摘要
为建立一种能检测出临床上绝大多数肠道病毒(EV)感染的快速、敏感、特异的逆转录聚合酶链反应(RT-PCR)方法,通过对EV基因组的序列分析,在其5′端非编码区设计一对引物,用该引物建立的RT-PCR方法对31种EV标准毒株和34例无菌性脑膜炎及11例无菌性脑炎患儿的脑脊液(CSF)分别进行扩增,其产物做琼脂糖凝胶电泳及斑点杂交检测。研究表明,31种EV标准毒株斑点杂交的敏感度达10-2~10-350%组织培养感染量(TCID50)。34例无菌性脑膜炎中21例阳性(61.8%),11例无菌性脑炎中8例阳性(72.7%);阳性患儿恢复期CSF,2例无菌性脑膜炎和1例无菌性脑炎仍为阳性。提示用RT-PCR方法检测EV感染是值得推广的。
To establish a rapid diagnostic method for enteroviral infections in clinic, the authors developed a reverse transcription and polymerase chain reaction (RT PCR) assay. Primers homologous to the conserved 5′ noncoding region were designed by analysis of enteroviral genomes, and then were used to enzymatically amplify enterovirus (EV) specific RNA fragment from 31 prototype enteroviral strains and cerebrospinal fluid (CSF) of 34 patients with aseptic meningitis and 11 patients with encephalitis of unknown etiology. The amplified products were detected by agar gel electrophoresis and slot blot hybridization analysis. The study on sensitivity of the RT PCR showed that the amplification could detect EV RNA from 10 -2 ~10 -3 50% tissue culture infective doses of the cultured viral strains. The results also showed that 21 (61.8%) of 34 aseptic meningitis cases and 8 (72.7%) of 11 encephalitis cases were positive for EV RNA in CSF samples. Two meningitis and one encephalitis cases were positive during convalescence. These results suggested that this RT PCR method was rapid, sensitive and specific in detection of most common EV infections.
出处
《中华儿科杂志》
CAS
CSCD
北大核心
1997年第11期597-600,共4页
Chinese Journal of Pediatrics
