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Direct detection of Mycobacterium avium subsp. Paratuberculosis in bovine milk by multiplex Real-time PCR

机译:直接检测鸟分枝杆菌亚种。多重实时荧光定量PCR检测牛乳中的副结核病

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The study aimed at direct detection of Mycobacterium avium subsp. Paratuberculosis (MAP) in milk by evaluating a multiplex real-time PCR assay targeting IS900 and ISMAV2 sequences including the amplification of PUC19-plasmid as internal control. The sensitivity of the assays was evaluated by testing MAP isolates in broad linear range of DNA (50 ng ¨C 5 fg/|ìl). For the validation of the specificity, 6 MAP isolates and 22 isolates of genus Mycobacteriaceae were tested. Results revealed that reproducible detection limit for real-time PCR targeting IS900 and ISMAV2 was 5 fg/|ìl and 50 fg/|ìl respectively. By targeting ISMAV2 sequence, 100% specificity was detected. However, a cross reaction with 5 ng/|ìl of genome of 3 M. avian subspecies avium strains was detected by targeting IS900 and negative in lower genome quantity (5pg/|ìl). To maximize the assay's detection sensitivity, an efficient strategy for MAP-DNA extraction from spiked milk was assessed. Targeting of IS900 was sensitive and targeting ISMAV2 was very specific. Therefore, a multiplex real-time PCR assay targeting IS900 and ISMAV2 in combination with two commercial DNA extraction kits could be an ideal sensitive and specific protocol for routine large-scale analysis of milk samples and other clinical specimens from man and animals
机译:该研究旨在直接检测鸟分枝杆菌亚种。通过评估针对IS900和ISMAV2序列的多重实时PCR分析(包括PUC19质粒的扩增作为内部对照),评估牛奶中的副结核病(MAP)。通过在宽线性范围内的DNA(50 ng-C 5 fg / | l)中测试MAP分离物来评估测定的敏感性。为了验证特异性,测试了6种MAP分离株和22种分枝杆菌科。结果表明,针对IS900和ISMAV2的实时PCR的可重复检测极限分别为5 fg / | l和50 fg / | l。通过靶向ISMAV2序列,检测到100%的特异性。但是,通过靶向IS900并检测到较低的基因组数量(5pg / | l),检测到了与3 ng禽亚种禽种菌株的5 ng / | l基因组的交叉反应。为了最大化测定的检测灵敏度,评估了从加标牛奶中提取MAP-DNA的有效策略。对IS900的定向很敏感,而对ISMAV2的定向则非常具体。因此,针对IS900和ISMAV2的多重实时PCR检测结合两个商业DNA提取试剂盒可能是常规,大规模常规分析人和动物奶样和其他临床标本的理想灵敏且特异的方案

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