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酿酒酵母中咪唑甘油磷酸合酶的表达与纯化

Expression and purification of imidazole glycerol phosphate synthase from Saccharomyces cerevisiae.

作者信息

Chittur S V, Chen Y, Davisson V J

机构信息

Department of Medicinal Chemistry, Purdue University, West Lafayette, Indiana, 47907, USA.

出版信息

Protein Expr Purif. 2000 Apr;18(3):366-77. doi: 10.1006/prep.2000.1207.

DOI:10.1006/prep.2000.1207
PMID:10733892
Abstract

Imidazole glycerol phosphate (IGP) synthase is a glutamine amidotransferase that catalyzes the formation of IGP and 5-aminoimidazole-4-carboxamide ribonucleotide (AICAR) from N(1)-[(5'-phosphoribulosyl)formimino]-5-aminoimidazole-4-car boxamide ribonucleotide (PRFAR). This enzyme represents a junction between histidine biosynthesis and de novo purine biosynthesis. The recent characterization of the HIS7 gene in the yeast Saccharomyces cerevisiae IGP synthase established that this protein is bifunctional, representing a fusion between the N-terminal HisH domain and a C-terminal HisF domain. Catalytically active yeast HIS7 was expressed in a bacterial system under the control of T7 polymerase promoter. The recombinant enzyme was purified to homogeneity and the native molecular weight and steady-state kinetic constants were determined. The yeast enzyme is distinguished from the Escherichia coli IGP synthase in its utilization of ammonia as a substrate. HIS7 displays a higher K(m) for glutamine and a lower turnover in the ammonia-dependent IGP synthase activity. As observed with the E. coli IGP synthase, HIS7 shows a low basal level glutaminase activity that can be enhanced 1000-fold in the presence of a nucleotide substrate or analog. The purification and characterization of the S. cerevisiae enzyme will enable a more detailed investigation of the biochemical mechanisms that mediate the ammonia-transfer process. The fused structural feature of the HIS7 protein and the development of a high-level production system for the active enzyme elevate the potential for determination of its three-dimensional structure through X-ray crystallography.

摘要

咪唑甘油磷酸(IGP)合酶是一种谷氨酰胺酰胺转移酶,它催化从N(1)-[(5'-磷酸核糖基)甲亚胺基]-5-氨基咪唑-4-甲酰胺核糖核苷酸(PRFAR)形成IGP和5-氨基咪唑-4-甲酰胺核糖核苷酸(AICAR)。这种酶代表了组氨酸生物合成和嘌呤从头生物合成之间的连接点。酿酒酵母IGP合酶中HIS7基因的最新特征表明,该蛋白具有双功能,代表N端HisH结构域和C端HisF结构域的融合。具有催化活性的酵母HIS7在T7聚合酶启动子的控制下在细菌系统中表达。重组酶被纯化至同质,并测定了其天然分子量和稳态动力学常数。酵母酶在利用氨作为底物方面与大肠杆菌IGP合酶不同。HIS7在依赖氨的IGP合酶活性中对谷氨酰胺表现出更高的K(m)值和更低的周转率。正如在大肠杆菌IGP合酶中观察到的那样,HIS7显示出低基础水平的谷氨酰胺酶活性,在核苷酸底物或类似物存在下可提高1000倍。酿酒酵母酶的纯化和表征将有助于更详细地研究介导氨转移过程的生化机制。HIS7蛋白的融合结构特征以及活性酶的高水平生产系统的开发提高了通过X射线晶体学确定其三维结构的可能性。

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