Rapid, simple and efficient method for detection of viral genomes on raspberries

A Perrin; J Loutreul; N Boudaud; I Bertrand; C Gantzer

doi:10.1016/j.jviromet.2015.08.005

Rapid, simple and efficient method for detection of viral genomes on raspberries

J Virol Methods. 2015 Nov:224:95-101. doi: 10.1016/j.jviromet.2015.08.005. Epub 2015 Aug 28.

Authors

A Perrin¹, J Loutreul², N Boudaud², I Bertrand¹, C Gantzer³

Affiliations

¹ Université de Lorraine, LCPME (Laboratoire de Chimie Physique et Microbiologie pour l'Environnement), UMR 7564, Nancy, France; CNRS, LCPME, UMR 7564, Nancy, France.
² ACTALIA, Food Safety Department, Villers-Bocage F-14310, France.
³ Université de Lorraine, LCPME (Laboratoire de Chimie Physique et Microbiologie pour l'Environnement), UMR 7564, Nancy, France; CNRS, LCPME, UMR 7564, Nancy, France. Electronic address: christophe.gantzer@univ-lorraine.fr.

PMID: 26318917
DOI: 10.1016/j.jviromet.2015.08.005

Abstract

In recent years, foodborne viruses, especially human noroviruses (NoV) and hepatitis A virus (HAV), have been increasingly reported as the causes of foodborne disease outbreaks. Soft red fruits, especially raspberries, have a high incidence among the types of food concerned. Due to low infectious doses and low concentrations of enteric viruses in food samples, it is necessary to have an efficient and rapid detection method to implement prevention measures. A standard method for virus detection and quantification in food, including raspberries (XP CEN ISO/TS 15216-1 and -2, 2013) is currently available. This method proposes a consensus detection approach by RT-real time PCR (RT-qPCR) but also a virus extraction procedure based on the elution-concentration principle. In this study, an alternative method of extraction in which RNAs are directly extracted from food matrices (based on direct RNA extraction) has been optimized. First, each step was improved to make it a highly rapid, specific and simple method. Second, the standard virus concentration method was compared with the optimized direct RNA extraction one. Human enteric viral surrogates, Murine Norovirus (MNV) and F-specific RNA bacteriophage GA, were selected according to their adhesion properties and resistance to pH close to our main targets (NoV and HAV). Raspberries were artificially contaminated using two different techniques (immersion and spotting) in order to define a recovery rate and the amounts of virus recovered. Results showed that the direct RNA extraction method revealed significantly higher viral extraction efficiency (46.2%) than the elution-concentration method (20.3%), with similar proportions of inhibitors for both. In the same way with inoculation by spotting, the best recovery rate of GA phage (39.7% against 0.7%) and MNV (42.8% against 0.5%) was observed by direct RNA extraction. For the lowest concentrations of phage and virus in the immersion bath, only the direct RNA extraction method allowed their recovery. Direct RNA extraction proved to be more effective (best recovery rate), faster (<8h) and simpler (fewer steps) than the one proposed in the CEN ISO standard method when it came to detecting enteric viruses on raspberries.

Keywords: Detection; F-specific RNA phage; Norovirus; RT-qPCR; Raspberries.

Publication types

Evaluation Study
Research Support, Non-U.S. Gov't

MeSH terms

Food Contamination*
Food Microbiology / methods*
Food Safety / methods*
Genome, Viral*
Molecular Diagnostic Techniques / methods*
RNA, Viral / isolation & purification
Rubus / virology*
Sensitivity and Specificity
Time Factors
Viruses / genetics
Viruses / isolation & purification*

Substances

RNA, Viral