelium containing Quercetin;Described liquid fermentation medium is that sterilizing 45 min prepares under the conditions of 120 DEG C, and
Every liter of liquid fermentation medium contains 23g glucose, 2.2g peptone and 0.05gK2HPO4;
(6) separation is extracted: by the tremella filament containing Quercetin obtained by step (5) and the fermentation containing ginkalide B
Liquid, respectively through extraction, obtains Quercetin and ginkalide B crystal.
It should be noted that and from the tremella filament containing Quercetin, produce Quercetin crystal described in step (6)
Method comprises the steps:
Obtained tremella filament is dried by A1, is then crushed to 20 mesh, the 80% of 13 times of volumes of addition mycelium weight
Ethanol, repeatedly extracts 4 times, obtains extracting solution one;
Extracting solution one obtained by step A1 is merged by A2, is then evaporated to the 1/30 of original volume, adds residual volume 5 times
Water, under the conditions of 4 DEG C crystallize 11 hours, then sucking filtration is dried, and i.e. obtains Quercetin crystal, and quercetin content is 98%.
In the present embodiment, from the fermentation liquid containing ginkalide B, ginkalide B crystal is produced described in step (6)
Method comprise the steps:
B1 is by the fermentation liquid concentrating under reduced pressure of obtained ginkalide B and is dried and to obtain product;
B2 adds 80% alcohol reflux 4 times of 13 times of weight in step B1 products therefrom, obtains extracting solution two;
Extracting solution two obtained by step B2 is merged by B3, is then evaporated to the 1/40 of original volume, ties under the conditions of-20 DEG C
Brilliant 11 hours;
Product after step B3 is crystallized by B4 carries out sucking filtration, and sucking filtration gained filtering residue ethyl acetate is redissolved, then by ethyl acetate
Decompression is concentrated to dryness mutually, then redissolves with dehydrated alcohol, and adds the water of 7 times of volumes, precipitation, sucking filtration, and gained filtering residue is dried and is
Ginkalide B, its content is 95%.
Embodiment 4
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin specifically includes following steps:
(1) test tube amplification culture: slant strains in Tremella aurantialba Bandoni et Zang test tube is cut into 3 × 3 mm fritter strains, inoculates a fritter to test tube
In slant medium, cultivating 12 days for 23 DEG C, prepare test tube slant strain, 4 DEG C, this test tube slant saves backup;
(2) liquid submerged culture: the test tube slant strain obtained by step (1) is cut into 3 × 3 mm fritter strains, picking 8 pieces
Being inoculated in the 250mL triangular flask equipped with 30mL liquid submerged culture base, triangular flask is 75 revs/min at rotating speed, temperature 20~35
Under conditions of DEG C, 30h cultivated by shaking table, makes liquid shaking bottle strain;Described liquid submerged culture base is sterilizing under the conditions of 100 DEG C
100 min prepare, and containing wheat bran 8g, the raw material of rice 12g in every liter of liquid submerged culture base;
(3) seed tank amplification culture: the liquid shaking bottle strain obtained by step (2) is inoculated in seed tank amplification culture base,
And described liquid shaking bottle strain and the inoculum concentration inoculation that seed tank amplification culture base is 4% by volume, it is 25 DEG C in temperature, stirs
Mixing rotating speed is 120 revs/min, in the volume being passed through gas per minute and leading to that seed tank amplification culture base volume ratio is 0.6:1
Under the conditions of tolerance, cultivate 35h, make Tremella aurantialba Bandoni et Zang seed tank strain;Described seed tank amplification culture base is sterilizing under the conditions of 100 DEG C
100 min prepare, and containing wheat bran 8g, the raw material of rice 15g in every liter of liquid submerged culture base;
(4) solid primary fermentation is cultivated: access the Tremella aurantialba Bandoni et Zang seed tank strain obtained by step (3) equipped with solid primary fermentation culture medium
Culture bag in, and described Tremella aurantialba Bandoni et Zang seed tank strain and the culture bag equipped with solid primary fermentation culture medium be 4% connect by volume
Plant amount inoculation, at temperature 22 DEG C, humidity 80% primary fermentation 25 days, wherein every 3 days, turn over bag once, prepare solid primary fermentation thing;
Described solid primary fermentation culture medium is that sterilizing 100 min prepares under the conditions of 100 DEG C, and each kilogram of solid primary fermentation culture medium
In containing peeling Semen Ginkgo 250g, Folium Ginkgo extract 35g and the raw material of rice 715g;Former in described solid primary fermentation culture medium
Material is mixed with water in the ratio of 1:0.6;
(5) liquid post-fermentation and culture: the solid primary fermentation thing obtained by step (4) is crushed to 20 mesh, joins liquid fermentation
In tank culture medium, described liquid fermentation tank culture volume is 6 with the weight ratio of solid primary fermentation thing, is 24 DEG C in temperature, stirs
Mixing rotating speed is 65 revs/min, at the volume being passed through gas per minute with liquid fermentation tank culture volume than the ventilation for 1.5:1
Under the conditions of ferment 60h, obtained fermented liquid is centrifugal under the conditions of 5000 revs/min prepares the fermentation containing ginkalide B
Liquid and the mycelium containing Quercetin;Described liquid fermentation medium is that sterilizing 50 min prepares under the conditions of 115 DEG C, and every liter
Liquid fermentation medium contains 30g glucose, 3g peptone and 0.09gK2HPO4;
(6) separation is extracted: by the tremella filament containing Quercetin obtained by step (5) and the fermentation containing ginkalide B
Liquid, respectively through extraction, obtains Quercetin and ginkalide B crystal.
