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幽门螺杆菌空泡毒素A等位基因多样性的扩展

Expanding allelic diversity of Helicobacter pylori vacA.

作者信息

van Doorn L J, Figueiredo C, Sanna R, Pena S, Midolo P, Ng E K, Atherton J C, Blaser M J, Quint W G

机构信息

Delft Diagnostic Laboratory, 2625 AD Delft, The Netherlands.

出版信息

J Clin Microbiol. 1998 Sep;36(9):2597-603. doi: 10.1128/JCM.36.9.2597-2603.1998.

DOI:10.1128/JCM.36.9.2597-2603.1998
PMID:9705399
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC105169/
Abstract

The diversity of the gene encoding the vacuolating cytotoxin (vacA) of Helicobacter pylori was analyzed in 98 isolates obtained from different geographic locations. The studies focused on variation in the previously defined s and m regions of vacA, as determined by PCR and direct sequencing. Phylogenetic analysis revealed the existence of four distinct types of s-region alleles: aside from the previously described s1a, s1b, and s2 allelic types, a novel subtype, designated s1c, was found. Subtype s1c was observed exclusively in isolates from East Asia and appears to be the major s1 allele in that part of the world. Three different allelic forms (m1, m2a, and m2b) were detected in the m region. On the basis of sequence alignments, universal PCR primers that allow effective amplification of the s and m regions from H. pylori isolates from all over the world were defined. Amplimers were subsequently analyzed by reverse hybridization onto a line probe assay (LiPA) that allows the simultaneous and highly specific hybridization of the different vacA s- and m-region alleles and tests for the presence of the cytotoxin-associated gene (cagA). This PCR-LiPA method permits rapid analysis of the vacA and cagA status of H. pylori strains for clinical and epidemiological studies and will facilitate identification of any further variations.

摘要

对从不同地理位置分离出的98株幽门螺杆菌编码空泡毒素(vacA)的基因多样性进行了分析。研究重点是通过聚合酶链反应(PCR)和直接测序确定的vacA基因先前定义的s区和m区的变异情况。系统发育分析揭示了s区等位基因存在四种不同类型:除了先前描述的s1a、s1b和s2等位基因类型外,还发现了一种新的亚型,命名为s1c。s1c亚型仅在东亚分离株中观察到,似乎是该地区的主要s1等位基因。在m区检测到三种不同的等位基因形式(m1、m2a和m2b)。基于序列比对,定义了通用PCR引物,可有效扩增来自世界各地幽门螺杆菌分离株的s区和m区。随后通过反向杂交在线性探针分析(LiPA)上分析扩增产物,该分析可实现不同vacA s区和m区等位基因的同时且高度特异性杂交,并检测细胞毒素相关基因(cagA)的存在。这种PCR-LiPA方法可快速分析幽门螺杆菌菌株的vacA和cagA状态,用于临床和流行病学研究,并将有助于识别任何进一步的变异。

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