猪cGAS基因的克隆与原核表达

doi:10.3864/j.issn.0578-1752.2016.09.016

摘要/Abstract

摘要： 【目的】环磷酸鸟苷-腺苷酸合成酶(cyclic guanosine monophosphate-adenosine monophosphate synthase, cGAS)是近期在哺乳动物细胞中发现的一种新型核酸转移酶，能够识别胞质DNA，催化ATP和GTP生成第二信使cGAMP，继而通过STING依赖的方式活化转录因子IRF3，启动机体固有免疫。通过构建含猪cGAS基因的重组质粒pBbB3a-His6-NusA-cGAS，进行原核表达，得到cGAS蛋白，为进行体外催化合成cGAMP及探讨其在天然免疫过程中的作用奠定基础。【方法】以猪脾脏cDNA为模板克隆猪cGAS的蛋白编码区 (open reading frame, ORF)，用非酶连接技术将此基因克隆至丙酸诱导型原核表达载体pBbB3a-His6-NusA-LIC中。菌液PCR进行阳性克隆鉴定并测序。将测序鉴定正确的克隆菌液提取质粒，转化至E.coli BL21 (DE3)中。当细菌生长到对数期时，丙酸钠诱导表达His6-NusA-cGAS融合蛋白，用20 mmol·L^-1丙酸钠在20℃，180 r/min分别诱导0, 2, 4, 6, 8, 10 h，以确定最佳诱导时间；然后，分别用0, 5, 10, 15, 20, 25, 30, 35, 40, 45 mmol·L^-1的丙酸钠在20℃，180 r/min诱导6 h，以确定最佳诱导丙酸钠诱导浓度；另外，分别在20℃，30℃，37℃条件下用20 mmol·L^-1丙酸钠，180 r/min培养6 h，以确定最佳诱导温度。筛选最佳诱导条件，并用SDS-PAGE和Western blotting进行鉴定。【结果】（1）本试验成功克隆了猪cGAS基因，其ORF长度为1 494 bp；（2）构建了cGAS丙酸诱导型原核表达载体pBbB3a-His6-NusA-cGAS；（3）His6-NusA-cGAS融合蛋白在37℃，添加20 mmol·L^-1丙酸钠，诱导6 h时表达量最高。（4）His6-NusA-cGAS融合蛋白在裂解菌液的上清和沉淀中均有表达，相对分子质量为111.87 kD。【结论】运用大肠杆菌表达系统成功表达了cGAS融合蛋白，本试验为体外表达cGAS融合蛋白提供技术方法。

关键词: 猪cGAS, 非酶连接, 丙酸诱导, 原核表达

Abstract: 【Objective】cGAS (cyclic guanosine monophosphate-adenosine monophosphate synthase), as a new type of nucleic transferase was found in mammalian cells recently. It can identify cytoplasmic DNA and catalyse ATP and GTP to generate the second messenger cGAMP, cGAMP binds to STING by dependent way, leading to activate transcription factor IRF3. Then the inherent immunity was starting. This experiment was conducted to construct a prokaryotic expression plasmid, pBbB3a-His6-NusA- cGAS, containing porcine cGAS gene. The gene expression was induced in E. coli, and the cGAS protein was obtained. Then a foundation of the research on the synthesis of cGAMP in vitro and its function in innate immune progress was made.【Method】 The open reading frame (ORF) of cGAS was amplified from the cDNA of porcine spleen, and cloned it into propionate inducible plasmid pBbB3a-His6-NusA-LIC by ligation-independent cloning (LIC) technology. Identification of individual clone was performed by bacteria liquid PCR followed by DNA sequencing. Plasmids were extracted from the confirmed bacteria and transformed into E.coli BL21 (DE3). When the bacteria grew to logarithmic phase, sodium propionate was used to induce the expression of His6-NusA- cGAS fusion protein, 20 mmol·L^-1 sodium propionate at 20℃, 180 r/min were induced by 2 h, 4 h, 6 h, 8 h, 10 h and 0 h, then the optimal induction time was determined. Sodium propionate at 0, 5, 10, 15, 20, 25, 30, 35, 40 and 45 mmol·L^-1, respectively, and at 20℃, 180 r/min induced for 6 h to determine the best induction concentration of sodium propionate. Under the conditions of 20, 30 and 37℃, 20 mmol·L^-1 sodium propionate was used at 180 r/min to cultivate for 6 h to determine the best temperature induction. The His6-NusA-cGAS fusion protein was induced by sodium propionate and identified by SDS-PAGE and Western Blot. 【Result】 (1) Porcine cGAS gene’ORF, which is 1 494 bp in length, was successfully cloned; (2) The propionate inducible plasmid pBbB3a-His6-NusA-cGAS was constructed; (3) At 37℃, 20 mmol·L^-1 sodium propionate to induce for 6 h, the His6-NusA-cGAS fusion protein’s expression amount was the highest. (4) His6-NusA-cGAS fusion protein was efficiently expressed in soluble form with a molecular weight of about 111.87 kD.【Conclusion】 These results indicate that cGAS fusion protein was successfully expressed in E.coli BL21 (DE3) and this will provide technology and methods for cGAS’s fusion protein expression in vitro.

Key words: porcine cGAS, ligation-independent cloning, propionate induction, prokaryotic expression

杜丽丽，樊爽爽，李赛赛，陈佩格，陈磊，孙士平，樊文杰，王江，王月影，钟凯. 猪cGAS基因的克隆与原核表达[J]. 中国农业科学, 2016, 49(9): 1803-1809.

DU Li-li, FAN Shuang-shuang, LI Sai-sai, CHEN Pei-ge, CHEN Lei, SUN Shi-ping, FAN Wen-jie, WANG Jiang, WANG Yue-ying, ZHONG Kai. Cloning and Prokaryotic Expression of Porcine cGAS Gene[J]. Scientia Agricultura Sinica, 2016, 49(9): 1803-1809.

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