It should be noted that and from the tremella filament containing Quercetin, produce Quercetin crystal described in step (6)
Method comprises the steps:
Obtained tremella filament is dried by A1, is then crushed to 20 mesh, the 95% of 18 times of volumes of addition mycelium weight
Ethanol, repeatedly extracts 3 times, obtains extracting solution one;
Extracting solution one obtained by step A1 is merged by A2, is then evaporated to the 1/30 of original volume, adds residual volume 5 times
Water, under the conditions of 4 DEG C crystallize 4 hours, then sucking filtration is dried, and i.e. obtains Quercetin crystal, Quercetin purity be more than 95%.
In the present embodiment, from the fermentation liquid containing ginkalide B, ginkalide B crystal is produced described in step (6)
Method comprise the steps:
B1 is by the fermentation liquid concentrating under reduced pressure of obtained ginkalide B and is dried and to obtain product;
B2 adds 95% alcohol reflux 4 times of 18 times of weight in step B1 products therefrom, obtains extracting solution two;
Extracting solution two obtained by step B2 is merged by B3, is then evaporated to the 1/40 of original volume, ties under the conditions of-20 DEG C
Brilliant 17 hours;
Product after step B3 is crystallized by B4 carries out sucking filtration, and sucking filtration gained filtering residue ethyl acetate is redissolved, then by ethyl acetate
Decompression is concentrated to dryness mutually, then redissolves with dehydrated alcohol, and adds the water of 9 times of volumes, precipitation, sucking filtration, and gained filtering residue is dried and is
Ginkalide B, its content is 92%.
Embodiment 5
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin specifically includes following steps:
(1) test tube amplification culture: slant strains in Tremella aurantialba Bandoni et Zang test tube is cut into 3 × 3 mm fritter strains, inoculates a fritter to test tube
In slant medium, cultivating 6 days for 32 DEG C, prepare test tube slant strain, 4 DEG C, this test tube slant saves backup;
(2) liquid submerged culture: the test tube slant strain obtained by step (1) is cut into 3 × 3 mm fritter strains, picking 4 pieces
Being inoculated in the 250mL triangular flask equipped with 40mL liquid submerged culture base, triangular flask is 160 revs/min at rotating speed, temperature 30 DEG C
Under the conditions of, 36h cultivated by shaking table, makes liquid shaking bottle strain;Described liquid submerged culture base is sterilizing 320 under the conditions of 128 DEG C
Min prepares, and containing wheat bran 6g, the raw material of rice 20g in every liter of liquid submerged culture base;
(3) seed tank amplification culture: the liquid shaking bottle strain obtained by step (2) is inoculated in seed tank amplification culture base,
And described liquid shaking bottle strain and the inoculum concentration inoculation that seed tank amplification culture base is 15% by volume, it is 30 DEG C in temperature, stirs
Mixing rotating speed is 160 revs/min, in the volume being passed through gas per minute and leading to that seed tank amplification culture base volume ratio is 0.6:1
Under the conditions of tolerance, cultivate 68h, make Tremella aurantialba Bandoni et Zang seed tank strain;Described seed tank amplification culture base is sterilizing under the conditions of 128 DEG C
320 min prepare, and containing wheat bran 15g, the raw material of rice 7g in every liter of liquid submerged culture base;
(4) solid primary fermentation is cultivated: access the Tremella aurantialba Bandoni et Zang seed tank strain obtained by step (3) equipped with solid primary fermentation culture medium
Culture bag in, and described Tremella aurantialba Bandoni et Zang seed tank strain and the culture bag equipped with solid primary fermentation culture medium be 6% connect by volume
Plant amount inoculation, at temperature 30 DEG C, humidity 80% primary fermentation 28 days, wherein every 5 days, turn over bag once, prepare solid primary fermentation thing;
Described solid primary fermentation culture medium is that sterilizing 320 min prepares under the conditions of 128 DEG C, and each kilogram of solid primary fermentation culture medium
In containing peeling Semen Ginkgo 350g, Folium Ginkgo extract 50g and the raw material of rice 600g;Former in described solid primary fermentation culture medium
Material is mixed with water in the ratio of 1:1.2;
(5) liquid post-fermentation and culture: the solid primary fermentation thing obtained by step (4) is crushed to 20 mesh, joins liquid fermentation
In tank culture medium, described liquid fermentation tank culture volume is 7 with the weight ratio of solid primary fermentation thing, is 30 DEG C in temperature, stirs
Mixing rotating speed is 120 revs/min, at the volume being passed through gas per minute with liquid fermentation tank culture volume than the ventilation for 1.6:1
Ferment under the conditions of amount 58h, and obtained fermented liquid centrifugal preparing under the conditions of 3000 revs/min contains sending out of ginkalide B
Ferment liquid and the mycelium containing Quercetin;Described liquid fermentation medium is that sterilizing 60 min prepares under the conditions of 128 DEG C, and often
Rise liquid fermentation medium and contain 35g glucose, 0.5g peptone and 0.04gK2HPO4;
(6) separation is extracted: by the tremella filament containing Quercetin obtained by step (5) and the fermentation containing ginkalide B
Liquid, respectively through extraction, obtains Quercetin and ginkalide B crystal.
