HIV-1 HXB2株Tat半胱氨酸富集区N端移位突变体的构建及在大肠杆菌中的高效表达  

作　　者：李存枚[1] 潘卫[2] 曹洁[2] 王锦红[2] 黄德圣[1] 庞强[2] 廖文婷[2] 邓松华[1] 

机构地区：[1]安徽医科大学病理生理学教研室,合肥230032 [2]第二军医大学微生物学教研室,上海200433

出　　处：《安徽医科大学学报》2009年第1期5-9,共5页Acta Universitatis Medicinalis Anhui

基　　金：国家自然科学基金资助项目(编号:30872246,30872405);上海市基础研究重点项目(编号:08JC1405200);国家“863”项目(编号:2006AA02A238);安徽省自然科学基金项目(编号:080413136)

摘　　要：目的构建HIV-1HXB2株Tat半胱氨酸富集区N端移位突变体,并在大肠杆菌E.coliBL21(DE3)中进行高效表达和纯化。方法应用PCR拼接的方法将首轮合成Tat基因的半胱氨酸富集区(64～111位核苷酸,22～37位氨基酸)移位至缺失半胱氨酸富集区的Tat(△C)的N末端,获得其突变体序列(Tat(CN)DNA),构建其原核表达质粒pET32a-Tat(CN),并转入大肠杆菌E.coli BL21(DE3)中进行诱导表达及纯化,经SDS-PAGE鉴定表达及纯化产物,纯化后的产物用间接ELISA进行鉴定。结果构建了pET32a-Tat(CN)突变体,pET32a-Tat(CN)融合蛋白在大肠杆菌中表达水平为5.17mg/ml,相对分子质量为31ku。间接的ELISA结果表明,pET32a-Tat(CN)能与Tat兔抗血清呈特异反应。结论成功构建了HIV-1 HXB2株Tat半胱氨酸富集区移位至TatN端的突变体,并能在大肠杆菌中高效表达,其纯化的蛋白pET32a-Tat(CN)很好地保留了与HIV-1Tat兔抗血清的免疫反应性,为HIV-1Tat的疫苗基础研究提供了一有价值的研究结论。Objective To construct mutant of HIV-1 HXB2 subtype Tat which shifted the cysteine-rich region to N terminal, and to effectively express and purify the mutant protein in E. coli BL21 （DE3）. Methods Tat mutant DNA shifted the eysteine-rich region （64-111 nucleotides, 22-37 amino acids） to N-terminal of Tat deleting the cysteine-rich region Tat（/XC）, named as Tat （CN） DNA, was obtained by PCR and cloned into pET32a vector. pET32a-Tat （CN） plasmid was established and transformed into E. coli BL21 （DE3） strains. The expressed and purified pET32a-Tat （CN） protein was analyzed by SDS-PAGE, then testified the reactivity of the purified protein by indirect ELISA. Results The mutant of pET32a-Tat （CN） was established, the dense of the purified fusion protein pET32a-Tat （CN） was 5.17 mg/ml expressed in E. coli BL21 （DE3） , and the relative molecular mass of the protein was 31 ku. Indirect ELISA showed that anti-sera of pET32a-Tat protein from rabbit could react specifically with pET32a-Tat （CN） protein and pET32a-Tat protein, and titers of the sera were 1 ： 128 000 and 1：64 000 respectively. The reaction of the sera with pET32a protein was rather weak. Conclusion The recombinant mutant of HIV-1 HXB2 subtype Tat which shift the cysteine-rich region to N terminal is successfully established, and expressed efficiently in E. coli. The purified pET32a-Tat （CN） protein remains good antigenicity with the anti-sera of pET32a-Tat protein from rabbit. The results provide a valuable conclusion for further development of HIV-1 Tat vaccine.

关 键 词：HIV-1/遗传学 大肠杆菌/遗传学 基因产物 TAT 基因表达 

分 类 号：R373.51[医药卫生—病原生物学] R378.2[医药卫生—基础医学]