Method for extracting plant tissue culture seedling genome DNA (Deoxyribose Nucleic Acid)
A plant tissue culture and genome technology, applied in the field of molecular biology, can solve the problems of increased genomic DNA contamination, loss of natural characteristics, time-consuming and labor-intensive in the extraction process, and achieves the protection of natural activity, shortening extraction time, and convenient process. Effect
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Embodiment 1
[0035] Select 0.5 g of fresh Pinellia tissue-cultured leaf tissue and put it into a commercial EP tube (specification 1.5 mL); add 1000 μL of SDS and CTAB mixed extract with a volume ratio of 2:1 after preheating with warm water at 65 °C, Shake for 5 minutes; use the tip of a pipette (200 μL) to insert into the bottom of the above EP tube, slowly rotate clockwise to pick up the filamentous viscous substance, which is the obtained genomic DNA, and dissolve it in 50 μL pure water; take the dissolved 3 μL of the final solution was carried out for 1% agarose electrophoresis detection, and the results were as follows figure 1 shown.
Embodiment 2
[0037] Select 0.5g fresh leaf tissue of Bletilla striata tissue culture seedlings at -20°C, put it into a commercial EP tube (1.5mL size); add 65°C warm water to preheat, and mix SDS and CTAB with a volume ratio of 3:1 for extraction Mix 1000 μL of solution for 5 minutes; use the tip of a pipette (200 μL) to insert into the bottom of the above-mentioned EP tube, slowly rotate clockwise to pick up the filamentous viscous substance, which is the obtained genomic DNA, and dissolve it in 50 μL of pure water ; Take 5 μL of the dissolved solution, and carry out 1% agarose electrophoresis detection, the result is as follows: figure 2 shown.
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