It should be noted that and from the tremella filament containing Quercetin, produce Quercetin crystal described in step (6)
Method comprises the steps:
Obtained tremella filament is dried by A1, is then crushed to 20 mesh, the 90% of 18 times of volumes of addition mycelium weight
Ethanol, repeatedly extracts 4 times, obtains extracting solution one;
Extracting solution one obtained by step A1 is merged by A2, is then evaporated to the 1/30 of original volume, adds residual volume 5 times
Water, under the conditions of 4 DEG C crystallize 12 hours, then sucking filtration is dried, and i.e. obtains Quercetin crystal, and quercetin content is 96%.
In the present embodiment, from the fermentation liquid containing ginkalide B, ginkalide B crystal is produced described in step (6)
Method comprise the steps:
B1 is by the fermentation liquid concentrating under reduced pressure of obtained ginkalide B and is dried and to obtain product;
B2 adds 70% alcohol reflux 5 times of 8 times of weight in step B1 products therefrom, obtains extracting solution two;
Extracting solution two obtained by step B2 is merged by B3, is then evaporated to the 1/40 of original volume, ties under the conditions of-20 DEG C
Brilliant 6 hours;
Product after step B3 is crystallized by B4 carries out sucking filtration, and sucking filtration gained filtering residue ethyl acetate is redissolved, then by ethyl acetate
Decompression is concentrated to dryness mutually, then redissolves with dehydrated alcohol, and adds the water of 4 times of volumes, precipitation, sucking filtration, and gained filtering residue is dried and is
Ginkalide B, its content is 92%.
Embodiment 6
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin specifically includes following steps:
(1) test tube amplification culture: slant strains in Tremella aurantialba Bandoni et Zang test tube is cut into 3 × 3 mm fritter strains, inoculates a fritter to test tube
In slant medium, cultivating 5 days for 32 DEG C, prepare test tube slant strain, 4 DEG C, this test tube slant saves backup;
(2) liquid submerged culture: the test tube slant strain obtained by step (1) is cut into 3 × 3 mm fritter strains, picking 4 pieces
Being inoculated in the 250mL triangular flask equipped with 20mL liquid submerged culture base, triangular flask is 170 revs/min at rotating speed, temperature 25 DEG C
Under the conditions of, 60h cultivated by shaking table, makes liquid shaking bottle strain;Described liquid submerged culture base is sterilizing 250 under the conditions of 110 DEG C
Min prepares, and containing wheat bran 16g, the raw material of rice 8g in every liter of liquid submerged culture base;
(3) seed tank amplification culture: the liquid shaking bottle strain obtained by step (2) is inoculated in seed tank amplification culture base,
And described liquid shaking bottle strain and the inoculum concentration inoculation that seed tank amplification culture base is 15% by volume, it is 25 DEG C in temperature, stirs
Mixing rotating speed is 120 revs/min, in the volume being passed through gas per minute and leading to that seed tank amplification culture base volume ratio is 1.6:1
Under the conditions of tolerance, cultivate 29h, make Tremella aurantialba Bandoni et Zang seed tank strain;Described seed tank amplification culture base is sterilizing under the conditions of 110 DEG C
250 min prepare, and containing wheat bran 14g, the raw material of rice 10g in every liter of liquid submerged culture base;
(4) solid primary fermentation is cultivated: access the Tremella aurantialba Bandoni et Zang seed tank strain obtained by step (3) equipped with solid primary fermentation culture medium
Culture bag in, and described Tremella aurantialba Bandoni et Zang seed tank strain and the culture bag equipped with solid primary fermentation culture medium be 6% connect by volume
Plant amount inoculation, at temperature 25 DEG C, humidity 80% primary fermentation 26 days, wherein every 5 days, turn over bag once, prepare solid primary fermentation thing;
Described solid primary fermentation culture medium is that sterilizing 250 min prepares under the conditions of 110 DEG C, and each kilogram of solid primary fermentation culture medium
In containing peeling Semen Ginkgo 276g, Folium Ginkgo extract 33g and the raw material of rice 691g;Former in described solid primary fermentation culture medium
Material is mixed with water in the ratio of 1:0.9;
(5) liquid post-fermentation and culture: the solid primary fermentation thing obtained by step (4) is crushed to 20 mesh, joins liquid fermentation
In tank culture medium, described liquid fermentation tank culture volume is 9 with the weight ratio of solid primary fermentation thing, is 25 DEG C in temperature, stirs
Mixing rotating speed is 110 revs/min, at the volume being passed through gas per minute with liquid fermentation tank culture volume than the ventilation for 1.4:1
Ferment under the conditions of amount 48h, and obtained fermented liquid centrifugal preparing under the conditions of 3500 revs/min contains sending out of ginkalide B
Ferment liquid and the mycelium containing Quercetin;Described liquid fermentation medium is that sterilizing 35 min prepares under the conditions of 110 DEG C, and often
Rise liquid fermentation medium and contain 34g glucose, 4g peptone and 0.03gK2HPO4;
(6) separation is extracted: by the tremella filament containing Quercetin obtained by step (5) and the fermentation containing ginkalide B
Liquid, respectively through extraction, obtains Quercetin and ginkalide B crystal.
