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采用聚合酶链反应检测无菌性脑膜炎患者粪便样本中的肠道病毒RNA。

Detection of enteroviral RNA by polymerase chain reaction in faecal samples from patients with aseptic meningitis.

作者信息

Glimåker M, Abebe A, Johansson B, Ehrnst A, Olcén P, Strannegård O

机构信息

Department of Infectious Diseases, Orebro Medical Centre Hospital, Sweden.

出版信息

J Med Virol. 1992 Sep;38(1):54-61. doi: 10.1002/jmv.1890380112.

Abstract

An assay based on the polymerase chain reaction (PCR) for detection of enteroviral RNA in stool samples was carried out using specimens from 74 patients with aseptic meningitis. The primer pair and probe were derived from the highly conserved 5' non-coding enterovirus genomic region. Enteroviral RNA was detected in faeces of all 36 patients in whom an enterovirus was isolated from stool. The PCR assay yielded positive results in additionally 3/6 cases where enterovirus diagnoses were obtained by virus isolation from cerebrospinal fluid and/or serological tests. Thus, the positive outcome of the PCR assay was 39 (93%) among the 42 patients with enterovirus diagnoses. Furthermore, 7/19 (37%) cases with an etiology that was not established by other means were positive in the test indicating that the PCR assay may give considerable additional etiological information in patients with aseptic meningitis. The limit of RNA detectability in the PCR assay was about 100 TCID50 when highly cytopathogenic enterovirus types (coxsackievirus type B5 and echovirus type 11) were tested. The PCR was negative in all 13 patients with non-enterovirus diagnoses except in one case with a herpes simplex virus type 2 infection. Since enterovirus-specific IgM antibodies could be detected in this case a dual infection seemed probable. All the negative controls, included in the study, were PCR-negative and no contamination was encountered. This study proves the usefulness of the PCR assay for detection of enteroviral RNA in stool samples and suggests that the test may be an alternative to virus isolation for rapid enterovirus diagnosis in patients with aseptic meningitis.

摘要

采用聚合酶链反应(PCR)检测74例无菌性脑膜炎患者粪便样本中的肠道病毒RNA。引物对和探针来源于高度保守的肠道病毒基因组5'非编码区。在所有36例从粪便中分离出肠道病毒的患者粪便中均检测到肠道病毒RNA。在另外3/6例通过脑脊液病毒分离和/或血清学检测确诊为肠道病毒感染的病例中,PCR检测结果呈阳性。因此,在42例确诊为肠道病毒感染的患者中,PCR检测阳性结果为39例(93%)。此外,在19例其他方法未能明确病因的病例中,有7例(37%)检测呈阳性,这表明PCR检测可为无菌性脑膜炎患者提供大量额外的病因学信息。当检测高细胞致病性肠道病毒类型(B5型柯萨奇病毒和11型埃可病毒)时,PCR检测中RNA的可检测下限约为100个半数组织培养感染剂量(TCID50)。除1例2型单纯疱疹病毒感染病例外,13例非肠道病毒感染诊断的患者PCR检测均为阴性。由于该病例中可检测到肠道病毒特异性IgM抗体,因此可能存在双重感染。研究中纳入的所有阴性对照PCR检测均为阴性,未发现污染情况。本研究证明了PCR检测在粪便样本中检测肠道病毒RNA的实用性,并表明该检测可能是无菌性脑膜炎患者快速诊断肠道病毒感染的病毒分离替代方法。

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