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        【原创】最简单的DNA提取方法

        丁香园论坛

        5138
        本人经常用以下方法提取DNA,做PCR,效果不错,很简单.大家可以尝试下!整个过程不需要离心.

        1. Lysis: the lysis buffer (usually 0.5ml) is added to the tissue or cell ( for a 75cm2 flask, add 5ml directly to the cell). Digestion is complete within several hours at 37C (cell, 2-3h) or 55C (tissue) with agitation.
        Lysis buffer
        100mM Tris Hcl pH 8.5 5ml
        0.5M EDTA 0.5ml
        10% SDS 1ml
        5M NaCl 2ml
        20mg/ml Proteinase K 0.25ml
        Bring up to 50ml with dd water
        2. isopropanol precipitation: one volume of isopropanol is added to the lysate and the samples are mixed or swirled until precipitation is complete ( about 10-20 min ) (viscosity completely gone).
        3. Recovery of precipitate: the DNA is recovered by lifting the aggregated precipitate from the solution using a disposable yellow tip. Excess liquid is dabbed off and the DNA is dispersed in a prelabeled Eppendorf tube containing, depending on the size of the precipitate, 20 to 500ul to 10mM Tris HCl, 0.1mM EDTA, pH 7.5. complete dissolution of the DNA may requires several hours of agitation at 37C or 55C (may need overnight). It is important that the DNA is completely dissolved to ensure the reproducible removal of aliquots for analysis.
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