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Comparative sequence analysis of the capsular polysaccharide loci of Actinobacillus pleuropneumoniae serovars 1-18, and development of two multiplex PCRs for comprehensive capsule typing

机译:Actinobacillus胸膜炎血清素塞洛瓦塞洛拉血清素塞洛瓦1-18的比较序列分析,以及两种多重PCR综合胶囊键入的开发

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摘要

Problems with serological cross-reactivity have led to development of a number of PCRs (individual and multiplex) for molecular typing of Actinobacillus pleuropneumoniae, the causative agent of porcine pleuropneumonia. Most of these assays were developed for detection of specific amplicons within capsule biosynthetic genes before the availability of complete sequences for the different serovars. Here we describe comparative analysis of the complete capsular loci for all 18 serovars of A. pleuropneumoniae, and development of two multiplex PCRs for comprehensive capsule typing of this important pig pathogen.
机译:血清学交叉反应性的问题导致了许多PCRS(个体和多重)的分子打字,用于分子胸腺嘧啶,猪胸膜炎的致病剂。 这些测定中的大多数用于检测胶囊生物合成基因内的特异性扩增子,在不同血清素的完整序列的可用性之前。 在这里,我们描述了A.Pleuropneumoniae的所有18个Serovars的完整荚膜基因座的对比分析,以及用于综合猪病原体的综合胶囊键入的两种多重PCR的开发。

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