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Use of Single-Point Genome Signature Tags as a Universal Tagging Method for Microbial Genome Surveys

机译:使用单点基因组签名标签作为微生物基因组调查的通用标记方法

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We developed single-point genome signature tags (SP-GSTs), a generally applicable, high-throughput sequencing-based method that targets specific genes to generate identifier tags from well-defined points in a genome. The technique yields identifier tags that can distinguish between closely related bacterial strains and allow for the identification of microbial community members. SP-GSTs are determined by three parameters: (i) the primer designed to recognize a conserved gene sequence, (ii) the anchoring enzyme recognition sequence, and (iii) the type IIS restriction enzyme which defines the tag length. We evaluated the SP-GST method in silico for bacterial identification using the genes rpoC, uvrB, and recA and the 16S rRNA gene. The best distinguishing tags were obtained with the restriction enzyme Csp6I upstream of the 16S rRNA gene, which discriminated all organisms in our data set to at least the genus level and most organisms to the species level. The method was successfully used to generate Csp6I-based tags upstream of the 16S rRNA gene and allowed us to discriminate between closely related strains of Bacillus cereus and Bacillus anthracis. This concept was further used successfully to identify the individual members of a defined microbial community.
机译:我们开发了单点基因组签名标签(SP-GST),一种通常适用的高通量测序的方法,其针对特定基因来生成来自基因组中的明确定义的点的标识符标签。该技术产生可区分密切相关的细菌菌株并允许鉴定微生物群落成员的标识符标签。 SP-GSTS由三个参数确定:(i)设计用于识别保守基因序列的引物(ii)锚定酶识别序列,和(iii)限定标签长度的IIS限制酶。我们在硅中评估了SP-GST方法,使用基因RPOC,UVRB和RECA和16S rRNA基因进行细菌鉴定。通过16S rRNA基因的上游的限制酶CSP6i获得了最佳区分标记,这将我们的数据中的所有生物区别为至少对物种水平的组水平和大多数生物。该方法已成功地用于生成16S rRNA基因上游的基于CSP6i的标签,并使我们能够区分芽孢杆菌和芽孢杆菌的密切相关菌株。该概念进一步成功地用于识别定义的微生物群落的个体成员。

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