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首页> 外文期刊>Microbes and Environments >Improvements in Bacterial Primers to Enhance Selective SSU rRNA Gene Amplification of Plant-associated Bacteria by Applying the LNA Oligonucleotide-PCR Clamping Technique
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Improvements in Bacterial Primers to Enhance Selective SSU rRNA Gene Amplification of Plant-associated Bacteria by Applying the LNA Oligonucleotide-PCR Clamping Technique

机译:通过应用LNA寡核苷酸PCR钳夹技术改进细菌引物以增强植物相关细菌的选择性SSU rRNA基因扩增

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摘要

PCR clamping by locked nucleic acid (LNA) oligonucleotides is an effective technique for selectively amplifying the community SSU rRNA genes of plant–associated bacteria. However, the original primer set often shows low amplification efficiency. In order to improve this efficiency, new primers were designed at positions to compete with LNA oligonucleotides. Three new sets displayed higher amplification efficiencies than the original; however, efficiency varied among the primer sets. Two new sets appeared to be available in consideration of bacterial profiles by next-generation sequencing. One new set, KU63f and KU1494r, may be applicable to the selective gene amplification of plant-associated bacteria.
机译:通过锁定核酸(LNA)寡核苷酸进行的PCR钳制是一种有效扩增植物相关细菌的SSU rRNA社区基因的有效技术。但是,原始引物组通常显示出低扩增效率。为了提高效率,在与LNA寡核苷酸竞争的位置设计了新的引物。三套新设备显示出比原始设备更高的放大效率;但是,引物组之间的效率各不相同。考虑到下一代测序的细菌概况,似乎有两套新产品可用。一套新的KU63f和KU1494r可用于植物相关细菌的选择性基因扩增。

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