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嗜热甲烷栖热菌中2,3-环二磷酸甘油酸代谢关键酶——2,3-环二磷酸甘油酸合成酶编码基因的克隆、测序及表达

Cloning, sequencing, and expression of the gene encoding cyclic 2, 3-diphosphoglycerate synthetase, the key enzyme of cyclic 2, 3-diphosphoglycerate metabolism in Methanothermus fervidus.

作者信息

Matussek K, Moritz P, Brunner N, Eckerskorn C, Hensel R

机构信息

FB 9 Mikrobiologie, Universität GH Essen, D-45117 Essen, Germany.

出版信息

J Bacteriol. 1998 Nov;180(22):5997-6004. doi: 10.1128/JB.180.22.5997-6004.1998.

DOI:10.1128/JB.180.22.5997-6004.1998
PMID:9811660
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC107676/
Abstract

Cyclic 2,3-diphosphoglycerate synthetase (cDPGS) catalyzes the synthesis of cyclic 2,3-diphosphoglycerate (cDPG) by formation of an intramolecular phosphoanhydride bond in 2,3-diphosphoglycerate. cDPG is known to be accumulated to high intracellular concentrations (>300 mM) as a putative thermoadapter in some hyperthermophilic methanogens. For the first time, we have purified active cDPGS from a methanogen, the hyperthermophilic archaeon Methanothermus fervidus, sequenced the coding gene, and expressed it in Escherichia coli. cDPGS purification resulted in enzyme preparations containing two isoforms differing in their electrophoretic mobility under denaturing conditions. Since both polypeptides showed the same N-terminal amino acid sequence and Southern analyses indicate the presence of only one gene coding for cDPGS in M. fervidus, the two polypeptides originate from the same gene but differ by a not yet identified modification. The native cDPGS represents a dimer with an apparent molecular mass of 112 kDa and catalyzes the reversible formation of the intramolecular phosphoanhydride bond at the expense of ATP. The enzyme shows a clear preference for the synthetic reaction: the substrate affinity and the Vmax of the synthetic reaction are a factor of 8 to 10 higher than the corresponding values for the reverse reaction. Comparison with the kinetic properties of the electrophoretically homogeneous, apparently unmodified recombinant enzyme from E. coli revealed a twofold-higher Vmax of the enzyme from M. fervidus in the synthesizing direction.

摘要

环2,3 - 二磷酸甘油酸合成酶(cDPGS)通过在2,3 - 二磷酸甘油酸中形成分子内磷酸酐键来催化环2,3 - 二磷酸甘油酸(cDPG)的合成。已知在一些嗜热产甲烷菌中,cDPG作为一种假定的热适应剂在细胞内积累至高浓度(>300 mM)。我们首次从产甲烷菌——嗜热古菌嗜热栖热菌中纯化出活性cDPGS,对编码基因进行测序,并在大肠杆菌中表达。cDPGS的纯化得到了在变性条件下电泳迁移率不同的两种同工型酶制剂。由于这两种多肽显示出相同的N端氨基酸序列,并且Southern分析表明嗜热栖热菌中仅存在一个编码cDPGS的基因,所以这两种多肽源自同一基因,但因尚未确定的修饰而有所不同。天然cDPGS是一种表观分子量为112 kDa的二聚体,以ATP为代价催化分子内磷酸酐键的可逆形成。该酶对合成反应表现出明显的偏好:合成反应的底物亲和力和Vmax比逆反应的相应值高8至10倍。与来自大肠杆菌的电泳均一、明显未修饰的重组酶动力学性质比较表明,嗜热栖热菌的酶在合成方向上的Vmax高两倍。

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