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钙结合蛋白D9k N端半饱和状态的表征:N56A突变体的核磁共振研究

Characterization of the N-terminal half-saturated state of calbindin D9k: NMR studies of the N56A mutant.

作者信息

Wimberly B, Thulin E, Chazin W J

机构信息

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

出版信息

Protein Sci. 1995 Jun;4(6):1045-55. doi: 10.1002/pro.5560040603.

DOI:10.1002/pro.5560040603
PMID:7549869
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2143144/
Abstract

Calbindin D9k is a small EF-hand protein that binds two calcium ions with positive cooperativity. The molecular basis of cooperativity for the binding pathway where the first ion binds in the N-terminal site (1) is investigated by NMR experiments on the half-saturated state of the N56A mutant, which exhibits sequential yet cooperative binding (Linse S, Chazin WJ, 1995, Protein Sci 4:1038-1044). Analysis of calcium-induced changes in chemical shifts, amide proton exchange rates, and NOEs indicates that ion binding to the N-terminal binding loop causes significant changes in conformation and/or dynamics throughout the protein. In particular, all three parameters indicate that the hydrophobic core undergoes a change in packing to a conformation very similar to the calcium-loaded state. These results are similar to those observed for the (Cd2+)1 state of the wild-type protein, a model for the complementary half-saturated state with an ion bound in the C-terminal site (II). Thus, with respect to cooperativity in either of the binding pathways, binding of the first ion drives the conformation and dynamics of the protein far toward the (Ca2+)2 state, thereby facilitating binding of the second ion. Comparison with the half-saturated state of the analogous E65Q mutant confirms that mutation of this critical bidentate calcium ligand at position 12 of the consensus EF-hand binding loop causes very significant structural perturbations. This result has important implications regarding numerous studies that have utilized mutation of this critical residue for site deactivation.

摘要

钙结合蛋白D9k是一种小的EF手型蛋白,能以正协同性结合两个钙离子。通过对N56A突变体半饱和状态进行核磁共振实验,研究了第一个离子在N端位点(1)结合的结合途径的协同性分子基础,该突变体表现出顺序性但协同性的结合(林斯·S,查津·WJ,1995年,《蛋白质科学》4:1038 - 1044)。对钙诱导的化学位移、酰胺质子交换率和核Overhauser效应(NOE)变化的分析表明,离子与N端结合环的结合会导致整个蛋白质的构象和/或动力学发生显著变化。特别是,所有这三个参数都表明疏水核心的堆积发生了变化,变为一种与钙负载状态非常相似的构象。这些结果与野生型蛋白(Cd2 +)1状态所观察到的结果相似,(Cd2 +)1状态是一个互补半饱和状态的模型,其中一个离子结合在C端位点(II)。因此,就任一结合途径中的协同性而言,第一个离子的结合将蛋白质的构象和动力学驱动至非常接近(Ca2 +)2状态,从而促进第二个离子的结合。与类似的E65Q突变体的半饱和状态进行比较证实,在共有EF手型结合环第12位的这个关键双齿钙配体发生突变会导致非常显著的结构扰动。这一结果对于众多利用该关键残基突变进行位点失活的研究具有重要意义。

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本文引用的文献

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High-resolution structure of calcium-loaded calbindin D9k.钙离子负载的钙结合蛋白D9k的高分辨率结构。
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Two-dimensional 1H nuclear magnetic resonance studies of the half-saturated (Ca2+)1 state of calbindin D9k. Further implications for the molecular basis of cooperative Ca2+ binding.钙结合蛋白D9k半饱和(Ca2+)1状态的二维1H核磁共振研究。对协同Ca2+结合分子基础的进一步启示。
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