阅读说明：本技术 一种获得两种夏天无多糖的提取方法、两种夏天无多糖及其应用 (Extraction method for obtaining two kinds of rhizoma corydalis Decumbentis polysaccharides, the two kinds of rhizoma corydalis Decumbentis polysaccharides and application thereof ) 是由 王昭晶 于 2021-08-17 设计创作，主要内容包括：本发明属于医药技术领域,特别是涉及一种获得两种夏天无多糖的提取方法、两种夏天无多糖及其应用。本发明提供了一种获得两种夏天无多糖的提取方法,所述提取方法包括粗提、醇沉、酶解和柱层析,经过上述提取方法能够分别获得夏天无多糖CPS1和夏天无多糖CPW2。本发明提供的提取方法通过一套方法准确地获得两种产物,能够有效提高夏天无多糖的提取效率。本发明提供的两种夏天无多糖具有显著的抗炎效果。夏天无多糖CPS1能显著降低LPS诱导的RAW264.7细胞中的TNF-α,IL-1β,IL-6和COX-2四种炎症因子的mRNA相对表达量；夏天无多糖CPW2则能显著降低TNF-α,COX-2和iNOS基因的表达量。(The invention belongs to the technical field of medicines, and particularly relates to an extraction method for obtaining two rhizoma corydalis Decumbentis polysaccharides, the two rhizoma corydalis Decumbentis polysaccharides and application thereof. The invention provides an extraction method for obtaining two rhizoma corydalis Decumbentis polysaccharides, which comprises crude extraction, alcohol precipitation, enzymolysis and column chromatography, wherein the rhizoma corydalis Decumbentis polysaccharide CPS1 and rhizoma corydalis Decumbentis polysaccharide CPW2 can be obtained by the extraction method. The extraction method provided by the invention can accurately obtain two products by a set of method, and can effectively improve the extraction efficiency of the corydalis amabilis polysaccharide. The two corydalis amabilis polysaccharides provided by the invention have a remarkable anti-inflammatory effect. Corydalis amabilis polysaccharide CPS1 can remarkably reduce the relative expression quantity of mRNA of TNF-alpha, IL-1 beta, IL-6 and COX-2 inflammatory factors in RAW264.7 cells induced by LPS; decumbent corydalis tuber polysaccharide CPW2 can obviously reduce the expression of TNF-alpha, COX-2 and iNOS genes.)

1. An extraction method for obtaining two polysaccharides of corydalis amabilis comprises the following steps:

mixing rhizoma corydalis Decumbentis with water, extracting with water to obtain water extractive solution, and concentrating the water extractive solution to obtain concentrated solution;

concentrating the concentrated solution to 1/25-1/35 of the volume of the water extract;

mixing absolute ethyl alcohol with the concentrated solution, centrifuging, and taking a precipitate to obtain a first crude extract; the volume ratio of the absolute ethyl alcohol to the concentrated solution is 2: 1;

mixing absolute ethyl alcohol with the centrifuged supernatant, centrifuging, and taking precipitate to obtain a second crude extract; the volume ratio of the absolute ethyl alcohol to the centrifuged supernatant is (0.7-1) to 1;

mixing trypsin and the first crude extract, carrying out enzymolysis to obtain an enzymolysis solution, carrying out first elution on the enzymolysis solution by using a chromatographic column filled with DEAE-Sepharose CL-6B gel to obtain a first eluent, and purifying the first eluent to obtain decumbent corydalis polysaccharide CPS 1;

the first elution comprises the steps of: eluting by using distilled water, not collecting eluent, and after the elution of the distilled water is finished, performing linear gradient elution by using 0.25-0.45 mol/L NaCl aqueous solution to obtain first eluent;

performing second elution on the second crude extract by using a chromatographic column filled with DEAE-Sepharose CL-6B gel to obtain a second eluent, and purifying the second eluent to obtain decumbent corydalis polysaccharide CPW 2;

the second elution comprises the steps of: eluting with distilled water to obtain a second eluate.

2. The extraction method according to claim 1, wherein the mass ratio of corydalis amabilis to water in the water extraction is 1 (10-100).

3. The extraction method according to claim 1, wherein the flow rates at the first elution and the second elution are respectively 0.8 mL/min.

4. The extraction method of claim 1, wherein the mass ratio of the trypsin to the proteins in the first crude extract is 1 (15-20).

5. The extraction method according to claim 1, wherein the temperature of enzymolysis is 37 ℃ and the time of enzymolysis is 20 h.

6. Rhizoma corydalis Decumbentis polysaccharide CPS1 extracted according to any one of claims 1-5, wherein rhizoma corydalis Decumbentis polysaccharide CPS1 is a homogeneous heteropolysaccharide with molecular weight of 360kDa, and is composed of glucose, galactose, mannose and arabinose;

the molar ratio of the glucose, the galactose, the mannose and the arabinose is 4.9:2.0:1: 1.9.

7. Corydalis amabilis polysaccharide CPW2 extracted by the extraction method of any one of claims 1-5, wherein corydalis amabilis polysaccharide CPW2 is formed by polymerization of homopolysaccharide, and monosaccharide of the homopolysaccharide is glucose;

the homopolysaccharide has molecular weight of 550KDa and 55 KDa; the molar ratio of the homopolysaccharide with the molecular weight of 550KDa to the homopolysaccharide with the molecular weight of 55KDa is 1: 4.

8. Use of two polysaccharides extracted from rhizoma corydalis Decumbentis according to the extraction method of claims 1-5, or the polysaccharide CPS1 of rhizoma corydalis Decumbentis provided by claim 6, or the polysaccharide CPW2 of rhizoma corydalis Decumbentis provided by claim 7 in preparing antiinflammatory agent and/or medicament.

9. Use of two polysaccharides extracted from rhizoma corydalis Decumbentis according to the extraction method of claims 1-5, or the polysaccharide CPS1 of rhizoma corydalis Decumbentis provided by claim 6, or the polysaccharide CPW2 of rhizoma corydalis Decumbentis according to claim 7 in preparation of preparation and/or medicament for inhibiting inflammatory factor expression; the inflammatory factors include TNF-alpha, IL-1 beta, IL-6 and COX-2.

