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1995年和1996年英格兰及威尔士甲型和乙型流感病毒监测的多重逆转录-聚合酶链反应

Multiplex reverse transcription-PCR for surveillance of influenza A and B viruses in England and Wales in 1995 and 1996.

作者信息

Ellis J S, Fleming D M, Zambon M C

机构信息

Enteric and Respiratory Virus Laboratory, Central Public Health Laboratory, Colindale, London, United Kingdom.

出版信息

J Clin Microbiol. 1997 Aug;35(8):2076-82. doi: 10.1128/jcm.35.8.2076-2082.1997.

Abstract

Multiple-target (multiplex) reverse transcription-PCR (RT-PCR) for detection, typing, and subtyping of the hemagglutinin gene of influenza type A (H3N2 and H1N1) and type B viruses was developed and applied prospectively to virological surveillance of influenza in England in the 1995-1996 winter season. During this season both influenza A H3N2 and H1N1 viruses were circulating, although at different times. Six hundred nineteen combined nose and throat swabs taken by general practitioners in sentinel practices from individuals presenting with "influenzalike illness" were analyzed by culture, multiplex RT-PCR, and immunofluorescence. Of the 619 samples, 246 (39.7%) were positive by multiplex RT-PCR compared with 200 (32.3%) which yielded influenza viruses on culture. There was 100% correlation between multiplex RT-PCR typing and subtyping and the influenza types and subtypes obtained from culture. There was also excellent correlation between the temporal detection of influenza A H3N2 and H1N1 viruses by multiplex RT-PCR and by culture. During the peak weeks of influenza virus activity, a total of 259 specimens were received, of which 101 (38.9%) yielded influenza viruses on culture while 149 (57.5%) were positive in multiplex RT-PCR, providing an increase in detection of influenza viruses of approximately 20%. The increased detection of influenza virus occurred in all the age groups sampled. Samples which were positive by multiplex RT-PCR but negative by culture were not detected significantly earlier or later in the winter of 1995-1996 but were detected during the peak weeks of clinical influenza virus activity. Multiplex RT-PCR was successfully used in surveillance of influenza to provide accurate, sensitive diagnosis directly on clinical specimens sent through the post.

摘要

开发了用于检测、分型和亚型分析甲型流感(H3N2和H1N1)及乙型流感病毒血凝素基因的多靶点(多重)逆转录聚合酶链反应(RT-PCR),并前瞻性地应用于1995 - 1996年冬季英格兰流感的病毒学监测。在这个季节,甲型流感H3N2和H1N1病毒均有传播,不过时间不同。由全科医生在哨点诊所采集的619份出现“流感样疾病”个体的鼻喉联合拭子样本,通过培养、多重RT-PCR和免疫荧光进行了分析。在619份样本中,多重RT-PCR检测出246份(39.7%)呈阳性,而培养出流感病毒的有200份(32.3%)。多重RT-PCR分型和亚型分析结果与从培养获得的流感类型和亚型之间存在100%的相关性。通过多重RT-PCR和培养对甲型流感H3N2和H1N1病毒进行的时间检测之间也存在极好的相关性。在流感病毒活动的高峰周期间,共收到259份标本,其中101份(38.9%)培养出流感病毒,而149份(57.5%)在多重RT-PCR中呈阳性,流感病毒检测率提高了约20%。流感病毒检测率的提高在所有采样年龄组中均有出现。多重RT-PCR呈阳性但培养呈阴性的样本在1995 - 1996年冬季并未在明显更早或更晚的时候被检测到,而是在临床流感病毒活动的高峰周期间被检测到。多重RT-PCR成功用于流感监测,可直接对通过邮寄送来的临床标本进行准确、灵敏的诊断。

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