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Review Article

A critical review of methods for detecting human noroviruses and predicting their infectivity

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Pages 295-309 | Received 04 May 2012, Accepted 04 Jul 2012, Published online: 20 Aug 2012
 

Abstract

Human noroviruses (hNoVs) are the single most common cause of acute non-bacterial gastroenteritis in the industrialized world but cannot be grown in simple culture systems. Different approaches for detecting hNoVs and predicting their infectivity are reviewed. Although reverse transcription quantitative PCR (RT-qPCR) is the most widely used method to detect human noroviruses (hNoVs) it is unable to discriminate between infectious and non-infectious particles. There is therefore a dilemma in assessing the risk to human health from samples detected as positive in RT-qPCR assays. In the absence of an efficient cell, culture based detection system for hNoVs RT-qPCR methods need to differentiate RT-qPCR signals from intact infective particles, intact defective particles, degraded particles (consisting of capsid protein and virus RNA, herein referred to as ribonucleoprotein complexes (RNPs), and “naked” RNA. This review provides a critical analysis of methods for detecting hNoVs, and differentiating such signals with reference to relevant studies of virus infectivity, structure, inactivation, and the disassembly of virus particles during infection. The application of these methods as an adjunct to the proposed RT-qPCR European Committee for Standards (CEN) methods for the detection of hNoVs in foods and the environment is discussed.

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Erratum

Acknowledgements

The authors gratefully acknowledge sight of the CEN working document (prEN XXXXX-2:2011) “Microbiology of food and animal feeding stuffs – Horizontal method for detection of hepatitis A virus and norovirus in food using real-time RT-PCR – Part 1” kindly supplied by Dr J. Lowther Centre for Environmental Fisheries and Aqua Science (CEFAS) Weymouth, UK.

Declaration of interest

This review was funded by the UK Food Standards Agency, project no. FS101036 with additional independent support from the Leatherhead Food Research food safety forum.

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