Screening test for neutralizing antibodies against yellow fever virus, based on a flavivirus pseudotype.

Séverine Mercier-Delarue,Jean-Claude Manuggera,Maria Dolores Fernandez Garcia,Christine Durier,Jean-Dominique Poveda,Nathalie Colin De Verdière,Stéphane Lastère,François Simon,Vincent Meiffrédy,Raymond Césaire,Jean-Michel Molina,Ali Amara

doi:10.1371/journal.pone.0177882

Abstract

Given the possibility of yellow fever virus reintroduction in epidemiologically receptive geographic areas, the risk of vaccine supply disruption is a serious issue. New strategies to reduce the doses of injected vaccines should be evaluated very carefully in terms of immunogenicity. The plaque reduction test for the determination of neutralizing antibodies (PRNT) is particularly time-consuming and requires the use of a confinement laboratory. We have developed a new test based on the use of a non-infectious pseudovirus (WN/YF17D). The presence of a reporter gene allows sensitive determination of neutralizing antibodies by flow cytometry. This WN/YF17D test was as sensitive as PRNT for the follow-up of yellow fever vaccinees. Both tests lacked specificity with sera from patients hospitalized for acute Dengue virus infection. Conversely, both assays were strictly negative in adults never exposed to flavivirus infection or vaccination, and in patients sampled some time after acute Dengue infection. This WN/YF17D test will be particularly useful for large epidemiological studies and for screening for neutralizing antibodies against yellow fever virus.

Highlights

Preliminary results after one year of storage at -80 ̊C showed that this infectivity of virus-like particles (VLP) 2013 fell from 25% to 15%
Use of pseudovirus technology to produce VLPs capable of a single infective cycle is yielding diagnostic tools that avoid the need to work in a high-level confinement laboratory [22]
The preliminary results obtained here with WNV/YFV17D VLP, in which the West Nile virus envelope is replaced with a yellow fever virus envelope, allow us to propose an alternative method for the detection of yellow fever neutralizing antibodies

Summary

Introduction

Cerba laboratories just provide the financial support as Dr Poveda’s salaries and have no role in the study design and analysis or decision to Yellow fever virus is an extremely dangerous pathogen transmitted by Aedes and Haemagogus mosquitoes. Since its development in the 1930s, the live attenuated vaccine against yellow fever (AAV) has been widely used, and an estimated 60 million doses are administered each year [3].

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Conclusion