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普氏立克次体与实时聚合酶链反应

Rickettsia prowazekii and real-time polymerase chain reaction.

作者信息

Svraka Sanela, Rolain Jean-Marc, Bechah Yassina, Gatabazi John, Raoult Didier

机构信息

Université de la Méditerranée, Marseilles, France.

出版信息

Emerg Infect Dis. 2006 Mar;12(3):428-32. doi: 10.3201/eid1203.050888.

DOI:10.3201/eid1203.050888
PMID:16704780
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3291444/
Abstract

Rickettsia prowazekii is the causative agent of epidemic typhus and a potential bioterrorism agent. Sensitive and specific rapid assays are needed to complement existing methods of detecting this organism. We developed a real-time quantitative polymerase chain reaction assay by using a species-specific probe targeting the gltA gene. This assay, which was rapid, specific for R. prowazekii only, and sensitive (cutoff detection of 1 to 5 copies per sample), detected and directly identified R. prowazekii in blood of 12 experimentally infected mice sampled at day 3 and 6 postinfection or in naturally or experimentally infected lice. Because our assay is highly standardized and easily adaptable, it could improve epidemic typhus surveillance in public health programs, especially for countries with underdiagnosed or unrecognized human cases.

摘要

普氏立克次体是流行性斑疹伤寒的病原体以及一种潜在的生物恐怖主义制剂。需要灵敏且特异的快速检测方法来补充现有的检测这种微生物的方法。我们通过使用靶向gltA基因的种特异性探针开发了一种实时定量聚合酶链反应检测法。该检测法快速、仅对普氏立克次体特异且灵敏(每个样本的检测下限为1至5个拷贝),在感染后第3天和第6天采集的12只经实验感染小鼠的血液中,或在自然感染或经实验感染的虱子中检测并直接鉴定出了普氏立克次体。由于我们的检测法高度标准化且易于调整,它可改善公共卫生项目中的流行性斑疹伤寒监测,尤其是对于那些人类病例诊断不足或未被识别的国家。

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