Technical Field

The invention belongs to the technical field of medicines, and particularly relates to an extraction method for obtaining two rhizoma corydalis Decumbentis polysaccharides, the two rhizoma corydalis Decumbentis polysaccharides and application thereof.

Background

Rhizoma Corydalis Decumbentis is dried tuber of Corydalis decumbens (Corydalis decumbens) belonging to Papaveraceae. It is bitter and slightly pungent in property, and is commonly used for treating headache, apoplexy, hemiplegia, lumbago and skelalgia. Modern pharmacological studies show that rhizoma corydalis Decumbentis has antiinflammatory, cerebral infarction resisting, arrhythmia resisting, and cranial nerve protecting effects. At present, researches on active ingredients of the corydalis amabilis mainly focus on alkaloid substances such as protopine, tetrahydropalmatine and palmatine, and at the present stage, the polysaccharides contained in the corydalis amabilis are rarely researched, and the polysaccharides contained in the corydalis amabilis are difficult to extract efficiently and are deeply researched.

Disclosure of Invention

In order to solve the problems, the invention provides an extraction method for obtaining two types of rhizoma corydalis Decumbentis polysaccharides, the two types of rhizoma corydalis Decumbentis polysaccharides and application thereof. The extraction method provided by the invention can be used for efficiently extracting two different decumbent corydalis tuber polysaccharides (decumbent corydalis tuber polysaccharide CPS1 and decumbent corydalis tuber polysaccharide CPW2) by using a set of extraction method. The two rhizoma corydalis Decumbentis polysaccharides have significant antiinflammatory effect.

In order to achieve the purpose, the invention provides the following technical scheme:

the invention provides an extraction method for obtaining two polysaccharides of corydalis amabilis, which comprises the following steps:

mixing rhizoma corydalis Decumbentis with water, extracting with water to obtain water extractive solution, and concentrating the water extractive solution to obtain concentrated solution;

concentrating the concentrated solution to 1/25-1/35 of the volume of the water extract;

mixing absolute ethyl alcohol with the concentrated solution, centrifuging, and taking a precipitate to obtain a first crude extract; the volume ratio of the absolute ethyl alcohol to the concentrated solution is 2: 1;

mixing absolute ethyl alcohol with the centrifuged supernatant, centrifuging, and taking precipitate to obtain a second crude extract; the volume ratio of the absolute ethyl alcohol to the centrifuged supernatant is (0.7-1) to 1;

mixing trypsin and the first crude extract, carrying out enzymolysis to obtain an enzymolysis solution, carrying out first elution on the enzymolysis solution by using a chromatographic column filled with DEAE-Sepharose CL-6B gel to obtain a first eluent, and purifying the first eluent to obtain decumbent corydalis polysaccharide CPS 1;

the first elution comprises the steps of: eluting by using distilled water, not collecting eluent, and after the elution of the distilled water is finished, performing linear gradient elution by using 0.25-0.45 mol/L NaCl aqueous solution to obtain first eluent;

performing second elution on the second crude extract by using a chromatographic column filled with DEAE-Sepharose CL-6B gel to obtain a second eluent, and purifying the second eluent to obtain decumbent corydalis polysaccharide CPW 2;

the second elution comprises the steps of: eluting with distilled water to obtain a second eluate.

Preferably, the mass ratio of the corydalis amabilis to the water in the water extraction is 1 (10-100).

Preferably, the flow rates of the first elution and the second elution are respectively 0.8 mL/min.

Preferably, the mass ratio of the trypsin to the proteins in the first crude extract is 1 (15-20).

Preferably, the temperature of the enzymolysis is 37 ℃, and the time of the enzymolysis is 20 h.

The invention also provides a decumbent corydalis polysaccharide CPS1 extracted according to the extraction method, wherein the decumbent corydalis polysaccharide CPS1 is a uniform heteropolysaccharide with the molecular weight of 360kDa and consists of glucose, galactose, mannose and arabinose;

the molar ratio of the glucose, the galactose, the mannose and the arabinose is 4.9:2.0:1: 1.9.

The invention also provides decumbent corydalis polysaccharide CPW2 extracted by the extraction method, wherein the decumbent corydalis polysaccharide CPW2 is formed by polymerization of homopolysaccharide, and monosaccharide of the homopolysaccharide is glucose;

the homopolysaccharide has molecular weight of 550KDa and 55 KDa; the molar ratio of the homopolysaccharide with the molecular weight of 550KDa to the homopolysaccharide with the molecular weight of 55KDa is 1: 4.

The invention also provides application of the two corydalis amabilis polysaccharides extracted by the extraction method or the corydalis amabilis polysaccharide CPS1 or the corydalis amabilis polysaccharide CPW2 in preparation of anti-inflammatory preparations and/or medicaments.

The invention also provides the application of the two corydalis amabilis polysaccharides extracted by the extraction method or the corydalis amabilis polysaccharide CPS1 or the corydalis amabilis polysaccharide CPW2 in preparing preparations and/or medicaments for inhibiting the expression of inflammatory factors; the inflammatory factors include TNF-alpha, IL-1 beta, IL-6 and COX-2.

The invention provides an extraction method for obtaining two rhizoma corydalis Decumbentis polysaccharides, which comprises crude extraction, alcohol precipitation, enzymolysis and column chromatography, wherein the rhizoma corydalis Decumbentis polysaccharide CPS1 and rhizoma corydalis Decumbentis polysaccharide CPW2 can be obtained by the extraction method. The extraction method provided by the invention can accurately obtain two products by a set of method, and can effectively improve the extraction efficiency of the corydalis amabilis polysaccharide.

The two corydalis amabilis polysaccharides provided by the invention have a remarkable anti-inflammatory effect. The embodiment shows that the polysaccharide CPS1 of corydalis amabilis provided by the invention can obviously reduce the relative expression quantity of mRNA of four inflammatory factors of TNF-alpha, IL-1 beta, IL-6 and COX-2 in RAW264.7 cells induced by LPS; decumbent corydalis tuber polysaccharide CPW2 can remarkably reduce the expression level of TNF-alpha, COX-2 and iNOS genes (P < 0.05).