It should be noted that and from the tremella filament containing Quercetin, produce Quercetin crystal described in step (6)
Method comprises the steps:
Obtained tremella filament is dried by A1, is then crushed to 20 mesh, the 70% of 16 times of volumes of addition mycelium weight
Ethanol, repeatedly extracts 5 times, obtains extracting solution one;
Extracting solution one obtained by step A1 is merged by A2, is then evaporated to the 1/30 of original volume, adds residual volume 5 times
Water, under the conditions of 4 DEG C crystallize 12 hours, then sucking filtration is dried, and i.e. obtains Quercetin crystal, and quercetin content is 98%.
In the present embodiment, from the fermentation liquid containing ginkalide B, ginkalide B crystal is produced described in step (6)
Method comprise the steps:
B1 is by the fermentation liquid concentrating under reduced pressure of obtained ginkalide B and is dried and to obtain product;
B2 adds 70% alcohol reflux 4 times of 10 times of weight in step B1 products therefrom, obtains extracting solution two;
Extracting solution two obtained by step B2 is merged by B3, is then evaporated to the 1/40 of original volume, ties under the conditions of-20 DEG C
Brilliant 8 hours;
Product after step B3 is crystallized by B4 carries out sucking filtration, and sucking filtration gained filtering residue ethyl acetate is redissolved, then by ethyl acetate
Decompression is concentrated to dryness mutually, then redissolves with dehydrated alcohol, and adds the water of 7 times of volumes, precipitation, sucking filtration, and gained filtering residue is dried and is
Ginkalide B, its content is 94%.
Embodiment 7
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin specifically includes following steps:
(1) test tube amplification culture: slant strains in Tremella aurantialba Bandoni et Zang test tube is cut into 3 × 3 mm fritter strains, inoculates a fritter to test tube
In slant medium, cultivating 13 days for 23 DEG C, prepare test tube slant strain, 4 DEG C, this test tube slant saves backup;
(2) liquid submerged culture: the test tube slant strain obtained by step (1) is cut into 3 × 3 mm fritter strains, picking 10 pieces
Being inoculated in the 250mL triangular flask equipped with 130mL liquid submerged culture base, triangular flask is 150 revs/min at rotating speed, temperature 23 DEG C
Under conditions of, 36h cultivated by shaking table, makes liquid shaking bottle strain;Described liquid submerged culture base is sterilizing under the conditions of 115 DEG C
260 min prepare, and containing wheat bran 9g, the raw material of rice 20g in every liter of liquid submerged culture base;
(3) seed tank amplification culture: the liquid shaking bottle strain obtained by step (2) is inoculated in seed tank amplification culture base,
And described liquid shaking bottle strain and the inoculum concentration inoculation that seed tank amplification culture base is 15% by volume, it is 21 DEG C in temperature, stirs
Mixing rotating speed is 120 revs/min, in the volume being passed through gas per minute and leading to that seed tank amplification culture base volume ratio is 0.3:1
Under the conditions of tolerance, cultivate 81h, make Tremella aurantialba Bandoni et Zang seed tank strain;Described seed tank amplification culture base is sterilizing under the conditions of 115 DEG C
260 min prepare, and containing wheat bran 19g, the raw material of rice 18g in every liter of liquid submerged culture base;
(4) solid primary fermentation is cultivated: access the Tremella aurantialba Bandoni et Zang seed tank strain obtained by step (3) equipped with solid primary fermentation culture medium
Culture bag in, and described Tremella aurantialba Bandoni et Zang seed tank strain and the culture bag equipped with solid primary fermentation culture medium be 4% connect by volume
Plant amount inoculation, at temperature 21 DEG C, humidity 80% primary fermentation 34 days, wherein every 6 days, turn over bag once, prepare solid primary fermentation thing;
Described solid primary fermentation culture medium is that sterilizing 250 min prepares under the conditions of 110 DEG C, and each kilogram of solid primary fermentation culture medium
In containing peeling Semen Ginkgo 370g, Folium Ginkgo extract 40g and the raw material of rice 590g;Former in described solid primary fermentation culture medium
Material is mixed with water in the ratio of 1:0.7;
(5) liquid post-fermentation and culture: the solid primary fermentation thing obtained by step (4) is crushed to 20 mesh, joins liquid fermentation
In tank culture medium, described liquid fermentation tank culture volume is 10 with the weight ratio of solid primary fermentation thing, is 21 DEG C in temperature, stirs
Mixing rotating speed is 60 revs/min, at the volume being passed through gas per minute with liquid fermentation tank culture volume than the ventilation for 1.4:1
Under the conditions of ferment 66h, obtained fermented liquid is centrifugal under the conditions of 5700 revs/min prepares the fermentation containing ginkalide B
Liquid and the mycelium containing Quercetin;Described liquid fermentation medium is that sterilizing 35 min prepares under the conditions of 110 DEG C, and every liter
Liquid fermentation medium contains 35g glucose, 5g peptone and 0.05gK2HPO4;
(6) separation is extracted: by the tremella filament containing Quercetin obtained by step (5) and the fermentation containing ginkalide B
Liquid, respectively through extraction, obtains Quercetin and ginkalide B crystal.
It should be noted that and from the tremella filament containing Quercetin, produce Quercetin crystal described in step (6)
Method comprises the steps:
Obtained tremella filament is dried by A1, is then crushed to 20 mesh, the 90% of 17 times of volumes of addition mycelium weight
Ethanol, repeatedly extracts 4 times, obtains extracting solution one;
Extracting solution one obtained by step A1 is merged by A2, is then evaporated to the 1/30 of original volume, adds residual volume 5 times
Water, under the conditions of 4 DEG C crystallize 18 hours, then sucking filtration is dried, and i.e. obtains Quercetin crystal, and quercetin content is 99.5%.
