红球菌低分子量型腈水合酶的异源激活及激活子的结构域功能  

作　　者：王甜忆 程中一 郭军玲[1] 夏媛媛 刘中美[1] 周哲敏[1] Tianyi Wang;Zhongyi Cheng;Junling Guo;Yuanyuan Xia;Zhongmei Liu;Zhemin Zhou(Key Laboratory of Industrial Biotechnology(MOE),School of Biotechnology,Jiangnan University,Wuxi 214122,Jiangsu,China)

机构地区：[1]江南大学生物工程学院,工业生物技术教育部重点实验室,江苏无锡214122

出　　处：《生物工程学报》2020年第8期1578-1589,共12页Chinese Journal of Biotechnology

基　　金：国家自然科学基金(No.21878125);国家重点研发计划(Nos.2016YFE0127400,SQ2017YFGH001004)资助。

摘　　要：腈水合酶激活子具有亚基自身交换伴随子或者金属离子伴随子的功能,能够辅助腈水合酶摄取金属离子,对于腈水合酶的活性表达必不可少。与腈水合酶自身相比,激活子的序列保守性低,研究其激活作用的特点,探索其结构与功能之间的关系,对于理解腈水合酶的成熟机制具有重要意义。将红球菌Rhodococcus rhodochrous J1低分子量型腈水合酶L-NHase分别与4种异源激活子组合共表达,测定异源激活子对L-NHase的激活作用,进一步对激活子进行序列分析和结构模拟,并研究关键结构域的功能。结果表明,4种异源激活子均能激活L-NHase,但激活后L-NHase的比酶活存在差异,激活子A对L-NHase的激活程度最高,激活后的L-NHase比酶活为出发酶的97.79%;激活子G对L-NHase的激活程度最低,激活后的L-NHase比酶活为出发酶的23.94%。激活子E和激活子G具有保守结构域TIGR03889,缺失其中部分序列会使两者的激活作用基本丧失。将激活子G的N端序列替换为激活子E的N端序列,并将激活子E的C端序列添加至激活子G的C端,能够使L-NHase的比酶活提高178.40%。激活子的激活作用具有普遍性和特异性,其保守结构域对激活作用至关重要,同时N端结构域和C端结构域也对激活作用产生重要影响。As self-subunit swapping chaperones or metallochaperones,the activators assist nitrile hydratases to take up metal ions and they are essential for active expression of nitrile hydratases.Compared with nitrile hydratases,the activators have a low sequence identity.Study of the activation characteristics and the relationships between structures and functions of the activators is of great significance for understanding the maturation mechanism of nitrile hydratase.We co-expressed low-molecular-mass nitrile hydratase(L-NHase)from Rhodococcus rhodochrous J1 with four heterologous activators respectively and determined their activation abilities.Then we made sequence analysis and structure modelling,and studied the functions of the important domains of the activators.Results showed that all four heterologous activators could activate L-NHase,however,the specific activities of L-NHases were different after activation.L-NHase showed the highest specific activity after being activated by activator A,which was 97.79% of that of the original enzyme,but the specific activity of L-NHase after being activated by activator G was only 23.94% of that of the original enzyme.Activator E and activator G had conserved domains(TIGR03889),and deletion of their partial sequences resulted in a substantial loss of activation abilities for both activators.Replacing the N-terminal sequence of activator G with the N-terminal sequence of activator E,and adding the C-terminal sequence of activator E to the C-terminus of activator G could increase the specific activity of L-NHase by 178.40%.The activation by nitrile hydratase activators was universal and specific,and the conserved domains of activators were critical for activation,while the N-terminal domain and C-terminal domain also had important effects on activation.

关 键 词：腈水合酶 激活子 结构模拟 蛋白质结构域 

分 类 号：Q936[生物学—微生物学]