Drawings

FIG. 1 is a graph of the extraction rate of total sugar in decumbent corydalis tuber versus liquid-to-feed ratio in example 1;

FIG. 2 is a graph of the extraction rate of total sugar in decumbent corydalis tuber versus the extraction time in example 1;

FIG. 3 is the curve of the extraction rate of total sugar of corydalis amabilis as a function of the extraction temperature in example 1;

FIG. 4 is a residual normal probability distribution diagram of example 1;

FIG. 5 is a model diagnostic graph-residual graph of example 1;

FIG. 6 is a model diagnostic plot-predicted value versus actual value scatter plot of example 1;

FIG. 7 is a sugar content distribution curve of the first crude extract after enzymolysis in example 2, after DEAE-Sepharose CL-6B and linear gradient elution with NaCl aqueous solution of 0.25mol/L to 0.45 mol/L;

FIG. 8 is a graph showing the distribution of sugar content after the second crude extract is eluted with distilled water using DEAE-Sepharose CL-6B in example 2;

FIG. 9 is a high performance size exclusion chromatogram of decumbent corydalis tuber polysaccharide CPS1 in application example 1;

FIG. 10 is a full wavelength scanning chart of decumbent corydalis tuber polysaccharide CPS1 in application example 1;

FIG. 11 is a high performance size exclusion chromatogram of decumbent corydalis tuber polysaccharide CPS1-P in application example 1;

FIG. 12 is a high performance size exclusion chromatogram of polysaccharide CPS1-E of decumbent corydalis tuber without enzymolysis in application example 1;

FIG. 13 is a full wavelength scanning chart of polysaccharide CPS1-E of decumbent corydalis tuber without enzymolysis in application example 1;

FIG. 14 is a high performance size exclusion chromatogram of decumbent corydalis amabilis polysaccharide CPW2 of application example 1;

FIG. 15 is a full wavelength scan of decumbent corydalis tuber polysaccharide CPW2 in application example 1;

FIG. 16 is a high performance size exclusion chromatogram of a first crude polysaccharide purified sample of CPW of application example 1;

FIG. 17 is a gas chromatogram of decumbent corydalis tuber polysaccharide CPS1 in application example 2;

FIG. 18 is a gas chromatogram of decumbent corydalis tuber polysaccharide CPW2 in application example 2;

FIG. 19 is a graph showing the effect of polysaccharide CPS1 of corydalis amabilis on LPS stimulation of mRNA expression of macrophage inflammatory factor in RAW264.7 mice in application example 3;

FIG. 20 is a graph showing the effect of corydalis amabilis CPW2 on LPS stimulation of mRNA expression of macrophage inflammatory factor in RAW264.7 mice in application example 3.

Detailed Description

The invention provides an extraction method for obtaining two polysaccharides of corydalis amabilis, which comprises the following steps:

mixing rhizoma corydalis Decumbentis with water, extracting with water to obtain water extractive solution, and concentrating the water extractive solution to obtain concentrated solution;

concentrating the concentrated solution to 1/25-1/35 of the volume of the water extract;

mixing absolute ethyl alcohol with the concentrated solution, centrifuging, and taking a precipitate to obtain a first crude extract; the volume ratio of the absolute ethyl alcohol to the concentrated solution is 2: 1;

mixing absolute ethyl alcohol with the centrifuged supernatant, centrifuging, and taking precipitate to obtain a second crude extract; the volume ratio of the absolute ethyl alcohol to the centrifuged supernatant is (0.7-1) to 1;

mixing trypsin and the first crude extract, carrying out enzymolysis to obtain an enzymolysis solution, carrying out first elution on the enzymolysis solution by using a chromatographic column filled with DEAE-Sepharose CL-6B gel to obtain a first eluent, and purifying the first eluent to obtain decumbent corydalis polysaccharide CPS 1;

the first elution comprises the steps of: eluting by using distilled water, not collecting eluent, and after the elution of the distilled water is finished, performing linear gradient elution by using 0.25-0.45 mol/L NaCl aqueous solution to obtain first eluent;

performing second elution on the second crude extract by using a chromatographic column filled with DEAE-Sepharose CL-6B gel to obtain a second eluent, and purifying the second eluent to obtain decumbent corydalis polysaccharide CPW 2;

the second elution comprises the steps of: eluting with distilled water to obtain a second eluate.

The extraction method provided by the invention has the advantages of low energy consumption and extremely high extraction rate, meanwhile, ethanol is adopted for fractional precipitation, the extracted corydalis amabilis polysaccharide has definite components, the sugar content of the two corydalis amabilis polysaccharides exceeds 97%, and the polysaccharide does not contain impurities such as protein, nucleic acid and the like, and the two corydalis amabilis polysaccharides can be simultaneously prepared by one method, so that the method is simple, effective, convenient and easy to operate.

The invention mixes decumbent corydalis tuber with water to carry out water extraction to obtain water extract, and concentrates the water extract to obtain concentrated solution. In the invention, the mass ratio of the corydalis amabilis to water in the water extraction is preferably 1 (10-100), and in the invention, the corydalis amabilis preferably comprises fresh or dry corydalis amabilis, and more preferably dry corydalis amabilis. When the corydalis amabilis is dry corydalis amabilis, the mass ratio of the dry corydalis amabilis to water is preferably 1: 60. In the invention, the water extraction method preferably comprises a constant-temperature water bath, the temperature of the constant-temperature water bath is preferably 50-80 ℃, the further preferable temperature is 68 ℃, and the time of the constant-temperature water bath is preferably 150-330 min, and the further preferable time is 250 min.

After the water extraction is finished, the centrifugal treatment is preferably carried out, the rotation speed of the centrifugation is preferably 3500-5000 r/min, more preferably 3500r/min, and the time of the centrifugation is preferably 5-10 min, more preferably 5 min.

After the centrifugation is finished, the invention carries out concentration, and the concentrated solution is concentrated to 1/25-1/35, more preferably 1/30 of the volume of water. The method can obtain the total sugar of the corydalis amabilis by the extraction method, can extract the total sugar of the corydalis amabilis to the maximum extent, and effectively saves energy.

After the concentrated solution is obtained, the invention mixes absolute ethyl alcohol with the concentrated solution, centrifuges the mixture, and obtains a first crude extract by taking the sediment. In the invention, the volume ratio of the absolute ethyl alcohol to the concentrated solution is 2: 1.

