Detection of neutralizing antibodies against Bluetongue virus serotype 8 by an optimized plasma neutralization test.

Abstract

The neutralization test is used commonly for quantifying neutralizing antibodies and for distinguishing among different virus serotypes (serotyping). Due to the co-circulation of multiple serotypes of Bluetongue virus (BTV), the neutralization test has become an important surveillance method in Europe. However, the existence of different protocols makes test standardization and interpretation of results difficult. The current paper describes the development of a neutralization test using plasma and addresses the factors critical for detection of neutralizing antibodies against BTV serotype 8 (BTV-8), such as virus propagation, stability of virus infectivity and origin of the BTV-8 strain. The results indicated that animals exposed to the Northern European BTV-8 strain developed low neutralizing antibody titers, particularly after vaccination and experimental infection. Although clearly ELISA-positive, these samples often yielded false negative results when tested by the neutralization test using the OIE recommended virus concentration of 100 TCID₅₀/50 μl. The sensitivity of the neutralization test could be improved significantly with retained specificity by using a reduced TCID₅₀ and the homologous European BTV-8 strain instead of the South African reference strain.