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检测到具有非编码突变的犬细小病毒 2c 及其对分子特征的影响。

Detection of a canine parvovirus type 2c with a non-coding mutation and its implications for molecular characterisation.

机构信息

Department of Veterinary Medicine, University of Bari, Valenzano, Bari, Italy.

出版信息

Vet J. 2013 Jun;196(3):555-7. doi: 10.1016/j.tvjl.2012.12.017. Epub 2013 Feb 1.

DOI:10.1016/j.tvjl.2012.12.017
PMID:23375346
Abstract

An epidemiological survey for canine parvovirus (CPV) was conducted by collecting 615 faecal samples from dogs with diarrhoea in different European countries. Molecular methods showed that CPV-2a was predominant in most countries, followed by CPV-2c and CPV-2b, whereas 30 strains were not characterised. By sequence analysis of the full-length VP2 gene, 20 of these viruses were characterised as CPV-2c mutants having the synonymous mutation A4061G in the probe-binding region that prevented correct strain characterisation. A real-time polymerase chain reaction (PCR) assay using a minor groove binder probe was able to recognise both mutant and classical CPV-2c strains. These results indicate that the emergence of CPVs with mutations affecting the oligonucleotide-binding region needs a continuous update of molecular diagnostic tools in order to detect efficiently those emerging strains.

摘要

采用收集来自不同欧洲国家患有腹泻的犬只的 615 份粪便样本的方法,对犬细小病毒(CPV)进行了一项流行病学调查。分子方法显示,CPV-2a 在大多数国家占主导地位,其次是 CPV-2c 和 CPV-2b,而有 30 株未被鉴定。通过全长 VP2 基因的序列分析,其中 20 株病毒被鉴定为 CPV-2c 突变株,在探针结合区域具有同义突变 A4061G,从而阻止了正确的菌株特征鉴定。使用小沟结合物探针的实时聚合酶链反应(PCR)检测能够识别突变体和经典 CPV-2c 菌株。这些结果表明,出现影响寡核苷酸结合区域的突变的 CPV 需要不断更新分子诊断工具,以便有效地检测到那些新出现的菌株。

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