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Method for rapid DNA extraction from bacterial communities of different soils

机译:从不同土壤细菌群落中快速提取DNA的方法

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摘要

A method for indirect DNA extraction from various soils significantly differing in their physicochemical properties has been developed. The proposed method is based on cell desorption from soil particles using a Tris-EDTA (TE) buffer supplemented with polyvinylpolypyrrolydone (PVPP) and sodium dodecylsulfate (SDS). Methods for subsequent cell lysis and purification of DNA preparations based on alkaline lysis followed by chromatography on ion-exchange resins were described by us earlier. The purity of the DNA preparations obtained did not depend on the type of soil. It was shown that the DNA preparations can be used for the amplification of rather large fragments, e.g., sequences spanning the complete 16S rRNA gene.
机译:已经开发了一种从各种物理化学性质明显不同的土壤中间接提取DNA的方法。所提出的方法是基于使用Tris-EDTA(TE)缓冲液补充了聚乙烯基聚吡咯烷酮(PVPP)和十二烷基硫酸钠(SDS)从土壤颗粒中解吸细胞的方法。我们先前已描述了随后的细胞裂解方法以及基于碱裂解法纯化DNA制品,然后在离子交换树脂上进行色谱分离的方法。获得的DNA制剂的纯度不取决于土壤的类型。结果表明,该DNA制备物可用于扩增相当大的片段,例如,跨越完整的16S rRNA基因的序列。

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