Method for preparing and regenerating phomopasis asparagi protoplast
A technology of asparagus stem blight and protoplasts, which is applied in the field of asparagus stem blight protoplast preparation and regeneration, and can solve the molecular mechanism and research of unfavorable pathogenic bacteria
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example 1
[0038] Example 1: Collect the conidia produced by the pycnidia on oat solid medium (OA), inoculate them in complete liquid medium (CM), and culture them on a shaker at 150r / min at 25°C for 36h to obtain fresh bacteria Silk, using a mixed enzyme of 1.5% lyase, 1.0% collapse enzyme, and 1.5% helicase: pH 6.00, enzymatically hydrolyze in a water bath at 30°C for 3.0h, and use 1.0mol / L MgSO 4 (10mmol / LPBS preparation, the volume ratio is MgSO 4 : PBS=3:1) as an osmotic pressure stabilizer; dilute the protoplast suspension 100 times with a 0.6mol / L sucrose solution, take 0.1mL of the diluted solution and spread it on a potato dextrose agar plate and a hyperosmotic potato dextrose agar plate Cultured at 25°C for 3-5 days, the number of protoplasts reached 1.7×10 7 cells / mL, the regeneration rate was 22.0%.
example 2
[0039] Example 2: Collect the conidia produced by the pycnidia on the oat solid medium (OA), and inoculate them in complete liquid medium (CM), and cultivate them on a shaker at 150r / min for 48 hours at 25°C to obtain fresh bacteria Silk, using a mixed enzyme of 1.5% lyase, 1.0% collapse enzyme and 1.5% helicase: pH 7.60, enzymolysis in 35°C water bath for 4.0h, with 1.0mol / L MgSO 4 (10mmol / LPBS preparation, the volume ratio is MgSO 4 : PBS=3:1) as an osmotic pressure stabilizer; dilute the protoplast suspension 100 times with a 0.6mol / L sucrose solution, take 0.1mL of the diluted solution and spread it on a potato dextrose agar plate and a hyperosmotic potato dextrose agar plate Cultured at 25°C for 3-5 days, the number of protoplasts reached 2.2×10 7 cells / mL, the regeneration rate was 22.5%.
example 3
[0040] Example 3: Collect the conidia produced by the pycnidia on the oat solid medium (OA), and inoculate them in complete liquid medium (CM), and cultivate them on a shaking table at 150r / min for 72h at 25°C to obtain fresh bacteria Silk, using a mixed enzyme of 1.5% lyase, 1.0% collapse enzyme and 1.5% helicase: pH 6.98, hydrolyze in a water bath at 33°C for 4.5h, and use 1.0mol / L MgSO 4 (10mmol / LPBS preparation, the volume ratio is MgSO 4 : PBS=3:1) as an osmotic pressure stabilizer; dilute the protoplast suspension 100 times with a 0.6mol / L sucrose solution, take 0.1mL of the diluted solution and spread it on a potato dextrose agar plate and a hyperosmotic potato dextrose agar plate Cultured at 25°C for 3-5 days, the number of protoplasts reached 2.8×10 7 cells / mL, the regeneration rate was 24.0%.
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