In the present embodiment, from the fermentation liquid containing ginkalide B, ginkalide B crystal is produced described in step (6)
Method comprise the steps:
B1 is by the fermentation liquid concentrating under reduced pressure of obtained ginkalide B and is dried and to obtain product;
B2 adds 65% alcohol reflux 5 times of 8 times of weight in step B1 products therefrom, obtains extracting solution two;
Extracting solution two obtained by step B2 is merged by B3, is then evaporated to the 1/40 of original volume, ties under the conditions of-20 DEG C
Brilliant 6 hours;
Product after step B3 is crystallized by B4 carries out sucking filtration, and sucking filtration gained filtering residue ethyl acetate is redissolved, then by ethyl acetate
Decompression is concentrated to dryness mutually, then redissolves with dehydrated alcohol, and adds the water of 5 times of volumes, precipitation, sucking filtration, and gained filtering residue is dried and is
Ginkalide B, its content is 99%.
Embodiment 8
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin specifically includes following steps:
(1) test tube amplification culture: slant strains in Tremella aurantialba Bandoni et Zang test tube is cut into 3 × 3 mm fritter strains, inoculates a fritter to test tube
In slant medium, cultivating 10 days for 29 DEG C, prepare test tube slant strain, 4 DEG C, this test tube slant saves backup;
(2) liquid submerged culture: the test tube slant strain obtained by step (1) is cut into 3 × 3 mm fritter strains, picking 8 pieces
Being inoculated in the 250mL triangular flask equipped with 60mL liquid submerged culture base, triangular flask is 160 revs/min at rotating speed, temperature 33 DEG C
Under the conditions of, 80h cultivated by shaking table, makes liquid shaking bottle strain;Described liquid submerged culture base is sterilizing 300 under the conditions of 120 DEG C
Min prepares, and containing wheat bran 19g, the raw material of rice 19g in every liter of liquid submerged culture base;
(3) seed tank amplification culture: the liquid shaking bottle strain obtained by step (2) is inoculated in seed tank amplification culture base,
And described liquid shaking bottle strain and the inoculum concentration inoculation that seed tank amplification culture base is 18% by volume, it is 33 DEG C in temperature, stirs
Mixing rotating speed is 140 revs/min, in the volume being passed through gas per minute and leading to that seed tank amplification culture base volume ratio is 1.6:1
Under the conditions of tolerance, cultivate 90h, make Tremella aurantialba Bandoni et Zang seed tank strain;Described seed tank amplification culture base is sterilizing under the conditions of 120 DEG C
300 min prepare, and containing wheat bran 18g, the raw material of rice 18g in every liter of liquid submerged culture base;
(4) solid primary fermentation is cultivated: access the Tremella aurantialba Bandoni et Zang seed tank strain obtained by step (3) equipped with solid primary fermentation culture medium
Culture bag in, and described Tremella aurantialba Bandoni et Zang seed tank strain and the culture bag equipped with solid primary fermentation culture medium be 9% connect by volume
Plant amount inoculation, at temperature 33 DEG C, humidity 80% primary fermentation 37 days, wherein every 6 days, turn over bag once, prepare solid primary fermentation thing;
Described solid primary fermentation culture medium is that sterilizing 350 min prepares under the conditions of 105 DEG C, and each kilogram of solid primary fermentation culture medium
In containing peeling Semen Ginkgo 400g, Folium Ginkgo extract 30g and the raw material of rice 570g;Former in described solid primary fermentation culture medium
Material is mixed with water in the ratio of 1:1.4;
(5) liquid post-fermentation and culture: the solid primary fermentation thing obtained by step (4) is crushed to 20 mesh, joins liquid fermentation
In tank culture medium, described liquid fermentation tank culture volume is 10 with the weight ratio of solid primary fermentation thing, is 33 DEG C in temperature, stirs
Mixing rotating speed is 150 revs/min, at the volume being passed through gas per minute with liquid fermentation tank culture volume than the ventilation for 1.6:1
Ferment under the conditions of amount 70h, and obtained fermented liquid centrifugal preparing under the conditions of 5800 revs/min contains sending out of ginkalide B
Ferment liquid and the mycelium containing Quercetin;Described liquid fermentation medium is that sterilizing 35 min prepares under the conditions of 105 DEG C, and often
Rise liquid fermentation medium and contain 38g glucose, 4g peptone and 0.09gK2HPO4;
(6) separation is extracted: by the tremella filament containing Quercetin obtained by step (5) and the fermentation containing ginkalide B
Liquid, respectively through extraction, obtains Quercetin and ginkalide B crystal.
It should be noted that and from the tremella filament containing Quercetin, produce Quercetin crystal described in step (6)
Method comprises the steps:
Obtained tremella filament is dried by A1, is then crushed to 20 mesh, the 100% of 19 times of volumes of addition mycelium weight
Ethanol, repeatedly extract 5 times, obtain extracting solution one;
Extracting solution one obtained by step A1 is merged by A2, is then evaporated to the 1/30 of original volume, adds residual volume 5 times
Water, under the conditions of 4 DEG C crystallize 16 hours, then sucking filtration is dried, and i.e. obtains Quercetin crystal, and quercetin content is 99%.
