荧光恒温扩增技术检测单纯疱疹病毒Ⅰ型RNA方法的建立

doi:10.3969/j.issn.1673-8640.2016.03.003

检验医学 ›› 2016, Vol. 31 ›› Issue (3): 163-167.DOI: 10.3969/j.issn.1673-8640.2016.03.003

荧光恒温扩增技术检测单纯疱疹病毒Ⅰ型RNA方法的建立

曹凌峰¹, 苏犁云¹, 施鹏², 董妞妞¹, 徐锦¹

1.复旦大学附属儿科医院临床检验中心,上海 201102
2.复旦大学附属儿科医院信息中心,上海 201102

收稿日期:2015-08-12 出版日期:2016-03-30 发布日期:2016-04-08
作者简介:null
作者简介：曹凌峰,男,1972年生,硕士,副主任技师,主要从事病毒学检验及感染机制研究。

通讯作者：徐锦,联系电话：021-64931893。
基金资助:
上海市公共卫生优秀学科带头人计划（GWDTT201221）

Detection of herpes simplex virus ⅠRNA using simultaneous amplification and testing

CAO Lingfeng¹, SU Liyun¹, SHI Peng², DONG Niuniu¹, XU Jin¹

1. Clinical Laboratory Center,Children's Hospital of Fudan University,Shanghai 201102,China
2. Information Center,Children's Hospital of Fudan University,Shanghai 201102,China

Received:2015-08-12 Online:2016-03-30 Published:2016-04-08

摘要/Abstract

摘要：

目的利用荧光恒温扩增技术（SAT）建立一种快速、可靠的单纯疱疹病毒Ⅰ型（HSV-1）检测方法。方法根据Genbank上获取HSV-1 开放读码框Us5区域的RNA序列设计扩增引物及优化探针,使用M-MLV反转录酶及T7 RNA多聚酶对HSV-1 RNA 进行核酸扩增,同时利用荧光定量聚合酶链反应（PCR）仪进行实时荧光信号收集和检测。收集儿童病毒性脑炎或疑似患儿样本212份（脑脊液样本150份、血浆样本62份）,以巢式PCR + 测序为参比方法,对SAT结果进行Kappa一致性分析。结果SAT检测HSV-1 RNA的灵敏度为100 拷贝/μL,采用SAT检测212份临床样本,共检测出18例HSV-1阳性样本,巢式PCR检出16例阳性,经测序证实其中12例为阳性结果。 SAT与巢式PCR + 测序方法的Kappa值为0.785,其敏感性为100.0%、特异性为97.0%。结论建立的SAT检测脑脊液和血浆中HSV-1 RNA的方法具有敏感性高、特异性强、准确、快速、可靠的优点,适用于临床对单纯疱疹病毒性脑炎早期的快速诊断。

关键词: 单纯疱疹病毒I型, 荧光恒温扩增技术, 单纯疱疹性脑炎, 特异性, 敏感性

Abstract:

Objective To establish a rapid and reliable simultaneous amplification and testing （SAT） for detecting herpes simplex virus Ⅰ（HSV-1）. Methods The specific primers were designed,and the probes were optimized according to RNA sequences in open reading frame Us5 region of HSV-1 from GenBank,and HSV-1 RNA was amplified by M-MLV reverse transcriptase and T7 RNA polymerase. The fluorescence signals were collected and determined by fluorescence quantitation polymerase chain reaction （PCR）. A total of 212 clinical specimens （150 cerebrospinal fluid specimens and 62 plasma specimens） were collected from child patients,who were diagnosed or suspected with viral meningitis,and they were determined. Using nested PCR plus sequencing as reference method,the Kappa consistency analysis was performed on the SAT results. Results The sensitivity of HSV-1 RNA by SAT was 100 copies/μL. A total of 18 specimens were positive by SAT, among which 16 specimens were positive by nested PCR,and 12 specimens were positive by sequencing. The Kappa value between SAT and nested PCR plus sequencing was 0.785,and the sensitivity and specificity were 100.0% and 97.0%,respectively. Conclusions The established SAT is a sensitive,specific,accurate,rapid and reliable method for detecting HSV-1 RNA in cerebrospinal fluid and plasma,and it should be a potential method in rapid diagnosis of herpes simplex encephalitis.

Key words: Herpes simplex virus Ⅰ, Simultaneous amplification and testing, Herpes simplex encephalitis, Specificity, Sensitivity

中图分类号:

R446.1

曹凌峰, 苏犁云, 施鹏, 董妞妞, 徐锦. 荧光恒温扩增技术检测单纯疱疹病毒Ⅰ型RNA方法的建立[J]. 检验医学, 2016, 31(3): 163-167.

CAO Lingfeng, SU Liyun, SHI Peng, DONG Niuniu, XU Jin. Detection of herpes simplex virus ⅠRNA using simultaneous amplification and testing[J]. Laboratory Medicine, 2016, 31(3): 163-167.

图/表 3

参考文献 16

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名称	序列（5′~3′）
含T7启动子的引物1	aatttaatacgactcactatagggagaGACGATAGTGTCACACGGCCGGGCTA
引物2	CCAAACCATGTCCGGCAGG
探针	CACCGGGCUAACCAGGAAAUCGGUG
竞争性内标探针巢式PCR引物	CCGACAGUGAUACGAGAGTCGG FIRST Primer F： TGCCGTTGTTCCCATTATCC FIRST Primer R： CGCCATCGCACCAATACACA Second primer F1： AACCCCAACTCCAGACCAC Second primer R： TGAGGAACGAGAACAGCGGGGTAT

名称	序列（5′~3′）
含T7启动子的引物1	aatttaatacgactcactatagggagaGACGATAGTGTCACACGGCCGGGCTA
引物2	CCAAACCATGTCCGGCAGG
探针	CACCGGGCUAACCAGGAAAUCGGUG
竞争性内标探针巢式PCR引物	CCGACAGUGAUACGAGAGTCGG FIRST Primer F： TGCCGTTGTTCCCATTATCC FIRST Primer R： CGCCATCGCACCAATACACA Second primer F1： AACCCCAACTCCAGACCAC Second primer R： TGAGGAACGAGAACAGCGGGGTAT

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荧光恒温扩增技术检测单纯疱疹病毒Ⅰ型RNA方法的建立

Detection of herpes simplex virus ⅠRNA using simultaneous amplification and testing

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参考文献 16

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Metrics

SAT	巢式PCR+测序		合计
SAT	阳性	阴性	合计
阳性	12	6	18
阴性	0	194	194
合计	12	200	212

SAT	巢式PCR+测序		合计
SAT	阳性	阴性	合计
阳性	12	6	18
阴性	0	194	194
合计	12	200	212