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钠钾ATP酶离子泵的渗透应激和粘性阻滞

Osmotic stress and viscous retardation of the Na,K-ATPase ion pump.

作者信息

Esmann Mikael, Fedosova Natalya U, Marsh Derek

机构信息

Institute of Physiology and Biophysics, University of Aarhus, DK-8000 Aarhus, Denmark. me@biophys

出版信息

Biophys J. 2008 Apr 1;94(7):2767-76. doi: 10.1529/biophysj.106.101774. Epub 2007 Nov 30.

Abstract

The transport function of the Na pump (Na,K-ATPase) in cellular ion homeostasis involves both nucleotide binding reactions in the cytoplasm and alternating aqueous exposure of inward- and outward-facing ion binding sites. An osmotically active, nonpenetrating polymer (poly(ethyleneglycol); PEG) and a modifier of the aqueous viscosity (glycerol) were used to probe the overall and partial enzymatic reactions of membranous Na,K-ATPase from shark salt glands. Both inhibit the steady-state Na,K-ATPase as well as Na-ATPase activity, whereas the K(+)-dependent phosphatase activity is little affected by up to 50% of either. Both Na,K-ATPase and Na-ATPase activities are inversely proportional to the viscosity of glycerol solutions in which the membranes are suspended, in accordance with Kramers' theory for strong coupling of fluctuations at the active site to solvent mobility in the aqueous environment. PEG decreases the affinity for Tl(+) (a congener for K(+)), whereas glycerol increases that for the nucleotides ATP and ADP in the presence of NaCl but has little effect on the affinity for Tl(+). From the dependence on osmotic stress induced by PEG, the aqueous activation volume for the Na,K-ATPase reaction is estimated to be approximately 5-6 nm(3) (i.e., approximately 180 water molecules), approximately half this for Na-ATPase, and essentially zero for p-nitrophenol phosphatase. The change in aqueous hydrated volume associated with the binding of Tl(+) is in the region of 9 nm(3). Analysis of 15 crystal structures of the homologous Ca-ATPase reveals an increase in PEG-inaccessible water space of approximately 22 nm(3) between the E(1)-nucleotide bound forms and the E(2)-thapsigargin forms, showing that the experimental activation volumes for Na,K-ATPase are of a magnitude comparable to the overall change in hydration between the major E(1) and E(2) conformations of the Ca-ATPase.

摘要

钠泵(Na,K - ATP酶)在细胞离子稳态中的转运功能涉及细胞质中的核苷酸结合反应以及向内和向外的离子结合位点交替暴露于水相。使用一种具有渗透活性的非渗透性聚合物(聚乙二醇;PEG)和一种水相粘度调节剂(甘油)来探究鲨鱼盐腺中膜状Na,K - ATP酶的整体和部分酶促反应。二者均抑制稳态的Na,K - ATP酶以及Na - ATP酶活性,而K⁺依赖性磷酸酶活性在二者浓度高达50%时几乎不受影响。根据克拉默斯理论,即活性位点的涨落与水相环境中溶剂流动性的强耦合,Na,K - ATP酶和Na - ATP酶活性均与悬浮膜的甘油溶液粘度成反比。PEG降低了对Tl⁺(K⁺的同类物)的亲和力,而甘油在存在NaCl的情况下增加了对核苷酸ATP和ADP的亲和力,但对Tl⁺的亲和力影响很小。根据对PEG诱导的渗透应激的依赖性,估计Na,K - ATP酶反应的水相活化体积约为5 - 6 nm³(即约180个水分子),Na - ATP酶的约为其一半,对硝基苯酚磷酸酶的基本为零。与Tl⁺结合相关的水合体积变化在9 nm³范围内。对同源Ca - ATP酶的15个晶体结构的分析表明,在E(1) - 核苷酸结合形式和E(2) - 毒胡萝卜素形式之间,PEG不可及的水空间增加了约22 nm³,这表明Na,K - ATP酶的实验活化体积与Ca - ATP酶主要E(1)和E(2)构象之间水合作用的总体变化幅度相当。

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