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通过聚合酶链反应检测无菌性脑膜炎患者脑脊液中的肠道病毒RNA。

Detection of enteroviral RNA by polymerase chain reaction in cerebrospinal fluid from patients with aseptic meningitis.

作者信息

Glimåker M, Johansson B, Olcén P, Ehrnst A, Forsgren M

机构信息

Department of Virology, Central Microbiological Laboratory of the Stockholm, Orebro Medical Center Hospital, Sweden.

出版信息

Scand J Infect Dis. 1993;25(5):547-57. doi: 10.3109/00365549309008542.

Abstract

An assay based on a 2-step (semi-nested) polymerase chain reaction (PCR) was developed and evaluated for detection of enterovirus-specific RNA in cerebrospinal fluid (CSF) from patients with aseptic meningitis of different etiology. The limit of detectability of enteroviral RNA was equivalent to about 0.25 tissue culture infective doses 50%. In samples, stored at -70 degrees C, analyzed without repeated thawing, enteroviral RNA was demonstrable in 21/22 CSF specimens from which an enterovirus had been isolated. Enteroviral RNA was shown to be degraded during freeze-thawing of the samples. In repeatedly freeze-thawed samples from 134 consecutive patients with aseptic meningitis, a lower sensitivity (34/48 = 0.71) was observed. In the latest phase of the study, comprising 35 consecutive patients, the PCR was performed in CSF stored at -20 degrees C without thawing. In this material, the PCR yielded positive results in 19 patients, whereas enteroviruses were isolated from 6 cases only. In the total clinical material of 169 patients, 67 (40%) were found positive by PCR, whereas an enterovirus was isolated from CSF in 54 (32%) cases. All the 13 isolated enterovirus serotypes found in the study were demonstrable by PCR, indicating that the assay is broad-reacting within the enterovirus group. The specificity appeared to be high, since all of 21 patients with non-enteroviral diagnoses were negative by the PCR test, except 1 with an Epstein-Barr virus infection. As serological evidence of enteroviral etiology was found in this patient, a dual infection seemed probable. This study indicates that enteroviral RNA can be detected in CSF by a 2-step PCR in meningitis caused by enterovirus and that the technique has the potential to become a screening method for routine diagnosis of enteroviral meningitis.

摘要

开发并评估了一种基于两步(半巢式)聚合酶链反应(PCR)的检测方法,用于检测不同病因无菌性脑膜炎患者脑脊液(CSF)中的肠道病毒特异性RNA。肠道病毒RNA的检测限相当于约0.25个组织培养感染剂量的50%。在储存在-70℃且未反复冻融的样本中,从22份已分离出肠道病毒的脑脊液标本中,21份检测到肠道病毒RNA。样本冻融过程中肠道病毒RNA会降解。在134例连续无菌性脑膜炎患者反复冻融的样本中,观察到较低的敏感性(34/48 = 0.71)。在研究的最后阶段,纳入35例连续患者,对储存在-20℃未解冻的脑脊液进行PCR检测。在此材料中,PCR在19例患者中得到阳性结果,而仅从6例中分离出肠道病毒。在169例患者的全部临床材料中,PCR检测发现67例(40%)呈阳性,而54例(32%)脑脊液中分离出肠道病毒。研究中发现的所有13种分离出的肠道病毒血清型均可通过PCR检测到,表明该检测方法在肠道病毒组内具有广泛反应性。特异性似乎较高,因为21例非肠道病毒诊断患者中,除1例感染爱泼斯坦-巴尔病毒外,其余PCR检测均为阴性。由于该患者发现有肠道病毒病因的血清学证据,可能存在双重感染。本研究表明,在肠道病毒引起的脑膜炎中,可通过两步PCR在脑脊液中检测到肠道病毒RNA,且该技术有可能成为肠道病毒性脑膜炎常规诊断的筛查方法。

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