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大肠杆菌K-12中吡哆醇(吡哆胺)5'-磷酸氧化酶的动力学限制和细胞数量

Kinetic limitation and cellular amount of pyridoxine (pyridoxamine) 5'-phosphate oxidase of Escherichia coli K-12.

作者信息

Zhao G, Winkler M E

机构信息

Department of Microbiology and Molecular Genetics, University of Texas, Houston Medical School 77030.

出版信息

J Bacteriol. 1995 Feb;177(4):883-91. doi: 10.1128/jb.177.4.883-891.1995.

Abstract

We report the purification and enzymological characterization of Escherichia coli K-12 pyridoxine (pyridoxamine) 5'-phosphate (PNP/PMP) oxidase, which is a key committed enzyme in the biosynthesis of the essential coenzyme pyridoxal 5'-phosphate (PLP). The enzyme encoded by pdxH was overexpressed and purified to electrophoretic homogeneity by four steps of column chromatography. The purified PdxH enzyme is a thermally stable 51-kDa homodimer containing one molecule of flavin mononucleotide (FMN). In the presence of molecular oxygen, the PdxH enzyme uses PNP or PMP as a substrate (Km = 2 and 105 microM and kcat = 0.76 and 1.72 s-1 for PNP and PMP, respectively) and produces hydrogen peroxide. Thus, under aerobic conditions, the PdxH enzyme acts as a classical monofunctional flavoprotein oxidase with an extremely low kcat turnover number. Comparison of kcat/Km values suggests that PNP rather than PMP is the in vivo substrate of E. coli PdxH oxidase. In contrast, the eukaryotic enzyme has similar kcat/Km values for PNP and PMP and seems to act as a scavenger. E. coli PNP/PMP oxidase activities were competitively inhibited by the pathway end product, PLP, and by the analog, 4-deoxy-PNP, with Ki values of 8 and 105 microM, respectively. Immunoinhibition studies suggested that the catalytic domain of the enzyme may be composed of discontinuous residues on the polypeptide sequence. Two independent quantitation methods showed that PNP/PMP oxidase was present in about 700 to 1,200 dimer enzyme molecules per cell in E. coli growing exponentially in minimal medium plus glucose at 37 degrees C. Thus, E. coli PNP/PMP oxidase is an example of a relatively abundant, but catalytically sluggish, enzyme committed to PLP coenzyme biosynthesis.

摘要

我们报道了大肠杆菌K-12中吡哆醇(吡哆胺)5'-磷酸(PNP/PMP)氧化酶的纯化及酶学特性,该酶是必需辅酶磷酸吡哆醛(PLP)生物合成中的关键限速酶。由pdxH编码的酶通过四步柱层析进行过表达并纯化至电泳纯。纯化后的PdxH酶是一种热稳定的51 kDa同型二聚体,含有一分子黄素单核苷酸(FMN)。在分子氧存在下,PdxH酶以PNP或PMP为底物(PNP和PMP的Km分别为2和105 μM,kcat分别为0.76和1.72 s-1)并产生过氧化氢。因此,在有氧条件下,PdxH酶作为一种典型的单功能黄素蛋白氧化酶,其kcat周转数极低。kcat/Km值的比较表明,PNP而非PMP是大肠杆菌PdxH氧化酶的体内底物。相比之下,真核酶对PNP和PMP的kcat/Km值相似,似乎起着清除剂的作用。大肠杆菌PNP/PMP氧化酶的活性受到途径终产物PLP和类似物4-脱氧-PNP的竞争性抑制,Ki值分别为8和105 μM。免疫抑制研究表明,该酶的催化结构域可能由多肽序列上不连续的残基组成。两种独立的定量方法显示,在37℃于添加葡萄糖的基本培养基中指数生长的大肠杆菌中,每细胞约有700至1200个二聚体酶分子存在PNP/PMP氧化酶。因此,大肠杆菌PNP/PMP氧化酶是一种相对丰富但催化缓慢的、参与PLP辅酶生物合成的酶的例子。

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