In the present invention, when the concentrated solution is mixed with absolute ethanol, it is preferable to slowly add absolute ethanol to the concentrated solution while stirring. According to the invention, after the absolute ethyl alcohol and the concentrated solution are mixed, the preferable step of standing is also included, the preferable temperature of standing is 2-5 ℃, the further preferable temperature is 4 ℃, and the preferable time of standing is 10-24 h, the further preferable time is 15 h. In the invention, the rotation speed of the centrifugation is preferably 3500-5000 r/min, more preferably 5000r/min, and the time of the centrifugation is preferably 5-10 min, more preferably 5 min.

And taking the supernatant obtained by centrifugation, mixing the supernatant with absolute ethyl alcohol, centrifuging, and taking the precipitate to obtain a second crude extract. In the present invention, when the supernatant is mixed with absolute ethanol, it is preferable to slowly add absolute ethanol to the concentrated solution while stirring. In the present invention, the volume ratio of the absolute ethanol to the centrifuged supernatant is preferably (0.7 to 1: 1), and more preferably 0.7: 1. In the present invention, after the supernatant is mixed with the absolute ethanol, the operation of standing is preferably further included. In the present invention, the conditions for the standing and centrifugation are preferably the same as those described above, and will not be described herein. In the present invention, after the centrifugation, an operation of drying the precipitate obtained by the centrifugation is preferably performed, and the drying preferably includes freeze-drying. In the separation process of the first crude extract and the second crude extract, ethanol is used for fractional precipitation, and an intermediate product containing a target substance can be accurately obtained.

After the first crude extract is obtained, mixing trypsin and the first crude extract for enzymolysis to obtain an enzymolysis solution, performing first elution on the enzymolysis solution by using a chromatographic column filled with DEAE-Sepharose CL-6B gel to obtain a first eluent, and purifying the first eluent to obtain decumbent corydalis polysaccharide CPS 1.

The first crude extract is preferably mixed with water for dissolution to obtain an aqueous solution of the first crude extract. The mass-volume ratio of the first crude extract to water is preferably (150-300) mg (10-20) mL, more preferably 300mg:10mL, and the dissolving temperature is preferably 40-60 ℃, more preferably 50 ℃.

After obtaining the aqueous solution of the first crude extract, the present invention preferably detects the protein content in the aqueous solution of the first crude extract.

And (3) after the protein content in the aqueous solution of the first crude extract is obtained, carrying out enzymolysis to obtain an enzymolysis liquid. In the present invention, the enzyme preferably comprises trypsin; in the invention, the mass ratio of the trypsin to the protein is preferably 1 (15-20), and more preferably 1:20, based on the protein content in the aqueous solution of the first crude extract. In the invention, the enzymolysis temperature is 37 ℃, the time is preferably 20-24 h, and the time is more preferably 20 h.

After obtaining the enzymolysis solution, the invention uses a chromatographic column filled with DEAE-Sepharose CL-6B gel to carry out first elution on the enzymolysis solution to obtain a first eluent. In the present invention, the first elution includes the steps of: eluting with distilled water, not collecting the eluent, and after the elution of the distilled water is finished, performing linear gradient elution with 0.25-0.45 mol/L NaCl aqueous solution to obtain a first eluent.

In the present invention, the time for eluting with distilled water is preferably 21 to 24 hours, and more preferably 21 hours.

After the first eluent is obtained, the invention purifies the first eluent to obtain decumbent corydalis polysaccharide CPS 1. In the present invention, the purification preferably comprises dialysis; the method of dialysis preferably comprises dialysis using a dialysis bag with a molecular weight cut-off of 5000;

in the dialysis, preferably, running water dialysis is used and then distilled water dialysis is used, wherein the running water dialysis time is preferably 18-24 h, more preferably 18h, and the distilled water dialysis time is preferably 18-24 h, more preferably 18 h. The extraction method provided by the invention can accurately extract and obtain decumbent corydalis polysaccharide CPS1 with high purity through enzymolysis and specific linear gradient elution of sodium chloride aqueous solution.

After the second crude extract is obtained, the second crude extract is subjected to second elution by using a chromatographic column filled with DEAE-Sepharose CL-6B gel to obtain a second eluent, and the second eluent is purified to obtain corydalis amabilis polysaccharide CPW 2.

Before the second elution, the second crude extract is preferably mixed and dissolved with water to obtain an aqueous solution of the second crude extract. In the invention, the mass-to-volume ratio of the second crude extract to water is preferably (150-300) mg (10-20) mL, and more preferably 300mg to 10 mL.

After obtaining the aqueous solution of the second crude extract, the present invention preferably centrifuges the aqueous solution of the second crude extract to obtain a supernatant of the aqueous solution of the second crude extract. In the invention, the rotation speed of the centrifugation is preferably 3500-5000 r/min, more preferably 5000r/min, and the time of the centrifugation is preferably 5-10 min, more preferably 5 min.

After obtaining the supernatant of the aqueous solution of the second crude extract, the invention uses a chromatographic column filled with DEAE-Sepharose CL-6B gel to carry out second elution on the second crude extract to obtain a second eluent.

In the present invention, the second elution includes the steps of: eluting with distilled water to obtain a second eluate.

In the present invention, the time for eluting with distilled water is preferably 6 hours or more, and more preferably 12 hours.

In the invention, after the second eluent is obtained, the second eluent is purified by the invention to obtain decumbent corydalis polysaccharide CPW 2. The purification preferably comprises dialysis, the method of dialysis preferably comprising dialysis using a dialysis bag with a molecular weight cut-off of 5000;

in the dialysis, preferably, running water dialysis is used and then distilled water dialysis is used, wherein the running water dialysis time is preferably 18-24 h, more preferably 18h, and the distilled water dialysis time is preferably 18-24 h, more preferably 18 h. The extraction method provided by the invention separates the decumbent corydalis polysaccharide CPS1 again after the extraction method is adopted, and can accurately extract and obtain the decumbent corydalis polysaccharide CPW2 with high purity.

In the present invention, the source of the above-mentioned materials is not particularly limited unless otherwise specified, and conventional commercially available products known to those skilled in the art may be used.

The invention also provides a decumbent corydalis polysaccharide CPS1 extracted according to the extraction method, wherein the decumbent corydalis polysaccharide CPS1 is a uniform heteropolysaccharide with the molecular weight of 360kDa and consists of glucose, galactose, mannose and arabinose; the molar ratio of the glucose, the galactose, the mannose and the arabinose is 4.9:2.0:1: 1.9. The polysaccharide CPS1 of corydalis amabilis provided by the invention can obviously reduce the mRNA relative expression quantity of four inflammatory factors of TNF-alpha, IL-1 beta, IL-6 and COX-2 in RAW264.7 cells induced by LPS.

