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Rapid Detection of Human Rhinoviruses in Nasopharyngeal Aspirates by a Microwell Reverse Transcription-PCR–Hybridization Assay

机译:微孔逆转录PCR-杂交分析法快速检测鼻咽液中的人类鼻病毒

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A rapid and sensitive microwell reverse transcription (RT)-PCR–hybridization assay was developed to detect human rhinoviruses in clinical specimens and cell culture suspensions. Two hundred three nasopharyngeal aspirates collected from children with symptoms of respiratory disease were analyzed by a classical rolling-tube cell culture method, microwell culture of HeLa Ohio cell monolayers, and RT-PCR with detection of the amplicons in a microwell hybridization assay. The RT-PCR was also done with harvests of the microwell cultures. RNA was extracted with a commercial kit, and the RT-PCR procedure was carried out with microtiter-format equipment. A confirmatory test that exploited a blocking oligonucleotide at the hybridization step was developed to reliably identify marginally positive specimens. Of the 203 nasopharyngeal aspirate specimens, rhinovirus or rhinoviral RNA was detected in 111 specimens (55%). Ninety-eight specimens (48%) were found to be positive by RT-PCR of the original nasopharyngeal aspirates, while the conventional rolling-tube cell culture method yielded 52 (26%) positive specimens. This RT-PCR method with solid-phase hybridization is easy to perform, sensitive, and specific and will be especially useful for analysis of large numbers of clinical specimens.
机译:开发了一种快速灵敏的微孔逆转录(RT)-PCR杂交测定法,以检测临床标本和细胞培养悬浮液中的人鼻病毒。通过经典滚动管细胞培养方法,HeLa Ohio细胞单层微孔培养和RT-PCR分析从呼吸道疾病症状患儿收集的203鼻咽抽吸物,并在微孔杂交测定中检测扩增子。 RT-PCR也用微孔培养物的收获物进行。用市售试剂盒提取RNA,并用微量滴定仪进行RT-PCR。开发了在杂交步骤中使用封闭寡核苷酸的验证性测试,以可靠地鉴定边缘阳性样本。在203例鼻咽抽吸物中,在111例标本中检出了鼻病毒或鼻病毒RNA(占55%)。 RT-PCR检测到最初的鼻咽抽吸物有98个标本(48%)呈阳性,而传统的滚管细胞培养方法产生了52个(26%)阳性标本。这种具有固相杂交的RT-PCR方法易于操作,灵敏且特异,对于分析大量临床标本特别有用。

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