土壤假单胞菌亚磷酸盐脱氢酶的基因克隆和原核表达及其酶活分析

doi:10.13560/j.cnki.biotech.bull.1985.2018-0250

生物技术通报 ›› 2018, Vol. 34 ›› Issue (8): 130-137.doi: 10.13560/j.cnki.biotech.bull.1985.2018-0250

土壤假单胞菌亚磷酸盐脱氢酶的基因克隆和原核表达及其酶活分析

袁航, 罗著, 杨玉梅, 刘延娟, 高艳秀, 刘娴, 龚明, 邹竹荣

云南师范大学生命科学学院云南省生物质能源和环境生物技术重点实验室教育部生物质能源持续发展和应用工程研究中心,昆明 650500

收稿日期:2018-03-21 出版日期:2018-08-26 发布日期:2018-09-04
作者简介:袁航,女,硕士研究生,研究方向：生物化学与分子生物学;E-mail：931124025@qq.com
基金资助:
国家自然科学基金项目（31460067,31760077）

Gene Cloning,Prokaryotic Expression and Enzymatic Analysis of the Phosphite Dehydrogenase from Soil Pseudomonas Species

YUAN Hang, LUO Zhu, YANG Yu-mei, LIU Yan-juan, GAO Yan-xiu, LIU Xian, GONG Ming, ZOU Zhu-rong

Engineering Research Center of Sustainable Development and Utilization of Biomass Energy（Ministry of Education）,Key Laboratory of Biomass Energy and Environmental Biotechnology of Yunnan Province,School of Life Sciences,Yunnan Normal University,Kunming 650500

Received:2018-03-21 Published:2018-08-26 Online:2018-09-04

摘要/Abstract

摘要： 亚磷酸盐脱氢酶（PTDH）以NAD⁺为辅助因子催化亚磷酸盐氧化生成正磷酸盐和NADH,在辅酶再生和基于亚磷酸盐的磷利用等方面有着潜在重大的应用价值。以土壤宏基因组DNA为模板,采用两轮PCR扩增得到全长亚磷酸盐脱氢酶基因PsPtx。通过酶切将它克隆到质粒pET32a（+）中,构建了原核表达载体pET（PsPtx）。序列分析表明,PsPtx基因的完整编码区大小为1 011 bp,其推导蛋白由336 个氨基酸组成,理论分子量大小为36.5 kD。保守结构域预测分析表明PsPtx编码蛋白属于亚磷酸盐脱氢酶,含有保守的NAD⁺结合基序和催化功能残基。系统进化树分析显示PsPtx基因来源于一无法确定种名的土壤假单胞菌。另外,PsPtx基因经IPTG诱导能在大肠杆菌BL21（DE3）中获得高效表达,重组PsPtx蛋白用组氨酸标签亲合层析纯化,其以亚磷酸钠盐为底物的酶比活性为3.75 U/mg。该PsPtx功能基因的获得为其后续应用研究打下了必要的基础。

关键词: 土壤假单胞菌, 亚磷酸盐脱氢酶, 基因克隆, 原核表达

Abstract: Phosphite dehydrogenase（PTDH）catalyzes the oxidation of phosphite to produce phosphate and NADH,using NAD⁺ as the cofactor. This enzyme is of large application potentials in the areas of coenzyme regeneration and phosphite-based phosphorus utilization,and etc. Herein,the full-length of a putative PTDH gene（PsPtx）was obtained by two rounds of PCR from the soil metagenome as DNA template,which was then subcloned into plasmid pET32a（+）by enzyme digestion to generate the prokaryotic expression vector pET（PsPtx）. Sequence analysis showed that the PsPtx gene had an entire coding region of 1 011 bp,encoding a protein of 336 aa and 36.5 kD. The results of the conserved domain prediction demonstrated that the deduced protein PsPtx was a member of the PTDH family,and had the conserved NAD⁺-binding motif as well as the crucial catalytic residues. Furthermore,phylogenetic analysis indicated that the PsPtx gene was originated from an undefined soil Pseudomonas species. In addition,PsPtx efficiently expressed in Escherichia coli strain BL21（DE3）by IPTG induction. The recombinant protein PsPtx was purified by His-tag affinity chromatography,and then detected to have a specific activity of 3.75 U/mg towards its substrate,sodium phosphite. Certainly,this cloned PsPtx gene with verified activity is of fundamental importance for its future application studies.

Key words: soil Pseudomonas species, phosphite dehydrogenase, gene cloning, prokaryotic expression

袁航, 罗著, 杨玉梅, 刘延娟, 高艳秀, 刘娴, 龚明, 邹竹荣. 土壤假单胞菌亚磷酸盐脱氢酶的基因克隆和原核表达及其酶活分析[J]. 生物技术通报, 2018, 34(8): 130-137.

YUAN Hang, LUO Zhu, YANG Yu-mei, LIU Yan-juan, GAO Yan-xiu, LIU Xian, GONG Ming, ZOU Zhu-rong. Gene Cloning,Prokaryotic Expression and Enzymatic Analysis of the Phosphite Dehydrogenase from Soil Pseudomonas Species[J]. Biotechnology Bulletin, 2018, 34(8): 130-137.

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土壤假单胞菌亚磷酸盐脱氢酶的基因克隆和原核表达及其酶活分析

Gene Cloning,Prokaryotic Expression and Enzymatic Analysis of the Phosphite Dehydrogenase from Soil Pseudomonas Species

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