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Development of fluorogenic probe-based PCR assays for the detection and quantification of bovine piroplasmids.

机译:基于荧光探针的PCR检测方法的开发,用于检测和定量牛螺胞质。

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摘要

This paper reports two new quantitative PCR (qPCR) assays, developed in an attempt to improve the detection of bovine piroplasmids. The first of these techniques is a duplex TaqMan assay for the simultaneous diagnosis of Babesia bovis and B. bigemina. This technique is ideal for use in South America where bovids harbour no theilerids. The second technique, which is suitable for the diagnosis of both babesiosis and theileriosis worldwide, involves fluorescence resonance energy transfer (FRET) probes. In FRET assays, Babesia bovis, B. divergens, Babesia sp. (B. major or B. bigemina), Theileria annae and Theileria sp. were all identifiable based on the melting temperatures of their amplified fragments. Both techniques provided linear calibration curves over the 0.1fg/microl to 0.01ng/microl DNA range. The assays showed good sensitivity and specificity. To assess their performance, both procedures were compared in two separate studies: the first was intended to monitor the experimental infection of calves with B. bovis and the second was a survey where 200 bovid/equine DNA samples from different countries were screened for piroplasmids. Comparative studies showed that duplex TaqMan qPCR was more sensitive than FRET qPCR in the detection of babesids.
机译:本文报告了两种新的定量PCR(qPCR)分析方法,旨在提高对牛螺旋体的检测。这些技术中的第一个是用于同时诊断牛肝杆菌和双歧杆菌的双重TaqMan测定法。这项技术非常适合在玻利维亚没有Theilerids的南美使用。第二种技术适用于全世界范围内的贝氏杆菌病和回虫病的诊断,它涉及荧光共振能量转移(FRET)探针。在FRET分析中,牛肝杆菌,B。divergens,巴贝斯虫sp.。 (B. major或B. bigemina),Theileria annae和Theileria sp。可以根据扩增片段的解链温度进行鉴定。两种技术均提供了在0.1fg /μl至0.01ng /μlDNA范围内的线性校准曲线。该测定显示出良好的敏感性和特异性。为了评估其性能,在两个单独的研究中对这两种方法进行了比较:第一个旨在监测牛双歧杆菌对小牛的实验感染,第二个是对来自不同国家的200个牛/马DNA样品进行筛查的调查。比较研究表明,双链TaqMan qPCR在检测婴儿方面比FRET qPCR更为灵敏。

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