In the present embodiment, from the fermentation liquid containing ginkalide B, ginkalide B crystal is produced described in step (6)
Method comprise the steps:
B1 is by the fermentation liquid concentrating under reduced pressure of obtained ginkalide B and is dried and to obtain product;
B2 adds 98% alcohol reflux 5 times of 18 times of weight in step B1 products therefrom, obtains extracting solution two;
Extracting solution two obtained by step B2 is merged by B3, is then evaporated to the 1/40 of original volume, ties under the conditions of-20 DEG C
Brilliant 17 hours;
Product after step B3 is crystallized by B4 carries out sucking filtration, and sucking filtration gained filtering residue ethyl acetate is redissolved, then by ethyl acetate
Decompression is concentrated to dryness mutually, then redissolves with dehydrated alcohol, and adds the water of 10 times of volumes, precipitation, sucking filtration, and gained filtering residue is dried and is
Ginkalide B, its content is 98%.
Embodiment 9
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin specifically includes following steps:
(1) test tube amplification culture: slant strains in Tremella aurantialba Bandoni et Zang test tube is cut into 3 × 3 mm fritter strains, inoculates a fritter to test tube
In slant medium, cultivating 6 days for 24 DEG C, prepare test tube slant strain, 4 DEG C, this test tube slant saves backup;
(2) liquid submerged culture: the test tube slant strain obtained by step (1) is cut into 3 × 3 mm fritter strains, picking 4 pieces
Being inoculated in the 250mL triangular flask equipped with 24mL liquid submerged culture base, triangular flask is 58 revs/min at rotating speed, temperature 24 DEG C
Under the conditions of, 20h cultivated by shaking table, makes liquid shaking bottle strain;Described liquid submerged culture base is sterilizing 100 under the conditions of 100 DEG C
Min prepares, and containing wheat bran 5g, the raw material of rice 5g in every liter of liquid submerged culture base;
(3) seed tank amplification culture: the liquid shaking bottle strain obtained by step (2) is inoculated in seed tank amplification culture base,
And described liquid shaking bottle strain and the inoculum concentration inoculation that seed tank amplification culture base is 3% by volume, it is 24 DEG C in temperature, stirs
Mixing rotating speed is 58 revs/min, is the ventilation for 0.3:1 at the volume being passed through gas per minute and seed tank amplification culture base volume ratio
Under the conditions of amount, cultivate 25h, make Tremella aurantialba Bandoni et Zang seed tank strain;Described seed tank amplification culture base is sterilizing under the conditions of 100 DEG C
100 min prepare, and containing wheat bran 5g, the raw material of rice 6g in every liter of liquid submerged culture base;
(4) solid primary fermentation is cultivated: access the Tremella aurantialba Bandoni et Zang seed tank strain obtained by step (3) equipped with solid primary fermentation culture medium
Culture bag in, and described Tremella aurantialba Bandoni et Zang seed tank strain and the culture bag equipped with solid primary fermentation culture medium be 3% connect by volume
Plant amount inoculation, at temperature 24 DEG C, humidity 80% primary fermentation 23 days, wherein every 3 days, turn over bag once, prepare solid primary fermentation thing;
Described solid primary fermentation culture medium is that sterilizing 150 min prepares under the conditions of 100 DEG C, and each kilogram of solid primary fermentation culture medium
In containing peeling Semen Ginkgo 220g, Folium Ginkgo extract 33g and the raw material of rice 747g;Former in described solid primary fermentation culture medium
Material is mixed with water in the ratio of 1:0.8;
(5) liquid post-fermentation and culture: the solid primary fermentation thing obtained by step (4) is crushed to 20 mesh, joins liquid fermentation
In tank culture medium, described liquid fermentation tank culture volume is 6 with the weight ratio of solid primary fermentation thing, is 24 DEG C in temperature, stirs
Mixing rotating speed is 55 revs/min, at the volume being passed through gas per minute with liquid fermentation tank culture volume than the ventilation for 0.3:1
Under the conditions of ferment 26h, obtained fermented liquid is centrifugal under the conditions of 2300 revs/min prepares the fermentation containing ginkalide B
Liquid and the mycelium containing Quercetin;Described liquid fermentation medium is that sterilizing 35 min prepares under the conditions of 100 DEG C, and every liter
Liquid fermentation medium contains 6g glucose, 0.6g peptone and 0.02gK2HPO4;
(6) separation is extracted: by the tremella filament containing Quercetin obtained by step (5) and the fermentation containing ginkalide B
Liquid, respectively through extraction, obtains Quercetin and ginkalide B crystal.
It should be noted that and from the tremella filament containing Quercetin, produce Quercetin crystal described in step (6)
Method comprises the steps:
Obtained tremella filament is dried by A1, is then crushed to 20 mesh, the 67% of 6 times of volumes of addition mycelium weight
Ethanol, repeatedly extracts 4 times, obtains extracting solution one;
Extracting solution one obtained by step A1 is merged by A2, is then evaporated to the 1/30 of original volume, adds residual volume 5 times
Water, under the conditions of 4 DEG C crystallize 5 hours, then sucking filtration is dried, and i.e. obtains Quercetin crystal, and quercetin content is 95%.
