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首页> 外文期刊>Journal of Applied Bacteriology >DIFFERENTIATION OF LISTERIA ISOLATES BY PCR AMPLICON PROFILING AND SEQUENCE ANALYSIS OF 16S-23S RRNA INTERNAL TRANSCRIBED SPACER LOCI
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DIFFERENTIATION OF LISTERIA ISOLATES BY PCR AMPLICON PROFILING AND SEQUENCE ANALYSIS OF 16S-23S RRNA INTERNAL TRANSCRIBED SPACER LOCI

机译:通过PCR扩增子扩增和分离16S-23S RRNA内部翻译间隔位点的方法鉴定LI草分离物

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摘要

The 16S-23S rRNA internal transcribed spacer region (ITS) in genomic DNA from Listeria species was amplified and sequenced so as to find sequence differences that would allow rapid species and strain differentiation. Agarose gel profiles of amplicons generated with primers designed to amplify ITS loci indicated that Listeria DNA can contain at least two distinct ITS regions. The direct sequencing of the smaller of these ITS amplicons (330 bp) was found useful for the rapid and accurate differentiation of various Listeria species. On the other hand analysis of ITS amplicons generated from a total of 27 L. monocytogenes strains indicated that 4/27 of these strains could be distinguished on the basis of their ITS profile (the presence of a unique 350 bp amplicon). The lack of sequence heterogeneity in the small 333 bp amplicon did not permit rapid strain differentiation.
机译:对来自李斯特菌属物种的基因组DNA中的16S-23S rRNA内部转录间隔区(ITS)进行了扩增和测序,以便发现可以实现快速物种和菌株分化的序列差异。用设计用于扩增ITS基因座的引物产生的扩增子的琼脂糖凝胶谱表明,李斯特菌DNA可以包含至少两个不同的ITS区域。发现较小的这些ITS扩增子(330 bp)的直接测序可用于快速准确地区分各种李斯特菌。另一方面,对总共27种单核细胞增生李斯特菌菌株产生的ITS扩增子的分析表明,根据它们的ITS谱(存在独特的350 bp扩增子),可以区分出4/27个菌株。 333 bp的小扩增子缺少序列异质性,无法快速区分菌株。

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