The invention also provides decumbent corydalis polysaccharide CPW2 extracted by the extraction method, wherein the decumbent corydalis polysaccharide CPW2 is formed by polymerization of homopolysaccharide, and monosaccharide of the homopolysaccharide is glucose;

the homopolysaccharide has molecular weight of 550KDa and 55 KDa; the molar ratio of the homopolysaccharide with the molecular weight of 550KDa to the homopolysaccharide with the molecular weight of 55KDa is 1: 4. The decumbent corydalis tuber polysaccharide CPW2 provided by the invention can obviously reduce the expression quantity of TNF-alpha, COX-2 and iNOS genes.

The invention also provides application of the two corydalis amabilis polysaccharides extracted by the extraction method or the corydalis amabilis polysaccharide CPS1 or the corydalis amabilis polysaccharide CPW2 in preparation of anti-inflammatory preparations and/or medicaments. The two corydalis amabilis polysaccharides provided by the invention have a remarkable effect of inhibiting inflammatory factors, the overexpression of the inflammatory factors is related to cerebral hemorrhage diseases, IL-1 beta can be expressed in a large amount in the acute phase of cerebral hemorrhage, after the cerebral hemorrhage diseases are ill, the concentration of TNF-alpha is in positive correlation with the amount of hemorrhage, the overexpression of IL-6 can aggravate blood brain barrier injury, and the overexpression of iNOS can release a large amount of nitric oxide, so that the injury of neuron cells is aggravated.

The invention also provides the application of the two corydalis amabilis polysaccharides extracted by the extraction method or the corydalis amabilis polysaccharide CPS1 or the corydalis amabilis polysaccharide CPW2 in preparing preparations and/or medicaments for inhibiting the relative expression of inflammatory factors; the inflammatory factors include TNF-alpha, IL-1 beta, IL-6 and COX-2. The decumbent corydalis tuber polysaccharide CPS1 provided by the invention can obviously reduce the mRNA relative expression quantity (P <0.05) of four inflammatory factors of TNF-alpha, IL-1 beta, IL-6 and COX-2 in RAW264.7 cells induced by LPS, and the specific embodiment proves that the decumbent corydalis tuber polysaccharide CPS1 with the mass concentration of 75 mu g/mL or 150 mu g/mL can obviously reduce the mRNA relative expression quantity of the four inflammatory factors of TNF-alpha, IL-1 beta, IL-6 and COX-2 in RAW264.7 cells induced by LPS; the decumbent corydalis tuber polysaccharide CPW2 can obviously reduce the expression quantity (P <0.05) of TNF-alpha, COX-2 and iNOS genes, and the specific examples prove that the decumbent corydalis tuber polysaccharide CPW2 with the mass concentration of 75 mu g/mL or 150 mu g/mL can obviously reduce the expression quantity of the TNF-alpha, COX-2 and iNOS genes.

For further illustration of the present invention, the following detailed description of the extraction method for obtaining two rhizoma corydalis Decumbentis polysaccharides, two rhizoma corydalis Decumbentis polysaccharides and their application provided by the present invention will be made with reference to the drawings and examples, which should not be construed as limiting the scope of the present invention.

Example 1

Response surface method for optimizing extraction process of total sugar of decumbent corydalis tuber

The experimental method comprises the following steps: a single-factor experiment is designed, and the influence of the feed-liquid ratio, the extraction time and the extraction temperature on the total sugar extraction rate of the corydalis amabilis is researched. The specific experimental scheme is that under the experimental conditions of two fixed factors, the experimental conditions of the other 1 factor are changed, so that the influence of the factor on the total sugar extraction rate of the corydalis amabilis under different experimental levels can be obtained.

A Box-Behnken model is adopted to arrange experiments, and the liquid-material ratio, the extraction temperature and the extraction time are taken as main experimental factors. Weighing 1g of crushed dried corydalis amabilis, adding corresponding distilled water according to the experimental design shown in Table 1, extracting at a specific extraction temperature for a specific time to obtain a crude extract, and detecting the total sugar extraction rate of the obtained crude extract by adopting a phenol-sulfuric acid method.

TABLE 1 Box-Behnken design scheme and extraction rate for total sugar extraction of corydalis amabilis

As a result: the single-factor experiment results are shown in figures 1-3, and the experiment level of the response surface experiment is arranged by taking 3 factors of liquid-material ratio, extraction time and extraction temperature as independent variables according to the single-factor experiment results shown in figures 1-3 (see table 2).

The decumbent corydalis tuber polysaccharide extraction process is optimized at the level of three factors by adopting a response surface analysis method so as to achieve the purpose of maximally extracting decumbent corydalis tuber polysaccharide (as shown in table 1). Performing quadratic polynomial fitting regression analysis on the data in table 1 by using Design-expert.V11.1.0 software to obtain a quadratic polynomial regression equation of the extraction rate of the decumbent corydalis tuber polysaccharide to extraction factors, wherein the quadratic polynomial regression equation comprises the following steps:

Y＝-166.55168+0.122058A+0.531025B+3.78316C+0.000450AB-0.000288AC-0.000475BC-0.001738A²-0.001046B²-0.026881C²。

TABLE 2 response surface test design factor levels and encodings

In order to verify the prediction effect of the model on the extraction scheme, the influence degree of each factor on the extraction rate of the polysaccharide of corydalis amabilis is further determined, the variance analysis is carried out on the test result, and the significance test result of the model coefficient is shown in table 3.

TABLE 3 regression equation analysis of variance and significance results

As can be seen from Table 3, the P value of this model is 0.0083: (<0.05), which indicates that the test model has significance; the mismatching term P of the model is 0.0889: (>0.05), which shows that the simulation-missing item test of the model is not obvious, the model selection is proper and the relative error of the test is small. From the influence degree of each parameter in the regression equation on the extraction rate of total sugar in rhizoma corydalis Decumbentis, secondary term (B) of extraction time and extraction temperature²、C²) Has very obvious influence on the extraction rate of polysaccharide of corydalis amabilis (P)<0.01)。

R of the equation²0.9021, the equation has good fitting degree, and can be used for preliminary analysis and prediction of process research of the extraction rate of the total sugar of the corydalis amabilis. Normal graph of residuals as shown in fig. 4, the distribution of residuals along a straight line indicates that residuals follow a normal distribution. As shown in fig. 5, all data points are within the acceptable range (± 4.82), and the results of the diagnostic map demonstrate the applicability and accuracy of the model.

