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Thanatin突变体在大肠杆菌中的表达及纯化

Journal of Southeast University(Medical Science Edition)(2007)

Cited 4|Views6
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Abstract
目的:在大肠杆菌中克隆表达thanatin突变体(Th-T)蛋白并纯化. 方法:PCR合成Th-T基因并克隆到pET32a载体的BamHⅠ和XhoⅠ酶切位点之间,构建Th-T原核表达载体(pET32a-Th-T)并转化到大肠杆菌BL21融合表达,通过正交实验优化表达条件,His-Bind介质纯化.考察经酶切纯化后的重组Th-T对4种供试菌的最低抑制浓度.结果:菌体在LB培养基(pH 6.5)培养4.5 h,IPTG 0.4 mmol·L-1诱导7 h,Th-T融合蛋白大量可溶性表达,经药敏试验证明纯化的重组Th-T具有预期的抗菌活性.结论:本研究为通过大肠杆菌体系表达重组Th-T抗菌药物奠定了基础.
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Key words
expression,chemosensitivity,fusion protein,Escherichia coli,purification,mutant,thanatin
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