| Literature DB >> 27318415 |
Qingqing Xu1, Ning Cui2, Xingjiang Ma2, Fangkun Wang3, Hongmei Li3, Zhiqiang Shen4, Xiaomin Zhao5.
Abstract
The prokaryotic expressed recombinant chimeric multi-epitope protein X (rCMEPX) had been evaluated with good immunogenicity and protective efficacy against subgroup J avian leukosis virus (ALV-J) in our previous study. In the present research, we cloned the chimeric multi-epitope gene X into the eukaryotic expression vector pVAX1 to evaluate its potency as a DNA vaccine. The purified recombinant gp85 protein and rCMEPX were used as positive controls and a DNA prime-protein boost strategy was also studied. Six experimental groups of 7-day-old chickens (20 per group) were immunized intramuscularly three times at 2weeks interval with PBS, gp85, rCMEPX, pVAX1, pVAX-X and pVAX-X+rCMEPX respectively. The antibody titers and cellular immune responses were assayed after immunization. The efficacy of immunoprotection against the challenge of ALV-J NX0101 strain was also examined. The results showed that the DNA vaccine could elicit both neutralizing antibodies and cellular responses. Immune-challenge experiments showed good protection efficacy against ALV-J infection. Particularly, the regimen involving one priming pVAX-X and twice recombinant rCMEPX boosting, induced the highest antibody titers in all immunized groups. Our results suggest that the constructed chimeric multi-epitope DNA has potential for a candidate vaccine against ALV-J when used in proper prime-boost combinations. The data presented here may provide an alternative strategy for vaccine design in chicken ALV-J prevention.Entities:
Keywords: Cellular immune response; Multi-epitope DNA vaccine; Neutralizing antibodies; Prime-boost strategy; Subgroup J avian leukosis virus
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Year: 2016 PMID: 27318415 DOI: 10.1016/j.vaccine.2016.06.004
Source DB: PubMed Journal: Vaccine ISSN: 0264-410X Impact factor: 3.641