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红螺菌中1,5-二磷酸核酮糖羧化酶在1.7埃分辨率下的晶体学精修与结构

Crystallographic refinement and structure of ribulose-1,5-bisphosphate carboxylase from Rhodospirillum rubrum at 1.7 A resolution.

作者信息

Schneider G, Lindqvist Y, Lundqvist T

机构信息

Swedish University of Agricultural Sciences, Uppsala Biomedical Centre, Department of Molecular Biology.

出版信息

J Mol Biol. 1990 Feb 20;211(4):989-1008. doi: 10.1016/0022-2836(90)90088-4.

DOI:10.1016/0022-2836(90)90088-4
PMID:2107319
Abstract

The amino acid sequence of ribulose-1,5-bisphosphate carboxylase/oxygenase from Rhodospirillum rubrum has been fitted to the electron density maps. The resulting protein model has been refined to a nominal resolution of 1.7 A using the constrained-restrained least-squares refinement program of Sussman and the restrained least-squares refinement program of Hendrickson & Konnert. The crystallographic refinement, based on 76,452 reflections with F greater than sigma (F) in the resolution range 5.5 to 1.7 A resulted in a crystallographic R-factor of 18.0%. The asymmetric unit contains one dimeric ribulose-1,5-biphosphate carboxylase molecule, consisting of 869 amino acid residues and 736 water molecules. The geometry of the refined model is close to ideal, with root-mean-square deviations of 0.018 A in bond lengths and 2.7 degrees in bond angles. Two loop regions, comprising residues 54 to 63 and 324 to 335, and the last ten amino acid residues at the C terminus are disordered in our crystals. The expected trimodal distribution is obtained for the side-chain chi 1-angles with a marked preference for staggered conformation. The hydrogen-bonding pattern in the N-terminal beta-sheet and the parallel sheet in the beta/alpha-barrel is described. A number of hydrogen bonds and salt bridges are involved in domain-domain and subunit-subunit interactions. The subunit-subunit interface in the dimer covers an area of 2800 A2. Considerable deviations from the local 2-fold symmetry are found at both the N terminus (residues 2 to 5) and the C terminus (residues 422 to 457). Furthermore, loop 8 in the beta/alpha-barrel domain has a different conformation in the two subunits. A number of amino acid side-chains have different conformations in the two subunits. Most of these residues are located at the surface of the protein. An analysis of the individual temperature factors indicates a high mobility of the C-terminal region and for some of the loops at the active site. The positions and B-factors for 736 solvent sites have been refined (average B: 45.9 A2). Most of the solvent molecules are bound as clusters to the protein. The active site of the enzyme, especially the environment of the activator Lys191 in the non-activated enzyme is described. Crystallographic refinement at 1.7 A resolution clearly revealed the presence of a cis-proline at the active site. This residue is part of the highly conserved region Lys166-Pro167-Lys168.

摘要

来自红螺菌的1,5 - 二磷酸核酮糖羧化酶/加氧酶的氨基酸序列已与电子密度图拟合。使用苏斯曼的约束 - 受限最小二乘精修程序以及亨德里克森和孔内特的受限最小二乘精修程序,将所得蛋白质模型精修至名义分辨率为1.7埃。基于在5.5至1.7埃分辨率范围内F大于σ(F)的76,452个反射进行的晶体学精修,得到晶体学R因子为18.0%。不对称单元包含一个二聚体1,5 - 二磷酸核酮糖羧化酶分子,由869个氨基酸残基和736个水分子组成。精修模型的几何结构接近理想状态,键长的均方根偏差为0.018埃,键角的均方根偏差为2.7度。在我们的晶体中,包含残基54至63和324至335的两个环区域以及C末端的最后十个氨基酸残基是无序的。对于侧链χ1角获得了预期的三峰分布,明显偏好交错构象。描述了N端β折叠和β/α桶中的平行折叠中的氢键模式。许多氢键和盐桥参与结构域 - 结构域和亚基 - 亚基相互作用。二聚体中的亚基 - 亚基界面覆盖面积为2800埃²。在N端(残基2至5)和C端(残基422至457)均发现与局部二重对称有相当大的偏差。此外,β/α桶结构域中的环8在两个亚基中具有不同的构象。一些氨基酸侧链在两个亚基中具有不同的构象。这些残基大多位于蛋白质表面。对各个温度因子的分析表明C末端区域以及活性位点处的一些环具有较高的流动性。已对736个溶剂位点的位置和B因子进行了精修(平均B:45.9埃²)。大多数溶剂分子以簇的形式与蛋白质结合。描述了该酶的活性位点,特别是未活化酶中激活剂赖氨酸191的环境。在1.7埃分辨率下的晶体学精修清楚地揭示了活性位点存在顺式脯氨酸。该残基是高度保守区域赖氨酸166 - 脯氨酸167 - 赖氨酸168的一部分。

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