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PCR-Based Method To Differentiate the Subspecies of the Mycobacterium tuberculosis Complex on the Basis of Genomic Deletions

机译:基于基因组缺失的基于PCR的区分结核分枝杆菌复合体亚种的方法

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摘要

The classical Mycobacterium tuberculosis complex (MtbC) subspecies include Mycobacterium tuberculosis, Mycobacterium africanum (subtypes I and II), Mycobacterium bovis (along with the attenuated M. bovis bacillus Calmette-Guérin [BCG]), and Mycobacterium microti; increasingly recognized MtbC groupings include Mycobacterium bovis subsp. caprae and “Mycobacterium tuberculosis subsp. canettii.” Previous investigations have documented each MtbC subspecies as a source of animal and/or human tuberculosis. However, study of these organisms is hindered by the lack of a single protocol that quickly and easily differentiates all of the MtbC groupings. Towards this end we have developed a rapid, simple, and reliable PCR-based MtbC typing method that makes use of MtbC chromosomal region-of-difference deletion loci. Here, seven primer pairs (which amplify within the loci 16S rRNA, Rv0577, IS1561′, Rv1510, Rv1970, Rv3877/8, and Rv3120) were run in separate but simultaneous reactions. Each primer pair either specifically amplified a DNA fragment of a unique size or failed, depending upon the source mycobacterial DNA. The pattern of amplification products from all of the reactions, visualized by agarose gel electrophoresis, allowed immediate identification either as MtbC composed of M. tuberculosis (or M. africanum subtype II), M. africanum subtype I, M. bovis, M. bovis BCG, M. caprae, M. microti, or “M. canettii” or as a Mycobacterium other than MtbC (MOTT). This MtbC PCR typing panel provides an advanced approach to determine the subspecies of MtbC isolates and to differentiate them from clinically important MOTT species. It has proven beneficial in the management of Mycobacterium collections and may be applied for practical clinical and epidemiological use.
机译:经典的结核分枝杆菌复合体(MtbC)亚种包括结核分枝杆菌,非洲分枝杆菌(I和II亚型),牛分枝杆菌(以及减毒的牛分枝杆菌卡莱姆-盖林[BCG])和微量分枝杆菌。越来越多的公认的MtbC分组包括牛分枝杆菌亚种。卡普拉和“结核分枝杆菌亚种。卡内蒂。”先前的调查已记录每个MtbC亚种为动物和/或人类结核病的来源。但是,由于缺乏能够快速,轻松地区分所有MtbC分组的单一方案,因此对这些生物的研究受到了阻碍。为此,我们开发了一种快速,简单且可靠的基于PCR的MtbC分型方法,该方法利用了MtbC染色体差异区缺失位点。在这里,七个引物对(在基因座16S rRNA,Rv0577,IS1561',Rv1510,Rv1970,Rv3877 / 8和Rv3120内扩增)在单独但同时的反应中运行。每个引物对要么特异性扩增独特大小的DNA片段,要么失败,这取决于分枝杆菌DNA的来源。琼脂糖凝胶电泳显示所有反应扩增产物的模式,可以立即鉴定为结核分枝杆菌(或非洲支原体亚型II),非洲支原体亚型I,牛分枝杆菌,牛分枝杆菌组成的MtbC。卡介苗,卡普拉分枝杆菌,微量分枝杆菌或“ M. canettii”或作为MtbC(MOTT)以外的分枝杆菌。该MtbC PCR分型小组提供了一种先进的方法来确定MtbC分离株的亚种,并将其与临床上重要的MOTT物种区分开。它已被证明对分枝杆菌收集的管理有益,并可用于实际的临床和流行病学用途。

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