Combining the mathematical analysis of the regression model to obtain the optimal process conditions of the rhizoma corydalis Decumbentis total sugar as follows: a (liquid-to-material ratio) 60: 1, 250min for B and 68 ℃ for C, and the average extraction rate of the total sugar of the corydalis amabilis is 32.740% which is 0.364% different from the theoretical value. The extraction conditions of the total sugar of the corydalis amabilis provided by the invention can be used for extracting the total sugar of the corydalis amabilis to the maximum extent.

Example 2

Simultaneously preparing two polysaccharides of corydalis amabilis

(1) Putting 50g of dried rhizoma corydalis Decumbentis root into 3000mL of distilled water, extracting in water bath at 68 deg.C for 250min, centrifuging at 3500r/min for 5min, and collecting extractive solution;

(2) concentrating the extracting solution obtained in the step (1) to 100mL, stirring while concentrating, slowly adding 200mL of absolute ethyl alcohol into the concentrated solution while stirring, covering a preservative film, and refrigerating and standing in a refrigerator at the temperature of 4 ℃ for 15 hours;

centrifuging after the cold storage and standing are finished, wherein the centrifuging condition is 5000r/min, the centrifuging time is 5min, and centrifuging to obtain a first precipitate and a supernatant;

drying the first precipitate to obtain a first crude extract, pouring the supernatant into a new beaker, slowly adding 200mL of absolute ethanol while stirring, standing in a refrigerator at 4 ℃ for 15h, centrifuging after the cold storage and standing are finished, centrifuging at 5000r/min for 5min, and centrifuging to obtain a second precipitate;

adding a small amount of distilled water into the second precipitate for dissolving, and then carrying out freeze drying to obtain a second crude extract;

(3) taking DEAE-Sepharose CL-6B gel, using a circulating water type vacuum pump to remove all gas in the gel, using a glass rod to drain the gas lightly, and filling gel suspension into a glass chromatographic column to avoid generating bubbles;

the constant flow pump was turned on and the column was equilibrated with 2000mL of distilled water. After the balance is finished, preparing a chromatographic column which has the diameter of 4.6cm and the height of 37cm and is filled with DEAE-Sepharose CL-6B gel;

the conditions of use of the column were: the flow rate of the constant flow pump is 0.8mL/min, the automatic part collector collects, and 10mL of collection is set for each pipe;

(4) taking 300mg of the first crude extract obtained in the step (2), dissolving the first crude extract in 10ml of distilled water, and placing the mixture in a water bath kettle at 50 ℃ until the first crude extract is completely dissolved to obtain a first crude extract water solution;

determining the protein content of the first crude extract aqueous solution according to protein: adding trypsin at the mass ratio of 20:1, sealing, keeping the temperature in a water bath kettle at 37 ℃ for 20 hours, and carrying out enzymolysis to obtain an enzymolysis liquid;

slowly loading the enzymolysis liquid into the chromatographic column filled with DEAE-Sepharose CL-6B gel prepared in the step (3), eluting with distilled water for 21h without collecting the eluent, then performing linear gradient elution by using 0.25-0.45 mol/L NaCl aqueous solution, and collecting by using an automatic part collector; the flow rate is 0.8mL/min, and 1 tube is used for collecting 10mL of chromatographic solution;

detecting the collected liquid, determining sugar content distribution in the collected liquid by using a phenol-sulfuric acid method (as shown in figure 7), detecting protein distribution by using an ultraviolet spectrophotometer detection method, combining the collected liquids of 37 th-50 th tubes according to the content distribution conditions of sugar and protein, dialyzing the collected liquid by using a dialysis bag with the molecular weight cut-off of 5000, dialyzing for 18h by using running water, dialyzing for 18h by using distilled water, obtaining a dialyzate A after dialysis is finished, carrying out rotary concentration on the dialyzate A to obtain a polysaccharide concentrated liquid A, and freeze-drying the polysaccharide concentrated liquid A to obtain the decumbent corydalis polysaccharide CPS 1.

(5) Taking 300mg of the second crude extract obtained in the step (2), dissolving the second crude extract in 10ml of distilled water, carrying out centrifugal treatment (5000r/min, and 5min of centrifugal time), slowly loading a supernatant into the chromatographic column filled with DEAE-Sepharose CL-6B gel prepared in the step (3), opening a constant flow pump, eluting for 12h by using distilled water, and collecting by using an automatic part collector;

detecting the collected liquid, measuring the sugar content distribution of the collected liquid by using a phenol-sulfuric acid method (as shown in figure 8), detecting the protein distribution by using an ultraviolet spectrophotometer, combining the collected liquids of 28 th to 56 th tubes according to the sugar and protein content distribution conditions, dialyzing the collected liquid by using a dialysis bag with the molecular weight cut-off of 5000, dialyzing for 18h by using running water, and dialyzing for 18h by using distilled water. And (3) obtaining dialysate B after dialysis, concentrating the dialysate B to obtain polysaccharide concentrated solution B, and freeze-drying the polysaccharide concentrated solution B to obtain corydalis amabilis polysaccharide CPW 2.

Comparative example 1

The remaining steps were in accordance with example 2.

The comparative example is different from example 2 in that in step (4), linear gradient elution is carried out by using NaCl solutions with the concentrations of 0 and 1mol/L, namely linear gradient elution is carried out by using NaCl aqueous solution with the concentration of 0-1 mol/L, and the obtained polysaccharide is named CPS 1-P.

Comparative example 2

The remaining steps were in accordance with example 2.

This comparative example differs from example 2 in that, in step (4), no enzymatic hydrolysis is carried out, the first crude extract is subjected directly to DEAE-Sepharose CL-6B chromatography, and the polysaccharide obtained is designated CPS 1-E.

Comparative example 3

The remaining steps were in accordance with example 2.

