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Multiple-Locus Variable-Number Tandem Repeat Analysis Reveals Genetic Relationships within Bacillus anthracis

机译:多位点可变数串联重复分析揭示了炭疽杆菌内的遗传关系。

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摘要

Bacillus anthracis is one of the most genetically homogeneous pathogens described, making strain discrimination particularly difficult. In this paper, we present a novel molecular typing system based on rapidly evolving variable-number tandem repeat (VNTR) loci. Multiple-locus VNTR analysis (MLVA) uses the combined power of multiple alleles at several marker loci. In our system, fluorescently labeled PCR primers are used to produce PCR amplification products from eight VNTR regions in the B. anthracis genome. These are detected and their sizes are determined using an ABI377 automated DNA sequencer. Five of these eight loci were discovered by sequence characterization of molecular markers (vrrC1, vrrC2, vrrB1, vrrB2, and CG3), two were discovered by searching complete plasmid nucleotide sequences (pXO1-aat and pXO2-at), and one was known previously (vrrA). MLVA characterization of 426 B. anthracis isolates identified 89 distinct genotypes. VNTR markers frequently identified multiple alleles (from two to nine), with Nei's diversity values between 0.3 and 0.8. Unweighted pair-group method arithmetic average cluster analysis identified six genetically distinct groups that appear to be derived from clones. Some of these clones show worldwide distribution, while others are restricted to particular geographic regions. Human commerce doubtlessly has contributed to the dispersal of particular clones in ancient and modern times.
机译:炭疽芽胞杆菌是描述的遗传上最均一的病原体之一,因此菌株识别特别困难。在本文中,我们提出了一种基于快速发展的可变数目串联重复序列(VNTR)基因座的新型分子分型系统。多基因座VNTR分析(MLVA)在几个标记位点使用多个等位基因的综合能力。在我们的系统中,使用荧光标记的PCR引物从炭疽芽孢杆菌基因组的八个VNTR区产生PCR扩增产物。使用ABI377自动DNA测序仪检测它们并确定其大小。通过分子标记(vrrC1,vrrC2,vrrB1,vrrB2和CG3)的序列表征发现了这八个基因座中的五个,通过搜索完整的质粒核苷酸序列(pXO1-aat和pXO2-at)发现了两个,而先前已知的一个(vrrA)。 426个炭疽芽孢杆菌分离株的MLVA表征鉴定出89种不同的基因型。 VNTR标记经常鉴定出多个等位基因(从2个到9个),Nei的多样性值在0.3和0.8之间。非加权成对组方法算术平均聚类分析确定了六个遗传上不同的组,这些组似乎来自克隆。这些克隆中有一些显示出全球分布,而另一些则局限于特定的地理区域。毫无疑问,人类贸易促成了古代和现代特定克隆的传播。

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