Failure of a recombinant Babesia bovis antigen to protect cattle against heterologous strain challenge

Groups of cattle were inoculated subcutaneously with (i) a recombinant DNA-derived Babesia bovis protein (KaBbl-GZ) fused to β-galactosidase and combined with adjuvants, or (ii) native β-galactosidase (GZ) plus adjuvant, or (iii) adjuvant only or (iv) a live, attenuated B bovis vaccine. KaBbl-GZ was...

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Veröffentlicht in:Research in veterinary science 1988-09, Vol.45 (2), p.267-269
Hauptverfasser: TIMMS, P., BARRY, D.N., GILL, A.C., SHARP, P.J., DE VOS, A.J.
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Sprache:eng
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Zusammenfassung:Groups of cattle were inoculated subcutaneously with (i) a recombinant DNA-derived Babesia bovis protein (KaBbl-GZ) fused to β-galactosidase and combined with adjuvants, or (ii) native β-galactosidase (GZ) plus adjuvant, or (iii) adjuvant only or (iv) a live, attenuated B bovis vaccine. KaBbl-GZ was produced in the λ gt11-amp3 system as a 5-10 kD babesial polypeptide linked to GZ. KaBbl has previously been shown to be an immunodominant antigen of B bovis, localised at the apex of the parasite, and present in a range of B bovis strains. High levels of GZ antibodies were observed in KaBbl-GZ and GZ inoculated cattle, but specific KaBbl antibodies could not be detected by klisa. Five months after primary inoculation, all cattle were blood challenged with a virulent heterologous B bovis strain. Despite four inoculations with KaBbl-GZ, significant protection against the challenge was not observed.
ISSN:0034-5288
1532-2661
DOI:10.1016/S0034-5288(18)30947-0