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基于rpoB基因对非色素沉着及迟色素沉着快速生长分枝杆菌的鉴定

rpoB-based identification of nonpigmented and late-pigmenting rapidly growing mycobacteria.

作者信息

Adékambi Toïdi, Colson Philippe, Drancourt Michel

机构信息

Unité des Rickettsies, CNRS UMR 6020 IFR 48, Faculté de Médecine, Université de la Méditerranée, Marseille, France.

出版信息

J Clin Microbiol. 2003 Dec;41(12):5699-708. doi: 10.1128/JCM.41.12.5699-5708.2003.

Abstract

Nonpigmented and late-pigmenting rapidly growing mycobacteria (RGM) are increasingly isolated in clinical microbiology laboratories. Their accurate identification remains problematic because classification is labor intensive work and because new taxa are not often incorporated into classification databases. Also, 16S rRNA gene sequence analysis underestimates RGM diversity and does not distinguish between all taxa. We determined the complete nucleotide sequence of the rpoB gene, which encodes the bacterial beta subunit of the RNA polymerase, for 20 RGM type strains. After using in-house software which analyzes and graphically represents variability stretches of 60 bp along the nucleotide sequence, our analysis focused on a 723-bp variable region exhibiting 83.9 to 97% interspecies similarity and 0 to 1.7% intraspecific divergence. Primer pair Myco-F-Myco-R was designed as a tool for both PCR amplification and sequencing of this region for molecular identification of RGM. This tool was used for identification of 63 RGM clinical isolates previously identified at the species level on the basis of phenotypic characteristics and by 16S rRNA gene sequence analysis. Of 63 clinical isolates, 59 (94%) exhibited <2% partial rpoB gene sequence divergence from 1 of 20 species under study and were regarded as correctly identified at the species level. Mycobacterium abscessus and Mycobacterium mucogenicum isolates were clearly distinguished from Mycobacterium chelonae; Mycobacterium mageritense isolates were clearly distinguished from "Mycobacterium houstonense." Four isolates were not identified at the species level because they exhibited >3% partial rpoB gene sequence divergence from the corresponding type strain; they belonged to three taxa related to M. mucogenicum, Mycobacterium smegmatis, and Mycobacterium porcinum. For M. abscessus and M. mucogenicum, this partial sequence yielded a high genetic heterogeneity within the clinical isolates. We conclude that molecular identification by analysis of the 723-bp rpoB sequence is a rapid and accurate tool for identification of RGM.

摘要

非色素沉着和迟色素沉着的快速生长分枝杆菌(RGM)在临床微生物实验室中越来越多地被分离出来。它们的准确鉴定仍然存在问题,因为分类是一项劳动密集型工作,而且新的分类单元并不经常被纳入分类数据库。此外,16S rRNA基因序列分析低估了RGM的多样性,并且不能区分所有的分类单元。我们测定了20株RGM标准菌株的rpoB基因的完整核苷酸序列,该基因编码RNA聚合酶的细菌β亚基。在使用内部软件分析并以图形方式展示沿核苷酸序列的60 bp可变区段后,我们的分析集中在一个723 bp的可变区域,该区域种间相似性为83.9%至97%,种内差异为0至1.7%。引物对Myco-F-Myco-R被设计为用于该区域PCR扩增和测序的工具,以对RGM进行分子鉴定。该工具用于鉴定63株RGM临床分离株,这些分离株先前已根据表型特征和16S rRNA基因序列分析在种水平上进行了鉴定。在63株临床分离株中,59株(94%)与所研究的20个种中的1个种的rpoB基因部分序列差异<2%,并被认为在种水平上鉴定正确。脓肿分枝杆菌和产黏液分枝杆菌分离株与龟分枝杆菌明显区分开;马格里特分枝杆菌分离株与“休斯顿分枝杆菌”明显区分开。4株分离株未在种水平上鉴定出来,因为它们与相应标准菌株的rpoB基因部分序列差异>3%;它们属于与产黏液分枝杆菌、耻垢分枝杆菌和猪分枝杆菌相关的三个分类单元。对于脓肿分枝杆菌和产黏液分枝杆菌,该部分序列在临床分离株中显示出高度的遗传异质性。我们得出结论,通过分析723 bp的rpoB序列进行分子鉴定是一种快速准确的RGM鉴定工具。

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