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首页> 外文期刊>Journal of Virological Methods >Improved detection of bovine coronavirus N gene in faeces of calves infected naturally by a semi-nested PCR assay and an internal control.
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Improved detection of bovine coronavirus N gene in faeces of calves infected naturally by a semi-nested PCR assay and an internal control.

机译:通过半巢式PCR测定法和内部对照,可以更好地检测自然感染的小牛粪便中的牛冠状病毒N基因。

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摘要

Bovine coronavirus (BCoV), a positive sense single-stranded RNA virus, is an important causative agent of neonatal diarrhoea in calves from beef and dairy cattle worldwide. The routine detection and diagnosis of BCoV have been mainly dependent on assays with low sensitivity. The aim of the present study was to develop and evaluate a semi-nested PCR (SN-PCR) to amplify a 251bp fragment of BCoV N gene from fresh (n=25) and frozen (n=25) diarrhoeic faecal samples of naturally infected calves. To improve detection of BCoV in faecal samples by the SN-PCR an internal control was developed, and the results were compared with a conventional RT-PCR assay. The rates of positive samples by SN-PCR and RT-PCR were 24% (12/50) and 8% (4/50), respectively (K=0.43). Only fresh samples were positive in RT-PCR while the SN-PCR detected BCoV in both fresh and frozen faecal samples. The sensitivity of SN-PCR was determined by 10-fold serial dilutions of the BCoV Kakegawa strain (HA titre: 256) that was detected until 10(-7) dilution. The specificity of the amplicons was assessed by restriction fragment length polymorphism and sequence analysis. The inclusion of an internal control provides a way to detect assay inhibition in faecal samples and failure of nucleic acid extraction that allow reduction of the number of false-negative results.
机译:牛冠状病毒(BCoV)是一种正向单链RNA病毒,是全球范围内来自牛肉和奶牛犊牛腹泻的重要病原体。 BCoV的常规检测和诊断主要取决于灵敏度低的检测方法。本研究的目的是开发和评估半嵌套式PCR(SN-PCR),以从自然感染的新鲜(n = 25)和冷冻(n = 25)腹泻粪便样本中扩增251bp的BCoV N基因片段小牛。为了通过SN-PCR改善粪便样品中BCoV的检测,开发了内部对照,并将结果与​​常规RT-PCR分析进行了比较。 SN-PCR和RT-PCR阳性样品的比率分别为24%(12/50)和8%(4/50)(K = 0.43)。 RT-PCR中仅新鲜样品呈阳性,而SN-PCR在新鲜和冷冻粪便样品中均检测到BCoV。 SN-PCR的灵敏度由BCoV挂川株的10倍系列稀释液(HA滴度:256)确定,直到10(-7)稀释液才被检测到。通过限制性片段长度多态性和序列分析来评估扩增子的特异性。内部对照的加入提供了一种检测粪便样品中测定抑制和核酸提取失败的方法,从而减少了假阴性结果的数量。

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