This comparative example differs from example 2 in that the first crude extraction was directly purified by step (5) to obtain a first crude polysaccharide purified sample, CPW.

Application example 1

Uniformity and purity identification

1. Uniformity and purity identification of rhizoma corydalis Decumbentis polysaccharide CPS1

1) Detection method

The homogeneity of the components of the decumbent corydalis polysaccharide CPS1 and comparative examples 1 and 2 was identified by High Performance Size Exclusion Chromatography (HPSEC).

The chromatography was carried out using a surfks-804 column with ultrapure water as a mobile phase at a flow rate of 1mL/min and a column temperature of 50 ℃ and was detected by a differential Refractometer (RIU). And (3) performing full spectrum scanning (190-800 nm) on 0.5-1 mg/mL decumbent corydalis polysaccharide CPS1 aqueous solution to detect the purity of the decumbent corydalis polysaccharide CPS1 and the purity of the comparative examples 1 and 2.

2) Results

The high performance size exclusion chromatography result of rhizoma corydalis Decumbentis polysaccharide CPS1 is shown in FIG. 9. FIG. 9 shows that only 1 peak appears in rhizoma corydalis Decumbentis polysaccharide CPS1 at 6.214min, and the peak has sharp and symmetrical shape, which indicates that CPS1 has good uniformity and single component.

Through 190-800 nm full-wavelength scanning, a full-wavelength scanning graph is shown in fig. 10, the corydalis amabilis polysaccharide CPS1 does not contain protein and nucleic acid impurities, and the purity of the extracted corydalis amabilis polysaccharide CPS1 is high.

The high performance size exclusion chromatogram of CPS1-P is shown in FIG. 11, and FIG. 11 shows that CPS1-P, which is a product not eluted by saline with a specific concentration, has other impurity peaks at 1.889min, 4.914min and 8.926min in addition to CPS1, and the 3 impurities account for about 35% according to peak area. The concentration range of the NaCl aqueous solution used for linear gradient elution is enlarged, and although the target polysaccharide can be obtained by elution, the impurities are more, which is not beneficial to obtaining the target product.

The high performance size exclusion chromatogram of CPS1-E is shown in FIG. 12, the full-wavelength scan is shown in FIG. 13, FIG. 12 shows that CPS1-E shows an absorption peak at 5.009min, which is an absorption peak of water-soluble impurities, and the impurities account for about 14% by peak area calculation. FIG. 13 shows CPS1-E showing an absorption peak at 280nm, indicating that CPS1-E contains a hetero protein.

In summary, in embodiment 1 of the present invention, the first crude extract aqueous solution is subjected to enzymolysis, and then subjected to chromatographic separation using a NaCl aqueous solution with a specific concentration, so that various impurities can be effectively removed.

2. Uniformity and purity identification of decumbent corydalis tuber polysaccharide CPW2

1) Detection method

The detection method is the same as that of polysaccharide CPS1 of rhizoma corydalis Decumbentis.

2) Results

The high performance size exclusion chromatography results of decumbent corydalis tuber polysaccharide CPW2 are shown in fig. 14. Fig. 14 shows that decumbent corydalis tuber polysaccharide CPW2 showed 2 peaks at 5.947min and 8.882min, indicating that the polysaccharide component of decumbent corydalis tuber CPW2 is not uniform. The total wavelength scanning of 190-800 nm shows that the decumbent corydalis tuber polysaccharide CPW2 contains no protein and nucleic acid impurities and has high purity as shown in FIG. 15.

The high performance size exclusion chromatogram of CPW is shown in fig. 16, showing at least 5 peaks in fig. 16, indicating that CPW contains many components and many impurities. As can be seen from a comparison of fig. 16 with fig. 14 and 15, the first crude extract does not contain CPW2, which is a target polysaccharide.

Application example 2

Characteristic analysis of rhizoma corydalis Decumbentis polysaccharide CPS1 and rhizoma corydalis Decumbentis polysaccharide CPW2

1. Molecular weight analysis

Identifying the component uniformity of rhizoma corydalis Decumbentis polysaccharide CPS1 and rhizoma corydalis Decumbentis polysaccharide CPW2 by High Performance Size Exclusion Chromatography (HPSEC), preparing molecular weight standard curve based on the peak time of the chromatography column of the supersks-804 according to dextran standard, and calculating the relative molecular mass of rhizoma corydalis Decumbentis polysaccharide CPS1 and rhizoma corydalis Decumbentis polysaccharide CPW 2.

2. Identification of characteristic functional groups of saccharides

The compound type of the sample was analyzed by infrared spectroscopy (FTIR), and 2mg of the sample (decumbent corydalis polysaccharide CPS1 or decumbent corydalis polysaccharide CPW2) was subjected to KBr tabletting and measured by nicolettnexus 470 type infrared spectrometer.

3. Monosaccharide composition analysis

Hydrolyzing 30mg sample (rhizoma corydalis Decumbentis polysaccharide CPS1 or rhizoma corydalis Decumbentis polysaccharide CPW2) with 1mol/L sulfuric acid at 100 deg.C for 8 hr, neutralizing hydrolysate with barium carbonate to neutrality, separating, and freeze drying supernatant to obtain monosaccharide hydrolysate. After derivatization of the hydrolyzate by trimethylsilylation, the derivatives were analyzed by gas chromatography: the hp-5 capillary chromatographic column is programmed to 160 ℃→ 180 ℃ (20 ℃/min) → 220 ℃ (8 ℃/min, 2min hold → 250 ℃ (2min), and the detector temperature is 280 ℃.

4. Results

1) Preparing a molecular mass standard curve according to the standard glucan to obtain an equation of-3.92 x +6.314 (R)²0.99), calculating the molecular mass of the polysaccharide CPS1 of the corydalis amabilis to be 360kDa according to the HPSEC peak time of the polysaccharide CPS1 of the corydalis amabilis of 6.214 min.

According to GC results of standard monosaccharide derivatives and gas chromatography results of decumbent corydalis tuber polysaccharide CPS1 (in FIG. 17, 1-4 marks in the figure represent glucose, galactose, mannose and arabinose isomers respectively), decumbent corydalis tuber polysaccharide CPS1 is composed of glucose, galactose, mannose and arabinose, and the molar ratio is 4.9:2.0:1: 1.9. The infrared spectrum result shows that the polysaccharide CPS1 of rhizoma corydalis Decumbentis is 3400cm^-1，2900cm^-1，1650cm^-1And 1100cm^-1The characteristic functional groups of the saccharides are present.