In the present embodiment, from the fermentation liquid containing ginkalide B, ginkalide B crystal is produced described in step (6)
Method comprise the steps:
B1 is by the fermentation liquid concentrating under reduced pressure of obtained ginkalide B and is dried and to obtain product;
B2 adds 65% alcohol reflux 3 times of 6 times of weight in step B1 products therefrom, obtains extracting solution two;
Extracting solution two obtained by step B2 is merged by B3, is then evaporated to the 1/40 of original volume, ties under the conditions of-20 DEG C
Brilliant 4 hours;Product after step B3 is crystallized by B4 carries out sucking filtration, and sucking filtration gained filtering residue ethyl acetate is redissolved, then by acetic acid
Ethyl ester reduces pressure mutually and is concentrated to dryness, then redissolves with dehydrated alcohol, and adds the water of 4 times of volumes, precipitation, sucking filtration, and gained filtering residue is dried
Being ginkalide B, its content is 91%.
Schematically being described the present invention and embodiment thereof above, this description does not has restricted, actual knot
Structure is not limited thereto.So, if those of ordinary skill in the art is enlightened by it, without departing from the invention objective
In the case of, design the frame mode similar to this technical scheme and embodiment without creative, all should belong to the present invention's
Protection domain.
Claims (10)
1. one kind utilizes the method that Tremella aurantialba Bandoni et Zang prepares ginkalide B and Quercetin simultaneously, it is characterised in that described preparation method is with greatly
Rice, peeling Semen Ginkgo and Folium Ginkgo extract are primary raw material, with Tremella aurantialba Bandoni et Zang as starting strain, sequentially pass through test tube amplification culture, liquid
Body shake-flask culture and seed tank amplification culture, the cultivation of solid primary fermentation, liquid post-fermentation and culture and extraction separating step prepare and contain
There are the fermentation liquid of ginkalide B and the mycelium containing Quercetin;Described fermentation liquid containing ginkalide B and containing Quercetin
Mycelium prepare ginkalide B and Quercetin crystal respectively through extracting again, wherein ginkalide B purity reaches 90%, Cortex querci dentatae
Element purity reaches 95%.
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin the most according to claim 1, its feature exists
In, described preparation method comprises the steps:
A1 test tube amplification culture: cultivate in slant strains is inoculated in potato dextrose medium in Tremella aurantialba Bandoni et Zang, prepares gold
Ear test tube slant strain;
A2 liquid submerged culture: the Tremella aurantialba Bandoni et Zang test tube slant strain obtained by step A1 is inoculated into equipped with liquid submerged culture base
In shaking flask, cultivate, prepare golden fungus liquid shaking flask strain;
A3 seed tank amplification culture: the golden fungus liquid shaking flask strain obtained by step A2 is inoculated in seed tank culture base and carries out
Cultivate, make Tremella aurantialba Bandoni et Zang seed tank strain;
A4 solid primary fermentation is cultivated: is inoculated in solid medium by the Tremella aurantialba Bandoni et Zang seed tank strain obtained by step A3, and mixes
Uniformly, carry out fermentation culture, prepare Tremella aurantialba Bandoni et Zang solid fermentation thing;
A5 liquid post-fermentation and culture: the Tremella aurantialba Bandoni et Zang solid primary fermentation thing obtained by step A4 is transferred to liquid fermentation tank culture medium
In, carry out liquid after fermentation, prepare the fermentation liquid containing ginkalide B and the tremella filament containing Quercetin;
A6 extracts separation: by the tremella filament containing Quercetin obtained by step A5 and the fermentation liquid containing ginkalide B
Respectively through extraction, obtain Quercetin and ginkalide B crystal.
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin the most according to claim 2, its feature exists
In, described preparation method is specific as follows:
B1 test tube amplification culture: slant strains in Tremella aurantialba Bandoni et Zang test tube is cut into 3 × 3 mm fritter strains, inoculates a fritter oblique to test tube
In the culture medium of face, cultivating 4~15 days for 20~35 DEG C, prepare test tube slant strain, 4 DEG C, this test tube slant saves backup;
B2 liquid submerged culture: the test tube slant strain obtained by step B1 is cut into 3 × 3 mm fritter strains, picking 3~10
Block is inoculated in the 250mL triangular flask equipped with 20~150mL liquid submerged culture bases, triangular flask rotating speed be 50~200 turns/
Point, under conditions of temperature 20~35 DEG C, 18-86h cultivated by shaking table, makes liquid shaking bottle strain;
B3 seed tank amplification culture: the liquid shaking bottle strain obtained by step B2 is inoculated in seed tank amplification culture base, and
Described liquid shaking bottle strain and seed tank amplification culture base are the inoculum concentration inoculation of 1~20% by volume, are 20~35 in temperature
DEG C, speed of agitator is 50~160 revs/min, the volume being passed through gas per minute and seed tank amplification culture base volume ratio for for
Under the conditions of the ventilation of 0.2~1.8:1, cultivate 18~96h, make Tremella aurantialba Bandoni et Zang seed tank strain;
B4 solid primary fermentation is cultivated: access the Tremella aurantialba Bandoni et Zang seed tank strain obtained by step B3 equipped with solid primary fermentation culture medium
In culture bag, and described Tremella aurantialba Bandoni et Zang seed tank strain is 2~10% with the culture bag equipped with solid primary fermentation culture medium by volume
Inoculum concentration is inoculated, and in temperature 20~35 DEG C, humidity 80% primary fermentation 20~40 days, wherein every 3~6 days, turns over bag once, prepares
Solid primary fermentation thing;
B5 liquid post-fermentation and culture: the solid primary fermentation thing obtained by step B4 is crushed to 20 mesh, joins liquid fermentation tank
In culture medium, described liquid fermentation tank culture volume is 5~10 with the weight ratio of solid primary fermentation thing, is 20~43 in temperature
DEG C, speed of agitator is 50~160 revs/min, at the volume being passed through gas per minute with liquid fermentation tank culture volume ratio is
Fermentation 24~72h under the conditions of the ventilation of 0.2-1.8:1, obtained fermented liquid is under the conditions of 2000~6000 revs/min
The centrifugal fermentation liquid prepared containing ginkalide B and the mycelium containing Quercetin;
B6 extracts separation: by the tremella filament containing Quercetin obtained by step A5 and the fermentation liquid containing ginkalide B
Respectively through extraction, obtain Quercetin and ginkalide B crystal.
