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腮腺炎病毒临床口漱液样本的一步法实时荧光定量PCR检测
引用本文:施海晶,王晶晶,陈俊英,陈巍,潘明,赵钢,孙强明.腮腺炎病毒临床口漱液样本的一步法实时荧光定量PCR检测[J].粉末涂料与涂装,2013,26(6):861-865.
作者姓名:施海晶  王晶晶  陈俊英  陈巍  潘明  赵钢  孙强明
作者单位:中国医学科学院北京协和医学院医学生物学研究所云南省重大传染病疫苗研发重点实验室,云南昆明,650118
基金项目:卫生部卫生行业科研专项(项目编号:200802035)
摘    要:目的建立腮腺炎病毒(mumps virus,MuV)临床口漱液样本一步法荧光定量PCR检测方法,为腮腺炎的临床诊断及免疫防控提供依据。方法对101份采集自中国南部3个省、自治区(云南、四川、广西)的临床疑似腮腺炎患者口漱液样本,分别采用细胞培养-MuV特异的巢式PCR法及TaqMan探针Real-time PCR法进行检测,比较两种方法检测MuV的灵敏性。结果细胞培养-MuV特异的巢式PCR法共检出31份MuV阳性样本,系统进化分析表明,该31株MuV均属于F基因亚型;TaqMan探针Real-time PCR法共检出41份MuV阳性样本,其中包含了细胞培养-MuV特异的巢式PCR法检出的31份阳性样本,TaqMan探针Real-time RT-PCR法对MuV的检出率(40.59%)高于传统细胞培养-巢式PCR法的检出率(30.69%)。结论 TaqMan探针Real-time PCR法的灵敏性、特异性和简便性均优于传统的细胞培养-MuV特异的巢式PCR法,可应用于腮腺炎的临床诊断及免疫防控。

关 键 词:腮腺炎病毒  口漱液  实时聚合酶链反应

One-step real-time fluorescent quantitative PCR assay for mumps virus in clinical saliva specimens
Abstract:Objective To develop an one-step real-time fluorescent quantitative PCR assay for mumps virus(MuV)in clinical saliva specimens and provide a basis for clinical diagnosis,prevention and control of mumps.Methods A total of 101 clinical saliva specimens collected from suspected patients with mumps in Yunnan and Sichuan Province as well as Guangxi Zhuang Autonomous Region,China were determined by cell culture-MuV specific nested PCR and real-time PCR with TaqMan probe respectively,based on which the sensitivities of the two methods were compared.Results Thirty-one MuV-positive specimens were found by cell culture-MuV specific nested PCR,all of which belonged to genotype F as proved by phylogenetic tree.However,41 MuV-positive specimens were found by real-time PCR with TaqMan probe,including the 31 positive specimens proved by cell culture-MuV specific nested PCR,indicating that the positive rate of Muv by real-time RT-PCR with TaqMan probe(40.59%)was higher than that by traditional cell culture-nested PCR(30.69%).Conclusion The sensitivity,specificity and simplicity of real-time PCR with TaqMan probe were higher than those of traditional cell culture-MuV specific nested PCR,which might be used for the clinical diagnosis,prevention and control of mumps.
Keywords:Mumps virus  Saliva  Real-time polymerase chain reaction
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