Method for preparing linseed polysaccharide having antiviral activity and immunological activity, and use of the linseed polysaccharide

The invention claimed is: 1. A method for preparing a linseed polysaccharide, comprising: (1) separation of the husks from the kernels of the linseeds: pulverizing the linseeds, sieving the pulverized linseeds to form linseed powder, then thoroughly mixing the linseed powder(s) with ethanol and glycerol, centrifuging for 20-30 minutes, and respectively collecting the linseed kernels in the upper layer and depositing the linseed husks in the bottom layer, wherein the volume ratio between the glycerol and the ethanol is 15: 3-4; (2) extraction of the linseed polysaccharides: extracting polysaccharides from the linseed husks obtained in step (1) by microwave-assisted hot water extraction, sieving the extracted solutions, collecting the concentrated solutions, and freeze-drying the concentrated solutions under vacuum; (3) separation of the linseed polysaccharides: deproteinizing the freeze-dried crude extracts obtained in step (2) by Sevage method to obtain a first supernatant, the first supernatant being subject to the Sevage method for 25-30 times to obtain a final supernatant; adding anhydrous ethanol into the final supernatants, standing for precipitation for 4-12 h, centrifuging at a speed of 3500-5000 r/min for 20-30 min to obtain precipitates, and freeze-drying the precipitates under vacuum, so as to obtain the linseed husk crude polysaccharides; wherein the Sevage method comprises mixing the freeze-dried crude extract obtained in step (2) or the first supernatant with Sevage reagent in a volume ratio of 1: 1-1:3, shaking for 20-30 min, centrifuging at a speed of 3500-5000 r/min; and wherein the Sevage reagent comprises chloroform and n-butanol with a volume ratio of 3: 1-5:1; and (4) purification of the linseed polysaccharides: formulating the linseed husk crude polysaccharides obtained in step (3) into 5-8 mg/mL solutions, purifying by a chromatographic column A, eluting with water, and detecting the polysaccharides by a phenol-sulfuric acid method, combining the collection liquids showing a positive result in the sugar reaction, concentrating by rotary evaporation at 50-60° C., dialyzing, then freeze-drying under vacuum; formulating the dried polysaccharides into 2-5 mg/mL solutions, purifying by a chromatographic column B, eluting with distilled water, collecting the polysaccharide components, dialyzing, ultra-filtrating, concentrating and freeze-drying, so as to obtain the linseed polysaccharide. 2. The method for preparing a linseed polysaccharide according to claim 1 , wherein the linseeds are pulverized, then sieved via a 20-mesh sieve. 3. The method for preparing a linseed polysaccharide according to claim 1 , wherein the microwave-assisted hot water extraction in step (2) is carried out under the conditions: solid-to-liquid ratio is 1: 20-1:30 (w/v), the extraction temperature is 60-100° C., the extraction time is 40-60 min, the output power is 600-800W, the stirring speed is 600-900 r/min, and the extracted solution obtained by the microwave-assisted hot water extraction is sieved via a 100-mesh sieve. 4. The method for preparing a linseed polysaccharide according to claim 1 , wherein in step (3), the amount of the anhydrous ethanol is 3-5 times of the volume of the linseed husk crude polysaccharide solution, and after the anhydrous ethanol is added, the solution is stood for precipitation at 4° C. for 4-12 h. 5. The method for preparing a linseed polysaccharide according to claim 1 , wherein in step (4), the chromatographic column A is a DEAE-Sepharose Fast Flow ion exchange column, the chromatographic column B is a Sephadex G-100 Sephadex gel column; the membrane in the ultra-filtration process has a molecular weight cutoff of 1×10 6 Da; the dialysis time is 48 hr, and the dialysis bag has a molecular weight cutoff of 3000-5000 Da.