Characterisation of antibody responses in pigs induced by recombinant oncosphere antigens fromTaenia solium

Recombinant antigens cloned from the oncosphere life cycle stage of the cestode parasiteTaenia solium(T. solium) have been proven to be effective as vaccines for protecting pigs against infections withT. solium.Previous studies have defined three different host protective oncosphere antigens, TSOL18...

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Veröffentlicht in:Vaccine 2012-12, Vol.30 (52), p.7475
Hauptverfasser: Jayashi, César M, Gonzalez, Armando E, Castillo Neyra, Ricardo, Kyngdon, Craig T, Gauci, Charles G, Lightowlers, Marshall W
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Sprache:eng
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Zusammenfassung:Recombinant antigens cloned from the oncosphere life cycle stage of the cestode parasiteTaenia solium(T. solium) have been proven to be effective as vaccines for protecting pigs against infections withT. solium.Previous studies have defined three different host protective oncosphere antigens, TSOL18, TSOL16 and TSOL45. In this study, we evaluated the potential for combining the antigens TSOL16 and TSOL18 as a practical vaccine. Firstly, in a laboratory trial, we compared the immunogenicity of the combined antigens (TSOL16/18) versus the immunogenicity of the antigens separately. Secondly, in a field trial, we tested the ability of the TSOL16/18 vaccine to induce detectable antibody responses in animals living under environmental stress and traditionally reared in areas whereT. soliumcysticercosis is endemic; and finally, we characterised the immune response of the study population. Pigs of 8-16 weeks of age were vaccinated with 200μg each of TSOL16 and TSOL18, plus 5mg of Quil-A. Specific total IgG, IgG1and IgG2antibody responses induced by TSOL16 and TSOL18 were determined with ELISA. The immunogenicity of both antigens was retained in the combined TSOL16/18 vaccine. The combined vaccine TSOL16/18 induced detectable specific anti-TSOL18 antibody responses in 100% (113/113) and specific anti-TSOL16 in 99% (112/113) of the vaccinated animals measured at 2 weeks following the booster vaccination. From the two IgG antibody subtypes analysed we found there was stronger response to IgG2.
ISSN:0264-410X
1873-2518
DOI:10.1016/j.vaccine.2012.10.057