首页> 美国卫生研究院文献>PLoS Clinical Trials >Approach to Analyze the Diversity of Myxobacteria in Soil by Semi-Nested PCR-Denaturing Gradient Gel Electrophoresis (DGGE) Based on Taxon-Specific Gene
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Approach to Analyze the Diversity of Myxobacteria in Soil by Semi-Nested PCR-Denaturing Gradient Gel Electrophoresis (DGGE) Based on Taxon-Specific Gene

机译:基于分类群特异性基因的半巢式PCR-变性梯度凝胶电泳(DGGE)分析土壤中黏细菌的多样性

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摘要

The genotypic diversity of insoluble macromolecules degraded myxobacteria, provided an opportunity to discover new bacterial resources and find new ecological functions. In this study, we developed a semi-nested-PCR-denaturing gradient gel electrophoresis (DGGE) strategy to determine the presence and genotypic diversity of myxobacteria in soil. After two rounds of PCR with myxobacteria-specific primers, an 194 bp fragment of mglA, a key gene involved in gliding motility, suitable for DGGE was obtained. A large number of bands were observed in DGGE patterns, indicating diverse myxobacteria inhabiting in soils. Furthermore, sequencing and BLAST revealed that most of the bands belonged to the myxobacteria-group, and only three of the twenty-eight bands belonged to other group, i.e., Deinococcus maricopensis. The results verified that myxobacterial strains with discrepant sequence compositions of gene mglA could be discriminated by DGGE with myxobacteria-specific primers. Collectively, the developed semi-nested-PCR-DGGE strategy is a useful tool for studying the diversity of myxobacteria.
机译:不溶性大分子的基因型多样性降解了粘杆菌,为发现新的细菌资源和发现新的生态功能提供了机会。在这项研究中,我们开发了一种半巢式PCR变性梯度凝胶电泳(DGGE)策略,以确定土壤中黏细菌的存在和基因型多样性。在使用粘细菌特异性引物进行两轮PCR之后,获得了194 bp的mglA片段,mglA是参与滑动运动的关键基因,适用于DGGE。在DGGE模式中观察到大量条带,表明土壤中存在多种多样的黏细菌。此外,测序和BLAST显示,大多数条带属于粘细菌群,而28个条带中只有三个属于其他组,即马氏弧菌(Deinococcus maricopensis)。结果证明,DGGE可以通过粘菌特异性引物来区分具有基因mglA的序列组成差异的粘菌菌株。总的来说,已开发的半巢式PCR-DGGE策略是研究粘细菌多样性的有用工具。

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