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Detection of Five Avian Eimeria Species by Species-Specific Real-Time Polymerase Chain Reaction Assay

机译:通过物种特异性实时聚合酶链反应分析法检测五种禽艾美耳虫物种

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摘要

To detect five different avian Eimeria species, we applied the SYBR Green-based real-time polymerase chain reaction (PCR) assay for the diagnosis of field-isolated parasites by using their individual species-specific primer sets. The primer sets were originally designed for Eimeria acervulina, E. brunetti, E. necatrix, and E. tenella based on the sequence of the internal transcribed spacer 1 region of ribosomal DNA, whereas for E. maxima the primer sets were derived from sequences reported previously. The detection limit of these assays was defined at 10po or 10p# oocysts depending on species. Melting curves from the real-time PCR assay showed that each species has a single peak and specific melting temperature value. Fecal samples from 32 poultryfarms, which were endemic for coccidiosis, were examined using this assay. The data showed that E. brunetti was found in 21 farms, E. maxima and E. necatrix in 16 farms, E. tenella in 12 farms, and E. acervulina in eight farms. This survey revealed thatE. brunetti was highly prevalent in Japan. This technique is not only easy and rapid but also available to detect Eimeria species specifically; therefore, it can be a valuable tool for diagnostic work for chicken coccidiosis.
机译:为了检测五种不同的禽艾美耳球虫物种,我们应用了基于SYBR Green的实时聚合酶链反应(PCR)分析法,通过使用它们各自的物种特异性引物组来诊断田间分离的寄生虫。引物组最初是根据核糖体DNA的内部转录间隔区1区域的序列设计的,用于艾美尔球虫,布鲁内特大肠杆菌,necatrix和tenella大肠杆菌,而对于大肠埃希氏菌,引物组来自报道的序列先前。根据种类的不同,这些测定的检测限定义为10po或10p#卵囊。实时PCR分析的熔解曲线表明,每个物种都有一个峰和特定的熔解温度值。使用此测定法检查了32种禽球虫病流行的粪便样本。数据显示,在21个养殖场中发现了布鲁氏大肠杆菌,在16个养殖场中发现了大肠埃希菌和necatrix,在12个养殖场中发现了黄粉虫,在八个养殖场中发现了小球藻。这项调查显示E. brunetti在日本非常流行。该技术不仅简单,快速,而且可用于特异性地检测艾美尔球虫。因此,它可以成为诊断鸡球虫病的有价值的工具。

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