Multicenter Quality Assessment of PCR Methods for Detection of Enteroviruses-Reference-Cited by-同舟云学术

Multicenter Quality Assessment of PCR Methods for Detection of Enteroviruses

Published:1999-05 Issue:5 Volume:37 Page:1409-1414
ISSN:0095-1137
Container-title:Journal of Clinical Microbiology
language:en
Short-container-title:J Clin Microbiol

Author:

Muir Peter¹,Ras Albert²,Klapper Paul E.³,Cleator Graham M.³,Korn Klaus⁴,Aepinus Christian⁵,Fomsgaard Anders⁶,Palmer Pierre⁷,Samuelsson Agneta⁸,Tenorio Antonio⁹,Weissbrich Benedikt¹⁰,van Loon A. M.²¹¹

Affiliation:

1. Department of Virology, Guy’s, King’s College & St Thomas’ Hospitals’ School of Medicine, London,1 and

2. Research Laboratory for Infectious Diseases, National Institute of Public Health and the Environmental (RIVM), Bilthoven,2 and

3. Division of Virology, Department of Pathological Sciences, Manchester Royal Infirmary, Manchester,3 United Kingdom;

4. Institute for Clinical and Molecular Virology der Friedrich-Alexander-Universität Erlangen-Nürnberg, Erlangen,4

5. Department of Molecular Pathology, University of Tübingen, Tübingen,5 and

6. Department of Virology, Statens Seruminstitut, Copenhagen, Denmark6;

7. Service de Bacteriologie, Virologie et Hygiene, Hôpital Saint Vincent de Paul, Paris, France7;

8. Clinical Virology F68, Huddinge University Hospital, Huddinge, Sweden8; and

9. C.N.M., Instituto de Salud Carlos III, Madrid, Spain9

10. Institut für Virologie und Immunobiologie, Universität Würzburg, Würzburg,10 Germany;

11. Department of Virology, Utrecht Academic Hospital, Utrecht,11 The Netherlands;

Abstract

ABSTRACT We conducted a multicenter evaluation of commercial and in-house PCR methods for the detection of enteroviruses. Three coded panels of test and control RNA samples, artificial clinical specimens, and representative enterovirus serotypes were used to assess amplification methods, RNA extraction methods, and reactivities with different enterovirus serotypes. Despite several differences between PCR methods, there was good agreement, although some variation in sensitivity was observed. Most PCR methods were able to detect enterovirus RNA derived from 0.01 50% tissue culture infective dose (TCID 50 ) and were able to detect at least 1 TCID 50 of enterovirus in cerebrospinal fluid, stool, or throat swab specimens. Most were also able to detect a wide range of enterovirus serotypes, although serotypic identification was not possible. Some laboratories experienced false-positive results due to PCR contamination, which appeared to result mainly from cross-contamination of specimens during RNA extraction. Provided that this problem is overcome, these PCR methods will prove to be a sensitive and rapid alternative to cell culture for the diagnosis of enterovirus infection.

Publisher

American Society for Microbiology

Subject

Microbiology (medical)

Link

https://journals.asm.org/doi/pdf/10.1128/JCM.37.5.1409-1414.1999

Reference45 articles.

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