Cloning, protein expression and immunogenicity of HBs-murine IL-18 fusion DNA vaccine.

Channarong, Sunee; Mitrevej, Ampol; Sinchaipanid, Nuttanan; Usuwantim, Kanchana; Kulkeaw, Kasem; Chaicumpa, Wanpen

Cloning, protein expression and immunogenicity of HBs-murine IL-18 fusion DNA vaccine.

Date

2007-12-12

Authors

Channarong, Sunee

Mitrevej, Ampol

Sinchaipanid, Nuttanan

Usuwantim, Kanchana

Kulkeaw, Kasem

Chaicumpa, Wanpen

Abstract

Hepatitis B is a global serious disease caused by hepatitis B virus (HBV). There is no known cure for hepatitis B. The best way to deal with the disease is by preventing with hepatitis B vaccine. However, the current protein-based vaccines made up of recombinant hepatitis B surface antigen (HBsAg) are ineffective in chronic HBV carriers and a significant number of the vaccinees do not mount the protective immune response. Novel DNA-based immunization may overcome the deficits of the protein-based immunization and may provide more effective prophylactic and therapeutic outcomes. In this study, we constructed a recombinant plasmid carrying gene encoding the HBV surface antigen (HBs) linked to DNA segment encoding full-length murine interleukin-18, i.e. pcDNA-HBs-IL-18. Immunogenicity of the DNA construct was carried out in BALB/c mice in comparison with mock, i.e. pcDNA3.1+ and vaccines comprised of pRc/CMV-HBs and pRc/CMV-HBs plus pcDNA-IL-18. All vaccinated mice revealed significant serum anti-HBs IgG response after two intramuscular injections of the vaccines at 28 day interval as compared to the level of mock. Co-administration of pRc/CMV-HBs and pcDNA-IL-18 elicited arbitrarily higher levels of anti-HBs IgG than the levels in mice immunized with pRc/CMV-HBs alone and mice that received pcDNA-HBs-IL-18 although not statistically different. Further experiments are needed to investigate the subisotypes of the IgG antibody, the kinetics of cytokine and the cell-mediated immune response. For this communication, the prototype HBs-IL-18 DNA vaccine was successfully constructed and the gene encoding murine IL-18 was successfully cloned. The latter can be co-injected with the antigen coding DNA or used as a fusion partner to the DNA for priming the immune response. The recombinant HBs and full-length IL-18 proteins have potential for other research purposes. They may be used also as standard proteins in the protein quantification assay.

Description

Published by the Allergy and Immunology Society of Thailand.

Citation

Channarong S, Mitrevej A, Sinchaipanid N, Usuwantim K, Kulkeaw K, Chaicumpa W. Cloning, protein expression and immunogenicity of HBs-murine IL-18 fusion DNA vaccine. Asian Pacific Journal of Allergy and Immunology. 2007 Dec; 25(4): 233-42