The genomic DNA was isolated and purified with the improved CTAB methods. The sequences of 16S rRNA gene were amplified by TD-PCR with the bacterium universal primers and the purified PCR products were directly sequenced.

  • 菌株经纯化培养;以改良CTAB法提取总DNA;采用细菌16S rRNA通用引物、TD-PCR方法(touchdown-PCR)进行16S rRNA基因序列扩增;PCR产物纯化后直接进行序列测定;序列经人工校对后用Clustal X进行比对分析;最后用MEGA3.;1软件构建系统发育树。
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