Literature DB >> 21593263

Rapid simultaneous detection of enterovirus and parechovirus RNAs in clinical samples by one-step real-time reverse transcription-PCR assay.

Susan Bennett1, Heli Harvala, Jeroen Witteveldt, E Carol McWilliam Leitch, Nigel McLeish, Kate Templeton, Rory Gunson, William F Carman, Peter Simmonds.   

Abstract

Enteroviruses (EVs) are recognized as the major etiological agent in meningitis in children and young adults. The use of molecular techniques, such as PCR, has substantially improved the sensitivity of enterovirus detection compared to that of virus culture methods. PCR-based methods also can detect a much wider range of EV variants, including those within species A, as well as human parechoviruses (HPeVs) that often grow poorly in vitro and which previously have been underdiagnosed by traditional methods. To exploit these developments, we developed a real-time one-step reverse transcription-PCR (RT-PCR) for the rapid and sensitive detection of EV and HPeV in clinical specimens. Two commercially available RT-PCR kits were used (method I, Platinum one-step kit; method II, Express qPCR one-step kit) with primers and probes targeting the EV and HPeV 5'-untranslated regions (5'UTR). Amplification dynamics (threshold cycle [C(T)]values and efficiencies) of absolutely quantified full-length RNA transcripts representative of EV species A to D and HPeV were similar, demonstrating the effectiveness of both assays across the range of currently described human EV and HPeV variants. Probit analysis of multiple endpoint replicates demonstrated comparable sensitivities of the assays for EV and HPeV (method I, approximately 10 copies per reaction for both targets; method II, 20 copies per reaction). C(T) values were highly reproducible on repeat testing of positive controls within assays and between assay runs. Considering the sample turnaround time of less than 3 h, the multiplexed one-step RT-PCR method provides rapid diagnostic testing for EV and HPeV in cases of suspected central nervous system infections in a clinically relevant time frame.

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Year:  2011        PMID: 21593263      PMCID: PMC3147812          DOI: 10.1128/JCM.02445-10

Source DB:  PubMed          Journal:  J Clin Microbiol        ISSN: 0095-1137            Impact factor:   5.948


  26 in total

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Authors:  E C McWilliam Leitch; H Harvala; I Robertson; I Ubillos; K Templeton; P Simmonds
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Journal:  J Infect Dis       Date:  2009-06-15       Impact factor: 5.226

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  14 in total

1.  Development and assay of RNA transcripts of enterovirus species A to D, rhinovirus species a to C, and human parechovirus: assessment of assay sensitivity and specificity of real-time screening and typing methods.

Authors:  Nigel J McLeish; Jeroen Witteveldt; Lucy Clasper; Chloe McIntyre; E Carol McWilliam Leitch; Alison Hardie; Susan Bennett; Rory Gunson; William F Carman; Susan A Feeney; Peter V Coyle; Barry Vipond; Peter Muir; Kimberley Benschop; Katja Wolthers; Matti Waris; Riikka Osterback; Ingo Johannessen; Kate Templeton; Heli Harvala; Peter Simmonds
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2.  Optimization of a combined human parechovirus-enterovirus real-time reverse transcription-PCR assay and evaluation of a new parechovirus 3-specific assay for cerebrospinal fluid specimen testing.

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9.  Changes in human parechovirus profiles in hospitalized children with acute gastroenteritis after a three-year interval in Lanzhou, China.

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10.  Community-acquired diarrhea among children and adults in urban settings in Senegal: clinical, epidemiological and microbiological aspects.

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