Technique for preparing fugui ostealgia compound by microorganism fermentation method
A microbial fermentation method and osmanthus bone technology, applied in the direction of microorganism-based methods, microorganisms, biochemical equipment and methods, etc., can solve the problems of large side effects, low content of active ingredients, and unclear active ingredients of guigu pain, and achieve Improve the curative effect of the drug, high drug efficacy, and increase the yield of the extract
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Embodiment 1
[0037] The preparation technology of embodiment 1 fermentation method production Fugui Gutong compound
[0038] 1. Preparation of Aspergillus niger Suspension
[0039] 1) Prepare plate medium:
[0040] Weigh 45g of nutrient agar and 20g of glucose, add it to 1000ml of distilled water, heat to boil, and stir with a glass rod at the same time, after the nutrient agar and glucose are completely dissolved in water (the water can be properly replenished when heating), put it into a triangular flask, and use 8 layers of gauze Make a stopper to stop the bottle mouth, then seal it with 4 layers of newspaper and cotton thread, and put it in a vertical pressure steam sterilizer to sterilize at 121°C for 20 minutes.
[0041] Quickly pour about 15ml of culture medium into a sterilized petri dish, cover and shake the petri dish so that the culture medium is evenly distributed on the bottom of the petri dish, place it flat on the table, and solidify to become a plate culture medium.
[00...
Embodiment 2
[0054] Example 2 Determination of the total alkaloid content of Aconitum aconitum in the extract by ion-pair extraction spectrophotometry
[0055] Aconitine was used as the reference substance. Precisely measure 50 mL of the extract prepared according to the method described in Example 1 "2. Compound Fermentation", adjust the pH value to 9 by adding ammonia to the test solution, extract 4 times with ether (25, 20, 15, 10 mL), and combine ether layer, and evaporated to dryness on a water bath. Add an appropriate amount of 0.01mol / L hydrochloric acid solution to the residue to dissolve it, transfer it to a 10mL measuring bottle, add 0.01mol / L hydrochloric acid solution to dilute to the mark, and shake well to obtain the test solution.
[0056] Precisely measure a certain amount of aconitine reference substance solution or test solution in a separatory funnel, add 5.0 mL of citric acid-disodium hydrogen phosphate buffer solution with a pH value of 3.50, 2.0 mL of BCG test soluti...
Embodiment 3
[0057] Example 3 Determination of Paeoniflorin Content in Extract by High Performance Liquid Chromatography
[0058] Be the chromatographic column Diamonsil C18 (150mm * 4.6mm, 5 μm) of filler with octadecylsilane bonded silica gel; Acetonitrile-0.1% phosphoric acid solution (14: 86) is mobile phase; Detection wavelength is 230nm; Column temperature is 40 ℃. Injection volume: 20 μL.
[0059] Accurately weigh a certain amount of paeoniflorin reference substance, add methanol to dissolve, and dilute to the scale solution to make a solution containing 0.5 μg per 1 mL, shake well to obtain paeoniflorin reference substance solution.
[0060] Accurately measure 1.5mL of the extract under item 2 with a pipette, evaporate to dryness in a water bath at low temperature, add 10mL of methanol to the residue, sonicate for 10 minutes to dissolve, centrifuge for 20 minutes (1500r / min), and transfer the supernatant to a 25mL volumetric flask, and make up to the mark with methanol. That is,...
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