A method for extracting the genome of wild rose endophytic fungi
An endophytic fungi and genome technology, applied in recombinant DNA technology, DNA preparation, etc., can solve the problems of low purity, poor extraction effect, and low extraction rate of genomic DNA, and achieve improved extraction rate, high yield and high purity. Effect
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Embodiment 1
[0023] Example 1 Liquid nitrogen grinding combined with CTAB (cetyltrimethylammonium bromide) method to extract wild rose endophytic fungus genome
[0024] (1) Preparation of reagents:
[0025] Sample pretreatment reagents include 0.5M EDTA (pH=8.0), 1M Tris-HCl solution, CTAB solution, β-mercaptoethanol, phenol: chloroform: isoamyl alcohol, isopropanol, ethanol with a concentration of 70% by mass, anhydrous Ethanol, 5% sodium hypochlorite; The preparation method of described reagent is as follows:
[0026] Preparation of 70% alcohol: measure 60mL sterile deionized water and 140mL absolute ethanol respectively, mix and store at room temperature.
[0027] Preparation of 5% sodium hypochlorite: Measure 100 mL of 10% sodium hypochlorite and 100 mL of sterile deionized water respectively, mix them, and store them in the dark at room temperature.
[0028] Preparation of 0.5M EDTA (pH=8.0): Take 186.1g Na 2 EDTA·2H 2 O, adjusted to pH = 8.0 with NaOH (about 20 g), filtered ddH 2 ...
Embodiment 2
[0047] Example 2 Liquid nitrogen grinding combined with soil microbial DNA strong extraction kit to extract wild rose endophytic fungus genome
[0048] (1) Preparation of reagents:
[0049] The sample pretreatment reagent has 70% dehydrated alcohol and 5% sodium hypochlorite. The preparation method is the same as in Example 1, and the DNA extraction kit adopts Reagent test kit, The kit contains Solution C1~Solution C6.
[0050] (2) Surface disinfection of samples
[0051] Weigh 2g of wild rose sample; divide the prepared 70% alcohol and 5% sodium hypochlorite solution into two 250mL sterile beakers; place the plant tissue in 70% alcohol to completely soak all the plant tissue, and the soaking time is 1 to 2 minutes; wash with sterile water three times; place the plant tissue block in 5% sodium hypochlorite solution to completely soak all the plant tissue for 30 to 60 seconds; wash with sterile water for five times; sterilize the surface Plant tissues were collected on st...
Embodiment 3
[0080] Example 3 liquid nitrogen grinding combined with CTAB mixed solution and Kit to extract endophytic fungus genome from wild rose
[0081] (1) Preparation of reagents:
[0082] Sample pretreatment reagents include 0.5M EDTA (pH=8.0), 1M Tris-HCl solution, CTAB extract, 70% absolute ethanol, 5% sodium hypochlorite, CTAB mixed solution, β-mercaptoethanol, PVP (polyvinylpyrrolidone); The preparation method of described reagent is as follows:
[0083] The preparation method of said 0.5M EDTA (pH=8.0), 1M Tris-HCl solution, CTAB extract, 70% dehydrated alcohol, 5% sodium hypochlorite is the same as described in Example 1
[0084] Preparation of the CTAB mixed solution: measure 200 mL of 2% CTAB extract, add 20 g of PVP, sterilize (115° C., 15 min), store at room temperature, add 4 mL of β-mercaptoethanol before use.
[0085] Other reagents can be provided by the kit or purchased through reagent companies.
[0086] (2) Surface disinfection of samples
[0087] Weigh 2g of w...
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