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作 者:孟莉[1] 韩保光[1] 马贤凯[1] 邹民吉[1] 凌世淦[1] 王嘉玺[1]
机构地区:[1]军事医学科学院基础医学研究所
出 处:《军事医学科学院院刊》1998年第4期260-264,312,共6页Bulletin of the Academy of Military Medical Sciences
摘 要:目的:构建具有λPR与T7双启动子的新型原核表达载体pDOG,以便使用同一载体研究不同诱导条件下,重组蛋白在大肠杆菌中表达、降解以及折叠的情况,从而选择最佳的诱导条件。方法:采用pBV220与pET-3表达载体作为原始材料,将pET-3上包括T7启动子与T7g-10翻译起始序列的一段序列克隆到pBV220载体λPR启动子的下游,构建了双启动子表达载体pDOG。结果:pDOG载体含有λPR与T7两个启动子,可以选择性地使用热诱导或在较低温度下使用化学诱导表达重组蛋白。该载体带有三个相位的多克隆位点,外源基因可以融合载体的少数几个氨基酸表达,也可以直接表达。该载体已成功地用于HIV-1核心蛋白、人IL-6等外源基因的高效表达。Objective: To construct novel E.coli expression vector that combines T7 and PR promoters for comparing degradation or refolding of the recombinant products under different induction conditions using the same vector. Methods: pBV220 And pET 3 are used as parent plasmids for the construction of the expression vector pDOG. This vector is generated by cloning the T7 g 10 leader sequence including T7 promoter and translation initiation region that is derived from pET 3 expression vector, downstream the λPR promoter of pBV220 vector. Results: pDOG Vector has PR and T7 promotes in tandem. Expression of foreign cDNA from the pDOG can be induced either by temperature induction, or by chemical induction at lower temperature. In addition, such vector contains multiple cloning sites where foreign cDNA can be inserted for expression as a fusion protein with 12 amino acids fused at its N terminus, and alternatively foreign gene can be cloned into NdeⅠ site for direct expression. The vector has been proved to be successful in over expression HIV 1 gag fragments and human IL 6. Conclusion: pDOG Vector has been demonstrated to be a valuable tool for optimizing expression of foreign gene in E.coli.
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