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1
Development and evaluation of nucleic acid sequence based amplification (NASBA) for diagnosis of enterovirus infections using the NucliSens Basic Kit.使用NucliSens Basic试剂盒开发和评估基于核酸序列扩增技术(NASBA)用于肠道病毒感染的诊断。
J Clin Virol. 2002 Feb;24(1-2):117-30. doi: 10.1016/s1386-6532(01)00241-4.
2
Evaluation of a one-tube RT-PCR system for detection of enteroviruses.用于检测肠道病毒的单管逆转录聚合酶链反应(RT-PCR)系统的评估
J Clin Virol. 2002 Feb;24(1-2):25-30. doi: 10.1016/s1386-6532(01)00234-7.
3
Rapid detection of enterovirus RNA in cerebrospinal fluid specimens with a novel single-tube real-time reverse transcription-PCR assay.用新型单管实时逆转录-聚合酶链反应分析法快速检测脑脊液标本中的肠道病毒RNA
J Clin Microbiol. 2001 Nov;39(11):4093-6. doi: 10.1128/JCM.39.11.4093-4096.2001.
4
Detection of enteroviral sequences from frozen spinal cord samples of Japanese ALS patients.从日本肌萎缩侧索硬化症患者的冷冻脊髓样本中检测肠道病毒序列。
Neurology. 2001 Jun 26;56(12):1777-8. doi: 10.1212/wnl.56.12.1777.
5
Absence of echovirus sequences in brain and spinal cord of amyotrophic lateral sclerosis patients.肌萎缩侧索硬化症患者的脑和脊髓中无肠道病毒序列。
Ann Neurol. 2001 Feb;49(2):249-53.
6
Pleconaril: a novel antipicornaviral drug.普来可那立:一种新型抗微小核糖核酸病毒药物。
Expert Opin Investig Drugs. 2001 Feb;10(2):369-79. doi: 10.1517/13543784.10.2.369.
7
Enterovirus infections: diagnosis and treatment.肠道病毒感染:诊断与治疗。
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Treatment of potentially life-threatening enterovirus infections with pleconaril.用普来可那立治疗潜在危及生命的肠道病毒感染。
Clin Infect Dis. 2001 Jan 15;32(2):228-35. doi: 10.1086/318452.
9
Detection and cellular localization of enterovirus RNA sequences in spinal cord of patients with ALS.肌萎缩侧索硬化症患者脊髓中肠道病毒RNA序列的检测及细胞定位
Neurology. 2000 Nov 14;55(9):1420-1. doi: 10.1212/wnl.55.9.1420.
10
Quantification of enterovirus RNA in sludge samples using single tube real-time RT-PCR.使用单管实时逆转录聚合酶链反应对污泥样本中的肠道病毒RNA进行定量分析。
Biotechniques. 2000 Jul;29(1):88-93. doi: 10.2144/00291st03.

通过实时聚合酶链反应对不同临床标本中的肠道病毒属所有成员进行快速灵敏的常规检测。

Rapid and sensitive routine detection of all members of the genus enterovirus in different clinical specimens by real-time PCR.

作者信息

Nijhuis Monique, van Maarseveen Noortje, Schuurman Rob, Verkuijlen Sandra, de Vos Machiel, Hendriksen Karin, van Loon Anton M

机构信息

Department of Virology G04.614, Eijkman Winkler Center for Microbiology, University Medical Center Utrecht, Heidelberglaan 100, 3584 CX Utrecht, The Netherlands.

出版信息

J Clin Microbiol. 2002 Oct;40(10):3666-70. doi: 10.1128/JCM.40.10.3666-3670.2002.

DOI:10.1128/JCM.40.10.3666-3670.2002
PMID:12354863
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC130891/
Abstract

We developed a rapid and sensitive method for the routine detection of all members of the enterovirus genus in different clinical specimens by using real-time TaqMan quantitative PCR. Multiple primer and probe sets were selected in the highly conserved 5'-untranslated region of the enterovirus genome. Our assay detected all 60 different enterovirus species tested, whereas no reactivity was observed with the viruses from the other genera of the picornaviridae family, e.g., hepatovirus and parechovirus. Weak cross-reactivity was observed with 7 of the 90 different high-titer rhinovirus stocks but not with rhinovirus-positive clinical isolates. Analysis of a well-characterized reference panel containing different enteroviruses at various concentrations demonstrated that the enterovirus real-time TaqMan PCR is as sensitive as most of the currently used molecular detection assays. Evaluation of clinical isolates demonstrated that the assay is more sensitive than the "gold standard" method, i.e., viral culture. Moreover, the PCR assay can be used on different clinical specimens, such as plasma, serum, nose and throat swabs, cerebrospinal fluid, and bronchoalveolar lavage, without apparent inhibition. Our data demonstrate that the real-time TaqMan PCR is a rapid and sensitive assay for the detection of enterovirus infection. The assay has a robust character and is easily standardized, which makes it an excellent alternative for the conventional time-consuming viral culture.

摘要

我们开发了一种快速灵敏的方法,通过实时TaqMan定量PCR对不同临床标本中的肠道病毒属所有成员进行常规检测。在肠道病毒基因组高度保守的5'-非翻译区选择了多组引物和探针。我们的检测方法检测了所测试的全部60种不同肠道病毒,而对微小核糖核酸病毒科其他属的病毒,如肝病毒和帕里病毒,未观察到反应性。在90种不同的高滴度鼻病毒毒株中有7种观察到弱交叉反应,但对鼻病毒阳性临床分离株未观察到交叉反应。对含有不同浓度不同肠道病毒的特征明确的参考样本进行分析表明,肠道病毒实时TaqMan PCR与目前使用的大多数分子检测方法一样灵敏。对临床分离株的评估表明,该检测方法比“金标准”方法即病毒培养更灵敏。此外,PCR检测可用于不同临床标本,如血浆、血清、鼻和咽拭子、脑脊液及支气管肺泡灌洗,且无明显抑制作用。我们的数据表明,实时TaqMan PCR是检测肠道病毒感染的一种快速灵敏的检测方法。该检测方法具有稳健的特性且易于标准化,这使其成为传统耗时的病毒培养的极佳替代方法。