Typing and subtyping clinical isolates of influenza virus using reverse transcription-polymerase chain reaction

Clinical and diagnostic virology Pub Date : 1996-11-01 DOI:10.1016/S0928-0197(96)00254-1

Robert L. Atmar , Barbara D. Baxter

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引用次数: 25

Abstract

Background: Influenza virus infections are a major cause of morbidity and the identification of the type or subtype of a clinical isolate has important clinical and epidemiological implications.

Objectives: To evaluate the ability of a reverse transcription-polymerase chain reaction (RT-PCR) assay to type and subtype clinical human isolates of influenza virus.

Study design: Reference strains of influenza $A H1N1$ , $A H3N2$ , and B viruses and human clinical isolates of influenza virus representing antigenic variants from the last 15 years were evaluated using an RT-PCR assay.

Results: Amplicons of 325, 198 and 365 base pairs in length were obtained from RNA extracted from influenza $A H1N1$ , $A H3N2$ and B viruses, respectively. All human-derived $A H1N1$ , $A H3N2$ , and B reference strains and antigenic variants tested were correctly identified.

Conclusions: RT-PCR is an effective alternative to traditional methods for typing and subtyping influenza viruses.

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应用逆转录-聚合酶链反应对流感病毒临床分离株进行分型和分型

背景:流感病毒感染是发病率的主要原因，临床分离株的类型或亚型的鉴定具有重要的临床和流行病学意义。目的:评价逆转录聚合酶链反应(RT-PCR)测定流感病毒临床分离株分型和分型的能力。研究设计:采用RT-PCR方法对过去15年的AH1N1、AH3N2和B型流感病毒参考株和人类临床分离流感病毒抗原变异株进行评估。结果:从AH1N1、AH3N2和B型流感病毒提取的RNA中分别获得长度为325、198和365个碱基对的扩增子。所有人源性AH1N1、AH3N2和B参考菌株及抗原变异均被正确鉴定。结论:RT-PCR是流感病毒分型和分型的有效替代方法。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Clinical and diagnostic virology

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