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甘油醛-3-磷酸脱氢酶中配体诱导的顺序构象变化的结构证据。

Structural evidence for ligand-induced sequential conformational changes in glyceraldehyde 3-phosphate dehydrogenase.

作者信息

Leslie A G, Wonacott A J

出版信息

J Mol Biol. 1984 Sep 25;178(3):743-72. doi: 10.1016/0022-2836(84)90250-x.

DOI:10.1016/0022-2836(84)90250-x
PMID:6492162
Abstract

Glyceraldehyde 3-phosphate dehydrogenase is a tetramer of four chemically identical subunits which requires the cofactor nicotinamide adenine dinucleotide (NAD) for activity. The structure of the holo-enzyme from Bacillus stearothermophilus has recently been refined using X-ray data to 2.4 A resolution. This has facilitated the structure determination of both the apo-enzyme and the enzyme with one molecule of NAD bound to the tetramer. These structures have been refined at 4 A resolution using the constrained-restrained parameter structure factor least-squares refinement program CORELS. When combined with individual atomic temperature factors from the holo-enzyme, these refined models give crystallographic R factors of 30.2% and 30.4%, respectively, for data to 3 A resolution. The apo-enzyme has 222 molecular symmetry, and the subunit structure is related to that of the holo-enzyme by an approximate rigid-body rotation of the coenzyme binding domain by 4.3 degrees with respect to the catalytic domains, which form the core of the tetramer. The effect of this rotation is to shield the coenzyme and active site from solvent in the holo-enzyme. In addition to the rigid-body rotation, there is a rearrangement of several residues involved in NAD binding. The structure of the 1 NAD enzyme is asymmetric. The subunit which contains the bound NAD adopts a conformation very similar to that of a holo-enzyme subunit, while the other three unliganded subunits are very similar to the apo-enzyme conformation. This result provides unambiguous evidence for ligand-induced sequential conformational changes in B. stearothermophilus glyceraldehyde 3-phosphate dehydrogenase.

摘要

3-磷酸甘油醛脱氢酶是由四个化学性质相同的亚基组成的四聚体,其活性需要辅因子烟酰胺腺嘌呤二核苷酸(NAD)。嗜热栖热芽孢杆菌全酶的结构最近利用X射线数据精修至2.4埃分辨率。这有助于确定脱辅酶和四聚体结合一分子NAD的酶的结构。这些结构已使用约束-受限参数结构因子最小二乘精修程序CORELS在4埃分辨率下进行精修。当与全酶的单个原子温度因子结合时,这些精修模型对于3埃分辨率的数据分别给出了30.2%和30.4%的晶体学R因子。脱辅酶具有222分子对称性,亚基结构与全酶的亚基结构相关,辅酶结合结构域相对于形成四聚体核心的催化结构域通过约4.3度的近似刚体旋转。这种旋转的作用是在全酶中使辅酶和活性位点免受溶剂影响。除了刚体旋转外,参与NAD结合的几个残基也有重排。1 NAD酶的结构是不对称的。含有结合NAD的亚基采取的构象与全酶亚基的构象非常相似,而其他三个未结合配体的亚基与脱辅酶构象非常相似。这一结果为嗜热栖热芽孢杆菌3-磷酸甘油醛脱氢酶中配体诱导的顺序构象变化提供了明确证据。

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