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心肌细胞中细胞外别构 Na(+) 与 Na(+),K(+)-ATP 酶的结合。

Extracellular allosteric Na(+) binding to the Na(+),K(+)-ATPase in cardiac myocytes.

机构信息

Department of Cardiology, Royal North Shore Hospital, Sydney, Australia; Kolling Institute, University of Sydney, Sydney, Australia.

Faculty of Biology, University of Konstanz, Konstanz, Germany.

出版信息

Biophys J. 2013 Dec 17;105(12):2695-705. doi: 10.1016/j.bpj.2013.11.004.

Abstract

Whole-cell patch-clamp measurements of the current, Ip, produced by the Na(+),K(+)-ATPase across the plasma membrane of rabbit cardiac myocytes show an increase in Ip over the extracellular Na(+) concentration range 0-50 mM. This is not predicted by the classical Albers-Post scheme of the Na(+),K(+)-ATPase mechanism, where extracellular Na(+) should act as a competitive inhibitor of extracellular K(+) binding, which is necessary for the stimulation of enzyme dephosphorylation and the pumping of K(+) ions into the cytoplasm. The increase in Ip is consistent with Na(+) binding to an extracellular allosteric site, independent of the ion transport sites, and an increase in turnover via an acceleration of the rate-determining release of K(+) to the cytoplasm, E2(K(+))2 → E1 + 2K(+). At normal physiological concentrations of extracellular Na(+) of 140 mM, it is to be expected that binding of Na(+) to the allosteric site would be nearly saturated. Its purpose would seem to be simply to optimize the enzyme's ion pumping rate under its normal physiological conditions. Based on published crystal structures, a possible location of the allosteric site is within a cleft between the α- and β-subunits of the enzyme.

摘要

全细胞膜片钳测量兔心肌细胞质膜上的 Na(+),K(+)-ATP 酶产生的电流 Ip 表明,在 0-50 mM 的细胞外 Na(+)浓度范围内,Ip 增加。这与 Na(+),K(+)-ATP 酶机制的经典 Albers-Post 方案不一致,在该方案中,细胞外 Na(+)应作为细胞外 K(+)结合的竞争性抑制剂,这对于刺激酶去磷酸化和将 K(+)离子泵入细胞质是必需的。Ip 的增加与 Na(+)结合到细胞外变构位点有关,与离子转运位点无关,通过加速决定 K(+)释放到细胞质的速率,E2(K(+))2 → E1 + 2K(+),从而增加周转率。在正常生理浓度的 140 mM 细胞外 Na(+)下,可以预期 Na(+)与变构位点的结合几乎达到饱和。它的目的似乎是在正常生理条件下优化酶的离子泵送速率。基于已发表的晶体结构,变构位点的一个可能位置在酶的α-和β-亚基之间的裂隙内。

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