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首页> 外文期刊>Journal of Clinical Microbiology >rpoB Gene Analysis as a Novel Strategy for Identification of Spirochetes from the Genera Borrelia,Treponema, and Leptospira
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rpoB Gene Analysis as a Novel Strategy for Identification of Spirochetes from the Genera Borrelia,Treponema, and Leptospira

机译:rpoB基因分析作为一种新的鉴定螺旋藻属,螺旋体和钩端螺旋体的策略

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摘要

Spirochetes are emerging pathogens for which culture and identification are partly unresolved. In fact, 16S rRNA-based sequencing is by far the most widely used PCR methodology that is able to detect such uncultivable pathogens. However, this assay actually has some limitations linked to potential problems of contamination, which hampers diagnosis. To circumvent this, we have devised a simple PCR strategy involving targeting of the gene encoding the RNA polymerase beta subunit (rpoB), a highly conserved enzyme. The complete sequence of the Leptospira biflexa (serovar patoc)rpoB gene was determined and compared with the published sequences for Borrelia burgdorferi and Treponema pallidum. From the resulting analysis, degenerate nucleotide primers were designed and tested for their ability to amplify a portion of the rpoB gene from various spirochetes. Using two different pairs of these primers, we succeeded in obtaining specificrpoB-amplified fragments for all members of the generaLeptospira, Treponema, and Borreliatested and no other bacteria. Our findings may have significant implications for the development of a new tool for the identification of spirochetes, especially if clinical samples are contaminated or when the infecting strain is uncultivable.
机译:螺旋体是新兴的病原体,其培养和鉴定尚不能部分解决。实际上,基于16S rRNA的测序是迄今为止使用最广泛的PCR方法,能够检测到这种无法培养的病原体。然而,该测定法实际上具有与潜在的污染问题相关的一些局限性,这限制了诊断。为了避免这种情况,我们设计了一种简单的PCR策略,涉及靶向编码高度保守的RNA聚合酶β亚基( rpoB )的基因。确定了 Leptospira biflexa (serovar patoc) rpoB 基因的完整序列,并将其与已发表的 Borrelia burgdorferi Treponema的序列进行比较。苍白的。从结果分析中,设计了简并的核苷酸引物,并测试了它们从各种螺旋体扩增部分 rpoB 基因的能力。使用两对不同的引物,我们成功地获得了对 Leptospira Treponema 的所有成员的特定 rpoB 扩增片段。已通过em> Borrelia 测试,没有其他细菌。我们的发现可能对开发一种鉴定螺旋体的新工具具有重要意义,尤其是在临床样品被污染或感染菌株无法培养的情况下。

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