Literature DB >> 27316440

Influenza A virus drift variants reduced the detection sensitivity of a commercial multiplex nucleic acid amplification assay in the season 2014/15.

Daniela Huzly1, Klaus Korn2, Sibylle Bierbaum1, Björn Eberle1, Valeria Falcone1, Antje Knöll2, Philipp Steininger2, Marcus Panning3.   

Abstract

The influenza season 2014/15 was dominated by drift variants of influenza A(H3N2), which resulted in a reduced vaccine effectiveness. It was not clear if the performance of commercial nucleic-acid-based amplification (NAT) assays for the detection of influenza was affected. The purpose of this study was to perform a real-life evaluation of two commercial NAT assays. During January-April 2015, we tested a total of 665 samples from patients with influenza-like illness using the Fast Track Diagnostics Respiratory pathogens 21, a commercial multiplex kit, (cohorts 1 and 2, n = 563 patients) and the Xpert Flu/RSV XC assay (cohort 3, n = 102 patients), a single-use cartridge system. An in-house influenza real-time RT-PCR (cohort 1) and the RealStar Influenza RT-PCR 1.0 Kit (cohort 2 and 3) served as reference tests. Compared to the reference assay, an overall agreement of 95.9 % (cohort 1), 95 % (cohort 2), and 98 % (cohort 3) was achieved. A total of 24 false-negative results were observed using the Fast Track Diagnostics Respiratory pathogens 21 kit. No false-negative results occurred using the Xpert Flu/RSV XC assay. The Fast Track Diagnostics Respiratory pathogens 21 kit and the Xpert Flu/RSV XC assay had sensitivities of 90.7 % and 100 % and specificities of 100 % and 94.1 %, respectively, compared to the RealStar 1.0 kit. Upon modification of the Fast Track Diagnostics Respiratory pathogens 21 kit, the sensitivity increased to 97.3 %. Influenza virus strains circulating during the 2014/15 season reduced the detection sensitivity of a commercial NAT assay, and continuous monitoring of test performance is therefore necessary.

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Year:  2016        PMID: 27316440     DOI: 10.1007/s00705-016-2930-8

Source DB:  PubMed          Journal:  Arch Virol        ISSN: 0304-8608            Impact factor:   2.574


  11 in total

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3.  Development of Mobile Laboratory for Viral Hemorrhagic Fever Detection in Africa.

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4.  Ad hoc laboratory-based surveillance of SARS-CoV-2 by real-time RT-PCR using minipools of RNA prepared from routine respiratory samples.

Authors:  Anna M Eis-Hübinger; Mario Hönemann; Jürgen J Wenzel; Annemarie Berger; Marek Widera; Barbara Schmidt; Souhaib Aldabbagh; Benjamin Marx; Hendrik Streeck; Sandra Ciesek; Uwe G Liebert; Daniela Huzly; Hartmut Hengel; Marcus Panning
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Authors:  Evan Toth; Erica D Dawson; Amber W Taylor; Robert S Stoughton; Rebecca H Blair; James E Johnson; Amelia Slinskey; Ryan Fessler; Catherine B Smith; Sarah Talbot; Kathy Rowlen
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9.  Identification of H3N2 NA and PB1-F2 genetic variants and their association with disease symptoms during the 2014-15 influenza season.

Authors:  Deena R Blumenkrantz; Thomas Mehoke; Kathryn Shaw-Saliba; Harrison Powell; Nicholas Wohlgemuth; Hsuan Liu; Elizabeth Macias; Jared Evans; Mitra Lewis; Rebecca Medina; Justin Hardick; Lauren M Sauer; Andrea Dugas; Anna DuVal; Andrew P Lane; Charlotte Gaydos; Richard Rothman; Peter Thielen; Andrew Pekosz
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Review 10.  Recent advances in the detection of respiratory virus infection in humans.

Authors:  Naru Zhang; Lili Wang; Xiaoqian Deng; Ruiying Liang; Meng Su; Chen He; Lanfang Hu; Yudan Su; Jing Ren; Fei Yu; Lanying Du; Shibo Jiang
Journal:  J Med Virol       Date:  2020-02-04       Impact factor: 2.327

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