PCR detection has become the gold standard for diagnosis and typing of enterovirus (EVs) and human parechovirus (HPeV) infections. Its effectiveness depends critically on using appropriate sample types and high assay sensitivity since viral loads in cerebrospinal fluid samples from meningitis and sepsis clinical presentation can be extremely low. This study evaluated the sensitivity and specificity of currently used commercial and in-house diagnostic and typing assays. Accurately quantified RNA transcript controls were distributed to 27 diagnostic and 12 reference laboratories in 17 European countries for blinded testing. Transcripts represented the 4 human EV species (EV-A71, echovirus 30, coxsackie A virus 21, EV-D68), HPeV-3 and specificity controls. Reported results from 48 in-house and 15 commercial assays showed 98% detection frequencies of high copy (1000 RNA copies/5µl) transcripts. In-house assays showed significantly greater detection frequencies of the low copy (10 copies/5µl) EV and HPeV transcripts (81%, 86% respectively) compared to commercial assays (56%, 50%; p = 7x10-5 ). EV-specific PCRs showed low cross-reactivity with human rhinovirus C (3/42 tests) and infrequent positivity in the negative control (2/63 tests). Most or all high copy EV and HPeV controls were successfully typed (88%, 100%) by reference laboratories, but showed reduced effectiveness for low copy controls (41%, 67%). Stabilised RNA transcripts provide an effective, logistically simple and inexpensive reagent for evaluation of diagnostic assay performance. The study provides reassurance of the performance of the many in-house assay formats used across Europe. However, it identified often substantially reduced sensitivities of commercial assays often used as point-of-care tests.
A European multi-centre evaluation of detection and typing methods for human enteroviruses and parechoviruses using RNA transcripts / A. Hayes, D. Nguyen, M. Andersson, A. Antón, J. Bailly, S. Beard, K.S.M. Benschop, N. Berginc, S. Blomqvist, E. Cunningham, D. Davis, J.L. Dembinski, S. Diedrich, S.G. Dudman, R. Dyrdak, G.J.A. Eltringham, S. Gonzales-Goggia, R. Gunson, H.C. Howson-Wells, A.J. Jääskeläinen, F.X. López-Labrador, M. Maier, M. Majumdar, S. Midgley, A. Mirand, U. Morley, S.A. Nordbø, S. Oikarinen, H. Osman, A. Papa, L. Pellegrinelli, A. Piralla, N. Rabella, J. Richter, M. Smith, A. Söderlund Strand, K. Templeton, B. Vipond, T. Vuorinen, C. Williams, E. Wollants, K. Zakikhany, T.K. Fischer, H. Harvala, P. Simmonds. - In: JOURNAL OF MEDICAL VIROLOGY. - ISSN 0146-6615. - (2019 Dec 28). [Epub ahead of print] [10.1002/jmv.25659]
A European multi-centre evaluation of detection and typing methods for human enteroviruses and parechoviruses using RNA transcripts
L. Pellegrinelli;
2019
Abstract
PCR detection has become the gold standard for diagnosis and typing of enterovirus (EVs) and human parechovirus (HPeV) infections. Its effectiveness depends critically on using appropriate sample types and high assay sensitivity since viral loads in cerebrospinal fluid samples from meningitis and sepsis clinical presentation can be extremely low. This study evaluated the sensitivity and specificity of currently used commercial and in-house diagnostic and typing assays. Accurately quantified RNA transcript controls were distributed to 27 diagnostic and 12 reference laboratories in 17 European countries for blinded testing. Transcripts represented the 4 human EV species (EV-A71, echovirus 30, coxsackie A virus 21, EV-D68), HPeV-3 and specificity controls. Reported results from 48 in-house and 15 commercial assays showed 98% detection frequencies of high copy (1000 RNA copies/5µl) transcripts. In-house assays showed significantly greater detection frequencies of the low copy (10 copies/5µl) EV and HPeV transcripts (81%, 86% respectively) compared to commercial assays (56%, 50%; p = 7x10-5 ). EV-specific PCRs showed low cross-reactivity with human rhinovirus C (3/42 tests) and infrequent positivity in the negative control (2/63 tests). Most or all high copy EV and HPeV controls were successfully typed (88%, 100%) by reference laboratories, but showed reduced effectiveness for low copy controls (41%, 67%). Stabilised RNA transcripts provide an effective, logistically simple and inexpensive reagent for evaluation of diagnostic assay performance. The study provides reassurance of the performance of the many in-house assay formats used across Europe. However, it identified often substantially reduced sensitivities of commercial assays often used as point-of-care tests.File | Dimensione | Formato | |
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