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作 者:耿昭[1] 卞继峰[1] 于修平[1] 卢翌[1] 胡海燕[1] 王晓明[1]
机构地区:[1]山东大学医学院分子生物学实验室,山东济南250012
出 处:《山东大学学报(医学版)》2004年第4期384-386,共3页Journal of Shandong University:Health Sciences
基 金:国家自然科学基金资助项目(3017004530200245)
摘 要:目的:研制携带CMVie和NirB两种双启动子的DNA疫苗新型载体pCMVnir(pCN)。方法:设计细菌IVI启动子nirB,置换pTriEx鄄4中p10和T7lac启动子,获得pCN,将报告基因pEGFP鄄N1和pDsRed2鄄N1分别插入pCN构建成pCN鄄EGFP和pCN鄄DsRed两种报告质粒,转化减毒沙门菌SalmonellaSL3261和大肠杆菌DH5α;同时采Fugene脂质体,转染Hela细胞和前列腺细胞,检测pCN启动子的活性。结果:pCN的两个启动子都可高效转录和表达两种荧光报告基因,并且nirB是温和厌氧依赖性的。结论:成功构建了一种双启动子DNA疫苗表达载体pCN。Objective: To obtain a new dual-promoter DNA vaccine expression plasmid pCMVnir with in vivo-inducible bacterial CMVie and nirB promoters. Methods: Native nirB promoter was derived from E.coli, and a modified version of nirB promoter was designed and synthesized by deleting the nir-response element, whose activation depends on low-level of oxygen tension. In order to study the activity of these promoters, two different reporter genes EGFP-N1 and Ds-Red were inserted into the pCMVnir. Both pCN-EGFP and pCN-DsRed reporter plasmids were transfected into attenuated Salmonella and E.coli DH5to naked eyes. When the bacteria were cultured on the LB agar containing ampicillin, the colonies became lightly red and green. The expression strength of the reporter genes were confirmed by the flow cytometer, and the data indicated that nirB was activated at normal condition. Conclusion: The pCMVnir promoter could express antigens in vivo, and it is suitable for developing intracellular bacteria-based DNA vaccine, so it can express the antigen genes in both intracellular bacteria and mammalian cells, and has the capacity to enhance the immunogenicity of DNA vaccine.
分 类 号:R373.9[医药卫生—病原生物学] Q782[医药卫生—基础医学]
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