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首页> 外文期刊>Journal of Clinical Microbiology >Comparison of Restriction Fragment Length Polymorphism with the Polymorphic Guanine-Cytosine-Rich Sequence and Spoligotyping for Differentiation of Mycobacterium tuberculosis Isolates with Five or Fewer Copies of IS6110
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Comparison of Restriction Fragment Length Polymorphism with the Polymorphic Guanine-Cytosine-Rich Sequence and Spoligotyping for Differentiation of Mycobacterium tuberculosis Isolates with Five or Fewer Copies of IS6110

机译:限制性片段长度多态性与多态鸟嘌呤-胞嘧啶-富集序列的比较和Spoligotyping区分IS6110的五个或更少副本的结核分枝杆菌分离株

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摘要

The use of IS6110 as a marker for molecular epidemiological studies is limited when a Mycobacterium tuberculosis isolate has five or fewer copies of IS6110. Restriction fragment length polymorphism analysis with a highly polymorphic GC-rich repetitive sequence located in the plasmid pTBN12 (PGRS RFLP) and spoligotyping (based on the polymorphism of the DR region) are two frequently used secondary typing methods. The aim of this study was to compare the performance of these two methods in a population-based study in San Francisco. We included all patients with culture-positive tuberculosis from 1999 to 2007 with IS6110 RFLP results presenting five or fewer bands. PGRS RFLP and spoligotyping were performed using standardized methods. We determined the concordance between the two methods regarding cluster status and the risk factors for an isolate to be in a cluster with each of the methods. Our data indicate that both methods had similar discriminatory power and that the risk factors associated with clustering by either method were the same. Although the cluster/unique status was concordant in 84% of the isolates, patients were clustered differently depending on the method. Therefore, the methods are not interchangeable, and the same method should be used for longitudinal studies.
机译:结核分枝杆菌分离物具有 IS6110 的五个或更少副本时,将IS 6110 用作分子流行病学研究的标记是有限的。使用位于质粒pTBN12(PGRS RFLP)中的高度多态性的富含GC的重复序列进行限制性片段长度多态性分析和spoligotyping(基于DR区的多态性)是两种常用的二级分型方法。这项研究的目的是在旧金山的一项基于人群的研究中比较这两种方法的效果。我们纳入了1999年至2007年的所有培养阳性结核病患者,IS 6110 RFLP结果显示了5条或更少的条带。 PGRS RFLP和基因分型使用标准方法进行。我们确定了关于群集状态的两种方法与每种方法在群集中的隔离株风险因素之间的一致性。我们的数据表明,这两种方法具有相似的区分能力,并且通过这两种方法进行聚类的风险因素都相同。尽管在84%的分离物中聚类/独特状态是一致的,但是根据方法的不同,患者的聚类也不同。因此,这些方法不可互换,纵向研究应使用相同的方法。

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