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin the most according to claim 3, its feature exists
In, liquid submerged culture base described in step B2 is that sterilizing 90~360 min prepares under the conditions of 100~130 DEG C, and every liter of liquid
Containing wheat bran 5~20g in body Shake flask medium, the raw material of rice 5~20g.
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin the most according to claim 3, its feature exists
In, the base of seed tank amplification culture described in step B3 is that sterilizing 90~360 min prepares under the conditions of 100~130 DEG C, and every liter
Containing wheat bran 5~20g in liquid submerged culture base, the raw material of rice 5~20g.
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin the most according to claim 3, its feature exists
In, the culture medium of solid primary fermentation described in step B4 is that sterilizing 90~360 min prepares under the conditions of 100~130 DEG C, and each
In kilogram solid primary fermentation culture medium containing peeling Semen Ginkgo 200~400g, Folium Ginkgo extract 30~50g and rice 750~
The raw material of 570g.
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin the most according to claim 6, its feature exists
In, the raw material in described solid primary fermentation culture medium is mixed with water in the ratio of 1:0.6~1.5.
A kind of method utilizing Tremella aurantialba Bandoni et Zang simultaneously to prepare ginkalide B and Quercetin the most according to claim 3, its feature exists
In, liquid fermentation medium described in step B5 is that sterilizing 30~60 min prepares under the conditions of 100~130 DEG C, and every liter of liquid
Body fermentation medium contains 5~40g glucoses, 0.5~4g peptone and 0.01~0.1gK2HPO4。
9., according to a kind of method utilizing Tremella aurantialba Bandoni et Zang to prepare ginkalide B and Quercetin described in Claims 2 or 3 simultaneously, it is special
Levying and be, the method producing Quercetin crystal described in step A6 or step B6 from the tremella filament containing Quercetin includes
Following steps:
Obtained tremella filament is dried by C1, is then crushed to 20 mesh, the 60 of 5~20 times of volumes of addition mycelium weight
~the ethanol of 100%, repeatedly extract 3~5 times, obtain extracting solution one;
Extracting solution one obtained by step C1 is merged by C2, is then evaporated to the 1/30 of original volume, adds residual volume 5 times
Water, under the conditions of 4 DEG C crystallize 3~18 hours, then sucking filtration is dried, and i.e. obtains Quercetin crystal, and Quercetin purity is more than
95%。
10., according to a kind of method utilizing Tremella aurantialba Bandoni et Zang to prepare ginkalide B and Quercetin described in Claims 2 or 3 simultaneously, it is special
Levy and be, the method producing ginkalide B crystal described in step A6 or step B6 from the fermentation liquid containing ginkalide B
Comprise the steps:
D1 is by the fermentation liquid concentrating under reduced pressure of obtained ginkalide B and is dried and to obtain product;
D2 adds 60~100% alcohol reflux 3~5 times of 5~20 times of weight in step D1 products therefrom, obtains extraction
Liquid two;
Extracting solution two obtained by step D2 is merged by D3, is then evaporated to the 1/40 of original volume, ties under the conditions of-20 DEG C
Brilliant 3~18 hours;
Product after step D3 is crystallized by D4 carries out sucking filtration, and sucking filtration gained filtering residue ethyl acetate is redissolved, then by ethyl acetate
Decompression is concentrated to dryness mutually, then redissolves with dehydrated alcohol, and adds the water of 3~10 times of volumes, precipitation, sucking filtration, and gained filtering residue is dried
Being ginkalide B, its purity is more than 90%.
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Citations (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN1602920A (en) * | 2004-08-03 | 2005-04-06 | 石雁羽 | Gingko leaf extracts with superior quality and its manufacturing technique |
| CN103882075A (en) * | 2014-01-28 | 2014-06-25 | 江苏河海科技工程集团有限公司 | Process for obtaining ginkgolide B by utilizing tremella aurantialba strains to transform ginkgo biloba extracts |
| CN104726276A (en) * | 2015-03-24 | 2015-06-24 | 淮南师范学院 | Method for brewing low-alcohol lily wine |
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2016
- 2016-06-07 CN CN201610393912.9A patent/CN105838752A/en active Pending
Patent Citations (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN1602920A (en) * | 2004-08-03 | 2005-04-06 | 石雁羽 | Gingko leaf extracts with superior quality and its manufacturing technique |
| CN103882075A (en) * | 2014-01-28 | 2014-06-25 | 江苏河海科技工程集团有限公司 | Process for obtaining ginkgolide B by utilizing tremella aurantialba strains to transform ginkgo biloba extracts |
| CN104726276A (en) * | 2015-03-24 | 2015-06-24 | 淮南师范学院 | Method for brewing low-alcohol lily wine |
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