稳定表达HBsAg的P815细胞株的建立及鉴定

目的:筛选并建立稳定表达亚洲人常见的adr亚型HBsAg的P815细胞株,为乙肝DNA疫苗的效果评价提供体外细胞感染模型.方法:用PCR方法扩增乙肝病毒的S基因片段后装入pcDNA3载体,并通过脂质体转染P815细胞,G418筛选.结果:构建了重组质粒pcDNA3-HBsAg(S),转染细胞及其培养上清中均可检测到HBsAg(S)的存在,PCR扩增也证实HBsAg(S)基因已稳定整合于P815细胞的染色体中.结论:获得了稳定表达HBsAg的P815细胞株,为今后在小鼠体内检测乙肝DNA疫苗激发的CTL反应奠定了基础.

Establishment and identification of P815 cell line stably expressing HBsAg

Objective: To screen for and establish P815 cell line stably expressing HBsAg (adr subtype) which is com-mon in Asian people, providing the cell infection model for evalution of the hepatitis B DNA vaccine effect in virto. Methods:S gene of hepatitis B virus was amplified and cloned into pcDNA3. The recombinant plasmid was transfected P815 by lipo-some and screened by G418. Results: Recombinant plasmid pcDNA3-HBsAg(S) coding hepatitis B (adr subtype) surface pro-tein S was constructed. HBsAg was detected both in the trans fected cell and its culture medium. It was confirmed by PCRthat HBsAg(S) gene was integrated into the chromosome of P8l5 stably. Conclusion: P815 cell line stably expressing HBsAgis obtained, providing bases for detecting the CTL reaction stimulated by hepatitis B DNA vaccine.