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载脂蛋白牛钙结合蛋白D9k的1H核磁共振共振归属、二级结构和整体折叠

1H NMR resonance assignments, secondary structure, and global fold of Apo bovine calbindin D9k.

作者信息

Skelton N J, Forsén S, Chazin W J

机构信息

Department of Molecular Biology, Research Institute of Scripps Clinic, La Jolla, California 92037.

出版信息

Biochemistry. 1990 Jun 19;29(24):5752-61. doi: 10.1021/bi00476a016.

DOI:10.1021/bi00476a016
PMID:2200514
Abstract

The solution structure and dynamics of apo bovine calbindin D9k have been studied by a wide range of two-dimensional 1H nuclear magnetic resonance experiments. Due to the presence of conformational heterogeneity in the wild-type protein, the sequential resonance assignment was carried out on a Pro43----Gly mutant. By use of a combination of scalar correlation experiments acquired from H2O solution, 61 of the 76 1H spin systems could be assigned to particular amino acid types. The remaining resonances were assigned by a parallel series of experiments acquired from 2H2O solution. These spin system assignments provided a basis for complete sequential resonance assignments from interresidue backbone nuclear Overhauser effects (NOEs). Elements of secondary structure were identified from sequential and medium-range NOEs, backbone spin-spin coupling constants, and slowly exchanging amide protons. Four sections of helix are delineated, together with a short antiparallel beta-sheet interaction between the peptide loops involved in Ca2+ binding. The global fold is provided by combining these elements of secondary structure with a subset of the long-range, interhelix NOEs. Comparison with similar studies on the Ca2(+)-saturated protein indicates that at this crude level the structures are very similar. However, removal of the Ca2+ does dramatically affect the dynamics of the protein, as judged by amide proton exchange rates and aromatic ring rotation. This is particularly evident in the increased flexibility of the residues in the hydrophobic core.

摘要

已通过一系列二维¹H核磁共振实验研究了脱钙牛钙结合蛋白D9k的溶液结构和动力学。由于野生型蛋白存在构象异质性,因此对Pro43→Gly突变体进行了序列共振归属。通过使用从H₂O溶液中获得的标量相关实验的组合,可以将76个¹H自旋系统中的61个归属到特定的氨基酸类型。其余的共振则通过从²H₂O溶液中获得的一系列平行实验进行归属。这些自旋系统归属为基于残基间主链核Overhauser效应(NOE)进行完整的序列共振归属提供了基础。从序列和中程NOE、主链自旋-自旋耦合常数以及缓慢交换的酰胺质子中确定了二级结构元件。描绘了四个螺旋区段,以及参与Ca²⁺结合的肽环之间的短反平行β-折叠相互作用。通过将这些二级结构元件与长程、螺旋间NOE的一个子集相结合,提供了整体折叠结构。与对Ca²⁺饱和蛋白的类似研究相比表明,在这个粗略水平上,结构非常相似。然而,从酰胺质子交换率和芳环旋转判断,去除Ca²⁺确实会显著影响蛋白质的动力学。这在疏水核心中残基的灵活性增加方面尤为明显。

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