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首页> 外文期刊>Veterinary Microbiology >Evaluation of PMS-PCR technology for detection of Mycobacterium avium subsp. paratuberculosis directly from bovine fecal specimens.
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Evaluation of PMS-PCR technology for detection of Mycobacterium avium subsp. paratuberculosis directly from bovine fecal specimens.

机译:评价PMS-PCR技术检测鸟分枝杆菌亚种。副结核病直接来自牛粪标本。

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Mycobacterium avium subsp. paratuberculosis (MAP) causes paratuberculosis, or Johne's disease, in animals. Diagnosis of MAP infection is challenging because of the pathogen's fastidious in vitro growth requirements and low-level intermittent shedding in feces during the preclinical phase of the infection. Detection of these "low-shedders" is important for effective control of paratuberculosis as these animals serve as sources of infection for susceptible calves. Magnetic separation technology, used in combination with culture or molecular methods for the isolation and detection of pathogenic bacteria, enhances the analytical sensitivity and specificity of detection methods. The aim of the present study was to evaluate peptide-mediated magnetic separation (PMS) capture technology coupled with IS900 PCR using the Roche real-time PCR system (PMS-PCR), in comparison with fecal culture using BACTEC-MGIT 960 system, for detection of MAP in bovine fecal samples. Among the 351 fecal samples 74.9% (263/351) were PMS-PCR positive while only 12.3% (43/351) were MGIT culture-positive (p=0.0001). All 43 MGIT culture-positive samples were also positive by PMS-PCR. Mean PMS-PCR crossing-point (Cp) values for the 13 fecal samples with the highest number of MAP, based on time to detection, (26.3) were significantly lower than for the 17 fecal samples with <100 MAP per 2 g feces (30.06) (p<0.05). PMS-PCR technology provided results in a shorter time and yielded a higher number of positive results than MGIT culture. Earlier and faster detection of animals shedding MAP by PMS-PCR should significantly strengthen control efforts for MAP-infected cattle herds by helping to limit infection transmission at earlier stages of the infection.
机译:鸟分枝杆菌亚种副结核病(MAP)在动物中引起副结核病或约翰氏病。 MAP感染的诊断具有挑战性,因为病原体对体外生长的要求很高,并且在感染的临床前阶段粪便中水平低的间歇性脱落。这些“低流失者”的检测对于有效控制副结核病很重要,因为这些动物是易感小牛的感染源。磁分离技术与培养或分子方法结合使用,可分离和检测病原细菌,可提高分析方法的灵敏度和特异性。本研究的目的是评估与使用BACTEC-MGIT 960系统进行粪便培养相比,使用Roche实时PCR系统(PMS-PCR)结合IS900 PCR进行的肽介导磁分离(PMS)捕获技术,检测牛粪便样品中的MAP。在351个粪便样品中,PMS-PCR阳性率为74.9%(263/351),而MGIT培养阳性的仅为12.3%(43/351)(p = 0.0001)。通过PMS-PCR,所有43个MGIT培养阳性样品也均为阳性。基于检测时间,具有最高MAP数量的13个粪便样品的平均PMS-PCR交叉点(Cp)值(26.3)显着低于每2 g粪便中<100 MAP的17个粪便样品( 30.06)(p <0.05)。与MGIT培养相比,PMS-PCR技术可在更短的时间内提供结果,并产生更多的阳性结果。通过PMS-PCR更快,更快速地检测到动物体内流失MAP的动物,应通过限制感染早期阶段的感染传播,从而大大加强对MAP感染牛群的控制力度。

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