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通过聚合酶链反应检测鼻洗液中的人鼻病毒RNA。

Detection of human rhinovirus RNA in nasal washings by PCR.

作者信息

Arruda E, Hayden F G

机构信息

Department of Internal Medicine, University of Virginia School of Medicine, Charlottesville 22908.

出版信息

Mol Cell Probes. 1993 Oct;7(5):373-9. doi: 10.1006/mcpr.1993.1055.

Abstract

A PCR assay was developed to detect human rhinovirus (HRV) RNA in nasal washings from individuals experimentally infected with HRV-39 or HRV strain Hanks. Total RNA was purified from samples stored in the presence of vanadyl ribonucleoside complex (VRC) by one of two methods: proteinase K digestion followed by multiple extractions with phenol/chloroform (PK-PC); or denaturation with guanidinium thiocyanate followed by one phenol/chloroform extraction (GTC). The limit of detection of HRV in nasal washings spiked with HRV-39 was lower with the GTC method (1 TCID50) than with the PK-PC method. In a study of 31 nasal washings extracted by the PK-PC method, the sensitivity (93%) and negative predictive value (94%) were sub-optimal in comparison to cell culture. In a study of 60 nasal washings extracted by the GTC method, the number of samples positive by PCR (25) exceeded by two the number positive by isolation in cell culture. A GTC-based method for HRV RNA extraction in nasal washings was superior to a proteinase K-phenol/chloroform-based method in regard to sensitivity, consumption of reagents, material and time.

摘要

开发了一种聚合酶链反应(PCR)检测方法,用于检测经鼻病毒39型(HRV-39)或汉克斯鼻病毒株实验性感染个体的鼻腔冲洗液中的人鼻病毒(HRV)RNA。通过以下两种方法之一从储存在钒核糖核苷复合物(VRC)中的样本中纯化总RNA:蛋白酶K消化,然后用苯酚/氯仿多次萃取(PK-PC);或用硫氰酸胍变性,然后进行一次苯酚/氯仿萃取(GTC)。用GTC方法检测加有HRV-39的鼻腔冲洗液中HRV的检测限(1个半数组织培养感染剂量(TCID50))低于PK-PC方法。在一项对31份用PK-PC方法提取的鼻腔冲洗液的研究中,与细胞培养相比,灵敏度(93%)和阴性预测值(94%)并不理想。在一项对60份用GTC方法提取的鼻腔冲洗液的研究中,PCR检测呈阳性的样本数量(25份)比细胞培养分离出的阳性样本数量多两份。就灵敏度、试剂消耗、材料和时间而言,基于GTC的鼻腔冲洗液中HRV RNA提取方法优于基于蛋白酶K-苯酚/氯仿的方法。

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