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首页> 外文期刊>Journal of Virological Methods >Development of a SYBR Green based real-time PCR assay for detection and quantitation of canine parvovirus in faecal samples.
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Development of a SYBR Green based real-time PCR assay for detection and quantitation of canine parvovirus in faecal samples.

机译:基于SYBR Green的实时PCR检测方法的开发,用于检测和定量粪便样品中的犬细小病毒。

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摘要

The present study describes the development of SYBR Green based real-time polymerase chain reaction (real-time PCR) for detection and quantitation of canine parvovirus type 2 (CPV 2) in faecal samples of dogs. In this assay, the primers were designed and custom-synthesized based on nucleotide sequence of VP2 gene of CPV 2. A standard curve was plotted using 10-fold serial dilution of standard plasmid DNA and Ct value. The standard curve was found to be linear over a 10-7 dilution. The real-time PCR results were expressed as the number of DNA copies of CPV 2 per mg of faecal samples and showed range of 1.0x103 to 7.0x109 copies of viral DNA per mg of stool samples. The analytical sensitivity of the SYBR Green based real-time PCR was shown to be equivalent to 10 copies. Faecal samples (47) from dogs suspected of CPV 2 infection were analyzed by real-time PCR, haemagglutination (HA) assay and by a conventional PCR and 24, 20 and 22 samples were found positive for CPV 2, respectively. Comparison between the results of three different assays revealed that real-time PCR is more sensitive than HA and conventional PCR and allow the detection of low titers of CPV 2 in infected dogs.
机译:本研究描述了基于SYBR Green的实时聚合酶链反应(实时PCR)的开发,用于检测和定量犬粪便样本中的2型犬细小病毒(CPV 2)。在该测定中,根据CPV 2 VP2基因的核苷酸序列设计引物并定制合成。使用标准质粒DNA的10倍系列稀释度和Ct值绘制标准曲线。发现标准曲线在10 -7 稀释下呈线性。实时PCR结果表示为每毫克粪便样品中CPV 2的DNA拷贝数,显示范围为1.0x10 3 至7.0x10 9 病毒每毫克粪便样本中的DNA。基于SYBR Green的实时PCR的分析灵敏度被证明相当于10个拷贝。通过实时PCR,血细胞凝集(HA)分析和常规PCR分析疑似CPV 2感染狗的粪便样本(47),分别发现24、20和22个样本对CPV 2呈阳性。三种不同检测方法的结果之间的比较表明,实时PCR比HA和常规PCR更为灵敏,可以检测到感染犬只中滴度较低的CPV 2。

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