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Flotation—A New Method to Circumvent PCR Inhibitors in the Diagnosis of Lawsonia intracellularis

机译:浮选—一种规避PCR抑制剂诊断胞内劳森氏菌的新方法

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摘要

The obligate intracellular bacterium Lawsonia intracellularis causes enteritis and poor growth in weaned pigs. Cultivation is difficult and diagnosis ante mortem is mainly based on techniques such as polymerase chain reaction. However, false negative results caused by the presence of PCR-inhibitory factors constitute a problem. This study aimed to develop and evaluate a new technique, flotation, to separate L. intracellularis from inhibitors in faeces prior to PCR. The technique was evaluated by comparison to two previously evaluated and commonly used methods, preparation by boiling lysate combined with nested PCR and preparation by a commercial kit combined with conventional PCR. Continuous density centrifugation of faecal samples containing L. intracellularis suggested the buoyant density of the microbe to be between 1.064 and 1.077 g/mL. Several flotation setups were tested to achieve optimal separation of the microbe from inhibitors and faecal particles. The finally selected setup floated whole L. intracellularis from the application site at the bottom to the upper part of the gradient while inhibitory components mainly remained in the bottom. PCR was performed directly on material recovered from the upper interphase. The method was evaluated on 116 clinical samples. As compared to sample preparation by boiling combined with nested PCR, fewer samples were inhibited but also fewer positives were identified. In comparison to preparation by a commercial kit combined with conventional PCR, presently used for routine diagnosis, similar results were obtained. However, the new method was comparably faster to perform. The new method, based on flotation of Lawsonia intracellularis combined with conventional PCR, was well suited for routine diagnosis.
机译:专一的细胞内细菌胞内劳森氏菌会引起断奶猪的肠炎和生长不良。耕种困难,并且事前诊断主要基于聚合酶链反应等技术。然而,由PCR抑制因子的存在引起的假阴性结果构成问题。这项研究旨在开发和评估一种新技术,即浮选,以在PCR前从粪便中的抑制剂中分离出胞内劳森氏菌。通过与两种先前评估和常用的方法进行比较来评估该技术,一种方法是将煮沸的裂解物与巢式PCR相结合,另一种是通过商业试剂盒与常规PCR相结合来制备。含有细胞内劳森氏菌的粪便样品的连续密度离心表明,微生物的浮力密度在1.064至1.077 g / mL之间。测试了几种浮选装置,以实现微生物与抑制剂和粪便颗粒的最佳分离。最终选择的设置将整个胞内劳氏菌从施用部位的底部漂浮到梯度的上部,而抑制成分则主要保留在底部。直接对从上层中间相回收的物质进行PCR。该方法在116个临床样品上进行了评估。与通过沸腾结合嵌套式PCR制备样品相比,抑制的样品更少,但鉴定出的阳性也更少。与目前用于常规诊断的商业试剂盒结合常规PCR的制备相比,获得了相似的结果。但是,新方法执行起来相对较快。基于细胞内劳森菌浮选结合常规PCR的新方法非常适合常规诊断。

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