钙离子(Ca²⁺)与膜结合至膜联蛋白3会调节其N端和结构域III的结构与动力学。
Ca(2+) and membrane binding to annexin 3 modulate the structure and dynamics of its N terminus and domain III.
作者信息
Sopkova Jana, Raguenes-Nicol Céline, Vincent Michel, Chevalier Anne, Lewit-Bentley Anita, Russo-Marie Françoise, Gallay Jacques
机构信息
L.U.R.E., Bâtiment 209D, Centre Universitaire Paris-Sud, F-91898 Orsay, France.
出版信息
Protein Sci. 2002 Jul;11(7):1613-25. doi: 10.1110/ps.4230102.
Annexin 3 (ANX A3) represents approximately 1% of the total protein of human neutrophils and promotes tight contact between membranes of isolated specific granules in vitro leading to their aggregation. Like for other annexins, the primary molecular events of the action of this protein is likely its binding to negatively charged phospholipid membranes in a Ca(2+)-dependent manner, via Ca(2+)-binding sites located on the convex side of the highly conserved core of the molecule. The conformation and dynamics of domain III can be affected by this process, as it was shown for other members of the family. The 20 amino-acid, N-terminal segment of the protein also could be affected and also might play a role in the modulation of its binding to the membranes. The structure and dynamics of these two regions were investigated by fluorescence of the two tryptophan residues of the protein (respectively, W190 in domain III and W5 in the N-terminal segment) in the wild type and in single-tryptophan mutants. By contrast to ANX A5, which shows a closed conformation and a buried W187 residue in the absence of Ca(2+), domain III of ANX A3 exhibits an open conformation and a widely solvent-accessible W190 residue in the same conditions. This is in agreement with the three-dimensional structure of the ANX A3-E231A mutant lacking the bidentate Ca(2+) ligand in domain III. Ca(2+) in the millimolar concentration range provokes nevertheless a large mobility increase of the W190 residue, while interaction with the membranes reduces it slightly. In the N-terminal region, the W5 residue, inserted in the central pore of the protein, is weakly accessible to the solvent and less mobile than W190. Its amplitude of rotation increases upon binding of Ca(2+) and returns to its original value when interacting with membranes. Ca(2+) concentration for half binding of the W5A mutant to negatively charged membranes is approximately 0.5 mM while it increases to approximately 1 mM for the ANX A3 wild type and to approximately 3 mM for the W190 ANX A3 mutant. In addition to the expected perturbation of the W190 environment at the contact surface between the protein and the membrane bilayer, binding of the protein to Ca(2+) and to membranes modulates the flexibility of the ANX A3 hinge region at the opposite of this interface and might affect its membrane permeabilizing properties.
膜联蛋白3(ANX A3)约占人类中性粒细胞总蛋白的1%,在体外可促进分离出的特定颗粒膜之间的紧密接触,导致颗粒聚集。与其他膜联蛋白一样,该蛋白发挥作用的主要分子事件可能是其通过位于分子高度保守核心凸面的钙离子结合位点,以钙离子依赖的方式与带负电荷的磷脂膜结合。正如该家族其他成员所示,这一过程可能会影响结构域III的构象和动力学。该蛋白20个氨基酸的N端片段也可能受到影响,并且可能在调节其与膜的结合中发挥作用。通过野生型和单色氨酸突变体中该蛋白两个色氨酸残基(分别为结构域III中的W190和N端片段中的W5)的荧光,研究了这两个区域的结构和动力学。与膜联蛋白A5不同,在没有钙离子的情况下,膜联蛋白A5呈现封闭构象且W187残基被掩埋,而在相同条件下,膜联蛋白A3的结构域III呈现开放构象且W190残基可广泛地被溶剂接触。这与结构域III中缺乏双齿钙离子配体的膜联蛋白A3 - E231A突变体的三维结构一致。然而,毫摩尔浓度范围内的钙离子会引起W190残基的大幅移动增加,而与膜的相互作用会使其略有降低。在N端区域,插入蛋白中心孔的W5残基对溶剂的可及性较弱,且比W190的移动性小。其旋转幅度在钙离子结合时增加,与膜相互作用时恢复到原始值。W5A突变体与带负电荷膜半结合的钙离子浓度约为0.5 mM,而膜联蛋白A3野生型增加到约1 mM,W190膜联蛋白A3突变体增加到约3 mM。除了在蛋白与膜双层接触表面预期的W190环境扰动外,蛋白与钙离子和膜的结合还会调节该界面相对侧的膜联蛋白A3铰链区的灵活性,并可能影响其膜通透特性。
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