毛白杨4-香豆酸：辅酶A连接酶可溶性原核表达及活性检测

Shaocai Li,Wenhui Chen,Bingyou Fan,Jiaojun Zhu,Xiaojuan Jin,Jinshu Shi,Jianxiong Lu,Mingpu Di,Xiaoli Hu,lishidong,sunxiaomei,Yujie Wang,Jun Gao,Wei Tan,Junxia Dou,xiaoshengchun,lifadong,Zhende Yang,Cunde Pan,yanrong,Nanhai Long,Bingyu Zhang,Shuangmin Xu,Yuqing Zhang,zhouchunjiang,Hongzhang Kang,Zhongke Feng,Yimin Xie,zhangyiping,sannai,mengping,hanhairong,lijianzhang,Hongxia Liu,Xiaoqing Tian,sunhailong,Shougong Zhang,liujunchang,Ruifeng Shi,luoxiuqin,Yunqi Wang,Qingke Zhu,songxianfang,Shiyu Hu,suxiaohua,xiaohonglang,caihuai,yueliangsong,wangxiaoshan,Bin Wu,Hai Lu,Qinyan Ma,Yiliang Li,Boguang Zhao,Wei Jiang,yangzhirong,Yan Zhang,Wenrui Zhou,Jiali Jiang,liuchangming,Shi Qi,Shuangju Zhao,Zhihui Li,Lei He,zhangjingsong,pujunwen,zhangyongan,Qinghai Song,jiangxiangning,Youke Zhao,Lita Yi,Jinzhao Zhu,yaoshan,Song Ge,Liwang Qi,zhangderong,Yan Zhang,Jingjie Yu,liuyuan,Jianmin Chu,Liping Shi,Cong Yang,Shoufang Lu,wuqingli,Liangjian Qu,Fengfeng Kang,Chaode Ma,cuibaoshan,Xinyu Liu,Yuzhu Wang,wangjianhua,Linfeng Zhu,Xiangchao Liu,Kun Hu,Yingchuan Tian,tou tune gen

毛白杨4-香豆酸：辅酶A连接酶可溶性原核表达及活性检测

2006

为了进一步研究毛白杨4CL1的酶学特性，构建了毛白杨4CL1原核表达载体pQE31-4CL1．经IPTG诱导在大肠杆菌中表达了毛白杨4CL1蛋白，SDS-PAGE电泳分析表明该新蛋白的分子量为60kD，与预测值一致．对毛白杨4CL1蛋白在大肠杆菌中的表达体系进行了优化，确定IPTG的最佳浓度为0．4mmol／L，诱导时的菌液密度OD600为0．3-0．5，最佳表达时间为2h．37℃下表达的4CL1融合蛋白以包涵体的形式存在，没有生物学活性．当表达温度从37℃降低为28℃时，可溶性的有生物学活性的毛白杨4CL1蛋白诱导表达获得成功，表达量达11％．以耦联有Ni^2＋-NTA的琼脂糖为亲和层析填料，金属鳌合亲和柱层析一步纯化获得了电泳纯4CL1蛋白，4CL1蛋白对5种底物的比活性分别为：4-香豆酸3949．0pkat／mg，咖啡酸2214．0pkat／mg，阿魏酸715．0pkat／mg，肉桂酸84．9pkat／mg，而对芥子酸没有生物活性．

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