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A robust PCR for the differentiation of potential virulent strains of Haemophilus parasuis

机译:用于鉴别副猪嗜血杆菌潜在强毒株的可靠PCR

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Background Haemophilus parasuis is the etiological agent of Gl?sser’s disease in swine. H. parasuis comprises strains with heterogeneous virulence capacity, from non-virulent to highly virulent. Determination of the pathogenic potential of the strains is important for diagnosis and disease control. The virulence-associated trimeric autotransporters ( vtaA ) genes have been used to predict H. parasuis virulence by PCR amplification of their translocator domains. Here, we report a new and improved PCR designed to detect a different domain of the vtaA genes, the leader sequence (LS) as a diagnostic tool to predict virulence. Methods A collection of 360 ? H. parasuis ?strains was tested by PCR with LS specific primers. Results of the PCR were compared with the clinical origin of the strains and, for a subset of strains, with their phagocytosis and serum resistance using a Chi-square test. Results LS-PCR was specific to H. parasuis , and allowed the differential detection of the leader sequences found in clinical and non-clinical isolates. Significant correlation was observed between the results of the LS-PCR and the clinical origin (organ of isolation) of the strains, as well as with their phagocytosis and serum susceptibility, indicating that this PCR is a good predictor of the virulence of the strains. In addition, this new PCR showed a full correlation with the previously validated PCR based on the translocator domain. LS-PCR could be performed in a wide range of annealing temperatures without losing specificity. Conclusion This newly described PCR based on the leader sequence of the vtaA genes, LS-PCR, is a robust test for the prediction of the virulence potential of H. parasuis strains.
机译:背景副猪嗜血杆菌是猪Gl?sser病的病原体。副猪嗜血杆菌包括从非毒力到高毒力具有不同毒力的菌株。确定菌株的致病潜力对诊断和疾病控制很重要。与毒力相关的三聚体自转运蛋白(vtaA)基因已被用于通过PCR对其易位域的PCR扩增来预测副猪嗜血杆菌的毒力。在这里,我们报告了一种新的和经过改进的PCR,旨在检测vtaA基因的不同域,即前导序列(LS)作为预测毒力的诊断工具。方法收集360?用LS特异性引物通过PCR检测副猪嗜血杆菌。使用卡方检验,将PCR结果与菌株的临床来源以及部分菌株的吞噬作用和血清抗性进行比较。结果LS-PCR特异于副猪嗜血杆菌,可以鉴别检测临床分离株和非临床分离株中的前导序列。 LS-PCR的结果与菌株的临床起源(分离器官)及其吞噬作用和血清敏感性之间存在显着相关性,表明该PCR可以很好地预测菌株的毒力。此外,这种新的PCR与基于转运蛋白域的先前验证的PCR显示出完全的相关性。 LS-PCR可以在宽范围的退火温度下进行而不会失去特异性。结论基于vtaA基因前导序列的新描述的LS-PCR是对副猪嗜血杆菌菌株毒力潜力进行预测的有力测试。

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