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临床标本和医院供水设施中的军团菌:分离株的分子检测与基因分型

Legionella in clinical specimens and hospital water supply facilities: molecular detection and genotyping of the isolates.

作者信息

Qasem J A, Mustafa A S, Khan Z U

机构信息

Department of Applied Medical Sciences, College of Health Sciences, The Public Authority for Applied Education and Training, Kuwait University, Kuwait.

出版信息

Med Princ Pract. 2008;17(1):49-55. doi: 10.1159/000109590.

Abstract

OBJECTIVE

To evaluate genus- and species-specific polymerase chain reactions (PCRs) for the detection of the genus Legionella and the species Legionella pneumophila in clinical specimens and hospital water supplies, and to establish a simple and reproducible random amplification of polymorphic DNA (RAPD)-PCR technique for genotyping of Legionella.

MATERIALS AND METHODS

A total of 70 respiratory tract specimens(bronchoalveolar lavage: n = 46; endotracheal secretions: n = 9; sputum: n = 15) from patients with atypical pneumonia, and 283 environmental samples (water: 20; swabs: 263) collected from water storage and supply facilities of the Mubarak Al-Kabeer Hospital, Kuwait, were tested by culture and genus-specific PCR for the detection of Legionella. The L. pneumophila isolates were subsequently typed by serology and RAPD-PCR using serotype-specific sera and arbitrary primers, respectively.

RESULTS

Of the 70 clinical samples, culture yielded 2 (2.9%) whereas genus-specific PCR detected Legionella in 20 (28.6%) samples. The 2 culture-positive specimens were also positive for L.-pneumophila-specific PCR. Testing of swab and water samples by culture and genus-specific PCR yielded 61 (21.6%) and 67 (23.7%) positive samples, respectively. All of the 61 culture-positive samples were also positive by genus-specific PCR and 45 of them were positive for L.-pneumophila-specific PCR. Serological typing of 43 L. pneumophila isolates showed that 8 of these belonged to serotype 1 and 35 to serotype 3; however, RAPD-PCR analyses demonstrated polymorphisms among the isolates of both serotypes.

CONCLUSION

A higher association between PCR and culture was observed for the environmental samples than for the clinical samples. The application of genus- and species-specific PCRs and RAPD is useful in the detection and typing of Legionella in clinical and environmental samples.

摘要

目的

评估属特异性和种特异性聚合酶链反应(PCR)用于检测临床标本和医院供水系统中嗜肺军团菌属及嗜肺军团菌的效果,并建立一种简单且可重复的随机扩增多态性DNA(RAPD)-PCR技术用于嗜肺军团菌的基因分型。

材料与方法

对科威特穆巴拉克·卡比尔医院的70份非典型肺炎患者的呼吸道标本(支气管肺泡灌洗标本:n = 46;气管内分泌物:n = 9;痰液:n = 15)以及283份环境样本(水:20份;拭子:263份)进行培养和属特异性PCR检测,以检测嗜肺军团菌。随后,分别使用血清型特异性血清和随机引物通过血清学和RAPD-PCR对嗜肺军团菌分离株进行分型。

结果

在70份临床样本中,培养法检出2份(2.9%),而属特异性PCR在20份(28.6%)样本中检测到嗜肺军团菌。2份培养阳性标本的嗜肺军团菌特异性PCR也呈阳性。对拭子和水样进行培养和属特异性PCR检测,分别有61份(21.6%)和67份(23.7%)样本呈阳性。61份培养阳性样本的属特异性PCR均为阳性,其中45份嗜肺军团菌特异性PCR呈阳性。对43株嗜肺军团菌分离株进行血清学分型显示,其中8株属于血清型1,35株属于血清型3;然而,RAPD-PCR分析表明两种血清型的分离株之间存在多态性。

结论

与临床样本相比,环境样本中PCR与培养法之间的关联性更高。属特异性和种特异性PCR以及RAPD的应用有助于临床和环境样本中嗜肺军团菌的检测和分型。

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