Basic Research
Copyright ©The Author(s) 2004. Published by Baishideng Publishing Group Inc. All rights reserved.
World J Gastroenterol. Jul 15, 2004; 10(14): 2072-2077
Published online Jul 15, 2004. doi: 10.3748/wjg.v10.i14.2072
Contribution of C3d-P28 repeats to enhancement of immune responses against HBV-preS2/S induced by gene immunization
Li-Xin Wang, Wei Xu, Qing-Dong Guan, Yi-Wei Chu, Ying Wang, Si-Dong Xiong
Li-Xin Wang, Wei Xu, Qing-Dong Guan, Yi-Wei Chu, Ying Wang, Si-Dong Xiong, Department of Immunology, Shanghai Medical College of Fudan University, 138 Yi Xue Yuan Road, Shanghai 200032, China
Li-Xin Wang, Department of Microbiology and Immunology, School of Basic Medical Science of Southeast University, 87 Ding Jia Qiao Road, Nanjing 210009, Jiangsu Province, China
Author contributions: All authors contributed equally to the work.
Supported by the Major State Basic Research Development Program of China, No. 2001CB510006; National Science Found for Distinguished Young Scholars from NSFC, No. 39925031 and Key Research Program of STCSM, No. 03DZ19229
Correspondence to: Dr. Si-Dong Xiong, Department of Immunology, Shanghai Medical College of Fudan University, 138 Yi Xue Yuan Road, Shanghai 200032, China. sdxiong@shmu.edu.cn
Telephone: +86-21-54237749 Fax: +86-21-54237749
Received: December 10, 2003
Revised: January 13, 2004
Accepted: February 1, 2004
Published online: July 15, 2004
Abstract

AIM: To investigate whether P28 derived from C3d can enhance the immune response to HBV-preS2/S induced by directly injection of naked plasmids containing variable repeats of P28 and HBV-preS2/S in fusion form.

METHODS: One to four copies of C3d-P28 coding gene, amplified by PCR and modified by restriction endonucleases digestion, were subcloned into a eukaryotic expression vector pVAON33 to construct pVAON33-P28, pVAON33-P28.2, pVAON33-P28.3 and pVAON33-P28.4 (pVAON33-P28.[1-4]). HBV-preS2/S coding sequence was then introduced into the pVAON33-P28.[1-4] and identified by both PCR and DNA sequencing. BALB/c mice were primed by intramuscular gene immunization with 100 μg different recombinant plasmids on day 0 and were boosted by subcutaneous inoculation with HBsAg protein (1 μg) 12 wk post-priming. The levels and avidity of specific IgG in sera collected at the indicated times from each group were determined by ELISA and NaSCN-displacement ELISA, respectively.

RESULTS: HBsAg specific antibody response was elicited in groups primed with plasmids pVAON33-S2/S-P28.[1-4] and pVAON33-S2/S. However, the response against HBsAg in the groups primed with pVAON33-S2/S-P28.[1-4] was significantly higher than that in pVAON33-S2/S group, the highest level of the specific antibody response was observed in the groups primed with pVAON33-S2/S-P28.4 (P < 0.01). After secondary immunization with specific antigen, the acceleration of antibody levels was significantly higher and faster in the mice primed with DNA expressing preS2/S-P28 fusions than that with DNA expressing preS2/S only (P < 0.05). Interestingly, mice primed with DNA expressing preS2/S-P28.4 fusions maintained the highest levels of anti-HBs antibodies in all animals. The avidity assay showed that the avidity index (AI) collected at 18 wk from mice primed with pVAON33-S2/S-P28.3 and pVAON33-S2/S-P28.4 were significantly higher than that from preS2/S-DNA vaccinated mice (P < 0.01).

CONCLUSION: Different repeats of C3d-P28 can enhance both humoral immune response and avidity maturation of specific antibodies induced by gene immunization, in which four copies of C3d-P28 may be necessary to achieve the most modest antibody response.

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