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用于粪便样本中禽分枝杆菌副结核亚种快速检测和特异性鉴定的三重实时荧光定量PCR的开发与验证

Development and validation of a triplex real-time PCR for rapid detection and specific identification of M. avium sub sp. paratuberculosis in faecal samples.

作者信息

Irenge Léonid M, Walravens Karl, Govaerts Marc, Godfroid Jacques, Rosseels Valérie, Huygen Kris, Gala Jean-Luc

机构信息

Defence Laboratories Department, Belgian Armed Forces, Brussels, Belgium.

出版信息

Vet Microbiol. 2009 Apr 14;136(1-2):166-72. doi: 10.1016/j.vetmic.2008.09.087. Epub 2008 Oct 21.

DOI:10.1016/j.vetmic.2008.09.087
PMID:19095382
Abstract

A triplex real-time (TRT-PCR) assay was developed to ensure a rapid and reliable detection of Mycobacterium avium subsp. paratuberculosis (Map) in faecal samples and to allow routine detection of Map in farmed livestock and wildlife species. The TRT-PCR assay was designed using IS900, ISMAP02 and f57 molecular targets. Specificity of TRT-PCR was first confirmed on a panel of control mycobacterial Map and non-Map strains and on faecal samples from Map-negative cows (n=35) and from Map-positive cows (n=20). The TRT-PCR assay was compared to direct examination after Ziehl-Neelsen (ZN) staining and to culture on 197 faecal samples collected serially from five calves experimentally exposed to Map over a 3-year period during the sub-clinical phase of the disease. The data showed a good agreement between culture and TRT-PCR (kappa score=0.63), with the TRT-PCR limit of detection of 2.5 x 10(2)microorganisms/g of faeces spiked with Map. ZN agreement with TRT-PCR was not good (kappa=0.02). Sequence analysis of IS900 amplicons from three single IS900 positive samples confirmed the true Map positivity of the samples. Highly specific IS900 amplification suggests therefore that each single IS900 positive sample from experimentally exposed animals was a true Map-positive specimen. In this controlled experimental setting, the TRT-PCT was rapid, specific and displayed a very high sensitivity for Map detection in faecal samples compared to conventional methods.

摘要

开发了一种三重实时(TRT-PCR)检测方法,以确保快速、可靠地检测粪便样本中的副结核分枝杆菌(Map),并实现对养殖家畜和野生动物物种中Map的常规检测。TRT-PCR检测方法是利用IS900、ISMAP02和f57分子靶点设计的。首先在一组对照分枝杆菌Map和非Map菌株以及来自Map阴性奶牛(n = 35)和Map阳性奶牛(n = 20)的粪便样本上确认了TRT-PCR的特异性。将TRT-PCR检测方法与齐尔-尼尔森(ZN)染色后的直接检查以及对从5头在疾病亚临床阶段经3年实验性暴露于Map的小牛连续采集的197份粪便样本进行培养的结果进行了比较。数据显示培养结果与TRT-PCR之间具有良好的一致性(kappa评分= 0.63),TRT-PCR对添加了Map的粪便的检测限为2.5 x 10(2)个微生物/克。ZN与TRT-PCR的一致性不佳(kappa = 0.02)。对三个单一IS900阳性样本的IS900扩增子进行序列分析,证实了样本中Map的真正阳性。因此,高度特异性的IS900扩增表明,来自实验性暴露动物的每个单一IS900阳性样本都是真正的Map阳性标本。在这种受控的实验环境中,与传统方法相比,TRT-PCT快速、特异,并且在粪便样本中对Map检测显示出非常高的灵敏度。

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