AimsTo provide a rapid and sensitive method for detecting NoV GI and NoV GII in water and to evaluate the use of the murine norovirus (MNV-1) as a process control. Methods and ResultsThe method is based on viral concentration by filtration on electropositive filters and direct lysis of adsorbed viruses from filters before RNA extraction and RT-qPCR amplification. An one-step multiplex RT-qPCR assay was developed for the simultaneous detection of NoV GI, NoV GII and MNV-1. Then, water samples were artificially contaminated to determine mean virus recoveries and method sensitivity. The method showed a higher sensitivity for detecting NoV GII (10(3) genome copies per 05l) than for NoV GI (10(4) genome copies per 05l) in the presence of MNV-1 regardless of the type of water. The data also showed that MNV-1 is a robust option as process control. ConclusionsThe method described provides a valuable tool for the monitoring of potential public health risks associated with NoV contamination in drinkable water. Significance and Impact of StudyGiven the increasing evidence for NoV involvement in food outbreaks, the one-step multiplex RT-qPCR assay we used in this study would be a very useful tool to investigate NoV contamination in other food products.