2) Preparing a molecular mass standard curve according to the standard glucan to obtain an equation of-3.92 x +6.314 (R)²0.99), the decumbent corydalis tuber polysaccharide CPW2 was calculated to be polymerized from heterogeneous polysaccharides having molecular weights of 550kDa and 55kDa, with a molar ratio of 1:4 calculated from the peak area.

According to standard monosaccharidesThe GC results of the derivatives and the gas chromatography results of the decumbent corydalis tuber polysaccharide CPW2 (fig. 18, in which the label of 1 represents glucose isomer) show that the decumbent corydalis tuber polysaccharide CPW2 is composed of single glucose, and the decumbent corydalis tuber polysaccharide CPW2 is a homopolysaccharide. The infrared spectrum result shows that CPW2 is 3400cm^-1，2900cm^-1，1650cm^-1And 1100cm^-1The characteristic functional groups of the saccharides are present.

Application example 3

Anti-inflammatory action research of rhizoma corydalis Decumbentis polysaccharide CPS1 and rhizoma corydalis Decumbentis polysaccharide CPW2

1. Cytotoxicity

RAW264.7 cells were cultured in DMEM medium, complete medium containing 10% serum and 1% diabody, and the cells were subcultured at 37 ℃ in a 5% carbon dioxide incubator for 48 h.

The cytotoxicity of the decumbent corydalis polysaccharide CPS1 and the decumbent corydalis polysaccharide CPW2 on RAW264.7 is detected by using an MTT method, and six mass concentrations of the decumbent corydalis polysaccharide, namely 600 mug/mL, 300 mug/mL, 150 mug/mL, 75 mug/mL, 25 mug/mL and 1 mug/mL, are set after cells are cultured in a 96-well plate.

The inhibition rate is generally considered to be below 20 percent, namely no cytotoxicity exists, and the inhibition effect of the rhizoma corydalis Decumbentis polysaccharide CPS1 added with 75 mu g/mL or 150 mu g/mL on the growth of RAW264.7 cells is respectively 15.7 percent and 16.1 percent through the cytotoxicity test, so that no cytotoxicity exists; the addition of decumbent corydalis tuber polysaccharide CPW2 with mass concentration of 600 μ g/mL or less has no cytotoxicity to RAW264.7 cell growth.

2. Anti-inflammatory action

Lipopolysaccharide (LPS) at 1. mu.g/mL was used to induce inflammation in RAW264.7 cells, and 3 replicates were set for each group, with samples of blank group (no inflammation induced), negative control group (inflammation induced by LPS at 1. mu.g/mL), positive control group (DXMS, dexamethasone at 75. mu.g/mL), polysaccharide CPS1 of decumbent corydalis (75. mu.g/mL or 150. mu.g/mL), and polysaccharide CPW2 of decumbent corydalis (75. mu.g/mL or 150. mu.g/mL).

Extracting total RNA from each group of cells according to the instruction of a total RNA extraction kit (Promega corporation), carrying out reverse transcription by using a reverse transcription kit to obtain cDNA, carrying out real-time fluorescence quantitative PCR by using a qPCR MasterMix kit (Promega corporation), taking housekeeping gene GAPDH as an internal reference gene, and carrying out 2^-ΔΔCTThe relative expression level of mRNA of each inflammatory factor was calculated by the method. The results of the measurements are shown in tables 4 and 5, and fig. 19 and 20;

in FIG. 19, A is an expression profile of TNF- α, B is an expression profile of IL-1 β, C is an expression profile of IL-6, and D is an expression profile of COX-2;

in FIG. 20, A is an expression profile of TNF-. alpha.B is an expression profile of IL-6, C is an expression profile of COX-2, and D is an expression profile of iNOS.

TABLE 4 inhibitory Effect of CPS1 on lipopolysaccharide-induced inflammatory factors in RAW264.7 cells

The anti-inflammatory results of decumbent corydalis tuber polysaccharide CPS1 are shown in FIG. 19 and Table 4, and the histograms corresponding to different letters in FIG. 19 show the expression influence of different groups on different inflammatory factors, and the difference is significant (P <0.05) through significance analysis. The decumbent corydalis polysaccharide CPS1 sample groups with the mass concentration of 75 mug/mL or 150 mug/mL can obviously reduce the relative expression quantity (P <0.05) of mRNA of inflammatory factors TNF-alpha and COX-2, and the inhibition rates (P >0.05) of the TNF-alpha and COX-2 expression of the two sample groups and a positive control group are not obviously different, which indicates that the anti-inflammatory effect of the decumbent corydalis polysaccharide CPS1 is equivalent to that of DXMS. The decumbent corydalis tuber polysaccharide CPS1 can also remarkably reduce the mRNA relative expression quantity (P <0.05) of inflammatory factors IL-1 beta and IL-6 in RAW264.7 cells induced by lipopolysaccharide.

TABLE 5 inhibitory Effect of CPW2 on LPS-induced inflammatory factors in RAW264.7 cells

The anti-inflammatory results of decumbent corydalis tuber polysaccharide CPW2 are shown in fig. 20 and table 5, and the histograms corresponding to different letters in fig. 20 show the expression effect of different groups on different inflammatory factors, and the difference is significant (P <0.05) through significance analysis. The corydalis amabilis polysaccharide CPW2 sample groups with the mass concentration of 75 mu g/mL or 150 mu g/mL can obviously reduce the relative expression quantity (P <0.05) of mRNA of inflammatory factors TNF-alpha and COX-2, and the two sample groups with different mass concentrations have no obvious difference, which indicates that no dose-effect relationship exists. The decumbent corydalis tuber polysaccharide CPW2 can also remarkably reduce the relative expression quantity (P <0.05) of mRNA of inflammatory factor iNOS in RAW264.7 cells induced by lipopolysaccharide.

In conclusion, the polysaccharide CPS1 and CPW2 of corydalis amabilis provided by the invention have good anti-inflammatory effect.

Although the present invention has been described with reference to the preferred embodiments, it should be understood that various changes and modifications can be made therein by those skilled in the art without departing from the spirit and scope of the invention as defined in the appended claims.