| Literature DB >> 28214171 |
Martine Chabaud-Riou1, Nadège Moreno1, Fabien Guinchard1, Marie Claire Nicolai1, Elisabeth Niogret-Siohan1, Nicolas Sève1, Catherine Manin2, Françoise Guinet-Morlot1, Patrice Riou1.
Abstract
The NIH test is currently used to assess the potency of rabies vaccine, a key criterion for vaccine release. This test is based on mice immunization followed by intracerebral viral challenge. As part of global efforts to reduce animal experimentation and in the framework of the development of Sanofi Pasteur next generation, highly-purified vaccine, produced without any material of human or animal origin, we developed an ELISA as an alternative to the NIH test. This ELISA is based on monoclonal antibodies recognizing specifically the native form of the viral G-protein, the major antigen that induces neutralizing antibody response to rabies virus. We show here that our ELISA is able to distinguish between potent and different types of sub-potent vaccine lots. Satisfactory agreement was observed between the ELISA and the NIH test in the determination of the vaccine titer and their capacity to discern conform from non-conform batches. Our ELISA meets the criteria for a stability-indicating assay and has been successfully used to develop the new generation of rabies vaccine candidates. After an EPAA international pre-collaborative study, this ELISA was selected as the assay of choice for the EDQM collaborative study aimed at replacing the rabies vaccine NIH in vivo potency test.Entities:
Keywords: ELISA; G-protein; In-process control; NIH test; Rabies vaccine; Release test
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Year: 2017 PMID: 28214171 DOI: 10.1016/j.biologicals.2017.02.002
Source DB: PubMed Journal: Biologicals ISSN: 1045-1056 Impact factor: 1.856