海栖热袍杆菌来源的极耐热碱性果胶裂解酶的表达纯化及定性.DOC

海栖热袍杆菌来源的极耐热碱性果胶裂解酶的表达、纯化及定性 李平1, 景庆庆1, 邵蔚蓝1,2 1 南京师范大学生命科学学院, 南京 2100462 江南大学生物工程学院, 无锡 214122 摘 要: 将来源于极端嗜热菌属海栖热袍杆菌Thermotoga maritima MSB8的编码碱性果胶裂解酶的结构基因pelA与新型热激质粒pHsh连接, 得到重组质粒pHsh-pelA, 运用mRNA二级结构预测软件对pHsh-pelA的翻译起始区的二级结构进行优化, 得到了具有最佳mRNA二级结构及自由能的质粒pHsh-pelC。将重组质粒pHsh-pelC转入大肠杆菌JM109(DE3)进行表达, 得到了一种极耐热性碱性果胶裂解酶(PelC)。对重组酶的酶学性质研究发现, 该酶的最适反应温度为90oC, 最适反应pH为8.5, 在pH 8.2~9.8之间酶活力稳定, 95oC酶活半衰期为2 h, 并且该酶依赖Ca2+作为活性离子。在工业生产常用温度60oC下, 该酶能够长时间保持稳定, 并具有较高的酶活力。以多聚半乳糖醛酸(PGA)为底物时, 其动力学参数Km值为0.11 mmol/L, Vmax值为327 U/mg。SDS结果显示该重组酶的分子量为43 kD, 与理论值相符。基于热激载体pHsh的重组表达系统具有诱导表达简便、诱导方式廉价的优点, 且重组酶热稳定性非常好, 这对该酶的大规模发酵应用具有重要意义。 关键词: 耐热碱性果胶裂解酶, 纯化定性, 热激载体 Expression, purification and characterization of athermostable pectate lyase from Thermotoga maritima Ping Li1, Qingqing Jing1, and Weilan Shao1,2 1 Department of Life Sciences, Nanjing Normal University, Nanjing 210046, China 2 School of Biotechnology, Jiangnan University, Wuxi 214122, China Abstract: The structure gene pelA from Thermotoga maritima MSB8 encoding pectate lyase was amplified and ligated into pHsh, resulting pHsh-pelA. Through structural optimization on pHsh-pelA, the ultimate plasmid, pHsh-pelC, which possessed the most appropriate structure and free energy of mRNA, was obtained. Pectate lyase C (PelC) was obtained after expressing pHsh-pelC in Escherichia coli JM109. The optimum activity of PelC was determined at pH 8.5 at 90oC, with a half-life for almost 2 h at 95oC. PelC was stable at the pH range of 8.2?9.8, and was dependent on Ca2+ for activity and stability. The enzyme kept stable for a long time and possessed a high level of activity at 60oC. The kinetic assay using polygalacturonic acid (PGA) as substrate gave Km and Vmax of 0.11 mmol/L and 327 U per mg of protein. SDSanalysis showed that the molecular mass of the expressed recombinant PelC was about 43 kD, which was exactly the size predicted. The expression vector system of the heat shock plasm