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用于军团菌属鉴定的基因间rRNA基因序列长度多态性分析的评估

An evaluation of intergenic rRNA gene sequence length polymorphism analysis for the identification of Legionella species.

作者信息

Fry N K, Harrison T G

机构信息

Respiratory and Systemic Infection Laboratory, PHLS Central Public Health Laboratory, London.

出版信息

J Med Microbiol. 1998 Aug;47(8):667-78. doi: 10.1099/00222615-47-8-667.

Abstract

There are currently more than 40 species of Legionella and the identification of most of these by standard methods is technically difficult. The aim of this study was to assess the suitability of a previously published PCR-based method of identifying Legionella spp. Intergenic 16S-23S rDNA spacer regions were amplified with primers complementary to conserved regions of the rRNA genes. Following electrophoretic separation of the products, data analyses were performed with the Taxotron software package. Computer-assisted analysis (with an empirically derived error tolerance of 3%) could differentiate only 26 of the 43 strains (representing 43 species), with the remaining 17 species clustering into four groups (group I, comprising 10 species; group II, three species; group III, two species and group IV, two species). Analysis of well-characterised 'non-type' strains of some Legionella spp. (e.g., from type culture collections) resulted in patterns distinct from the corresponding type strain in most cases. Furthermore, recent isolates (identified by conventional methods) were identified by this PCR method to the presumed correct species (or species group) in only a minority of cases. Well characterised strains and recent isolates of Legionella showed heterogeneity within many species. This intra-species variation severely limits the usefulness of the method for the identification of isolates. However, this property may be useful for epidemiological typing within such species.

摘要

目前已知嗜肺军团菌有40多个种,采用标准方法对其中大多数种进行鉴定在技术上存在困难。本研究的目的是评估一种先前发表的基于聚合酶链反应(PCR)的嗜肺军团菌鉴定方法的适用性。用与rRNA基因保守区互补的引物扩增基因间16S - 23S rDNA间隔区。产物经电泳分离后,用Taxotron软件包进行数据分析。计算机辅助分析(经验性误差容限为3%)仅能区分43个菌株(代表43个种)中的26个,其余17个种聚为四组(第一组,包含10个种;第二组,3个种;第三组,2个种;第四组,2个种)。对一些嗜肺军团菌种的特征明确的“非模式”菌株(如来自模式培养物保藏中心)进行分析,在大多数情况下得到的图谱与相应模式菌株不同。此外,用这种PCR方法对近期分离株(用传统方法鉴定)进行鉴定时,只有少数情况下能鉴定到假定正确的种(或种组)。特征明确的嗜肺军团菌菌株和近期分离株在许多种内表现出异质性。这种种内变异严重限制了该方法在分离株鉴定中的实用性。然而,这种特性可能在这些种的流行病学分型中有用。

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