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天然和重组钠钾ATP酶性质之间的异同。

Similarities and differences between the properties of native and recombinant Na+/K+-ATPases.

作者信息

Xie Z, Wang Y, Liu G, Zolotarjova N, Periyasamy S M, Askari A

机构信息

Department of Pharmacology, Medical College of Ohio, Toledo 43699-0008, USA.

出版信息

Arch Biochem Biophys. 1996 Jun 1;330(1):153-62. doi: 10.1006/abbi.1996.0237.

Abstract

Progress of mutagenesis studies on the relation of the structure of Na+/K+-ATPase to its reaction mechanism has been impeded by the paucity of information on the properties of small amounts of impure recombinant enzyme obtained in the currently available expression systems, and the uncertainty of whether expression in a new environment alters the various catalytic activities of this membrane enzyme. Hence, our aim was to make a detailed comparison of the properties of the extensively studied canine kidney Na+/K+-ATPase with those of its alpha1,beta1 subunits expressed in the baculovirus-infected Sf-9 cells. The active fraction of the recombinant enzyme, containing 10-20% of the expressed a subunits, was found to have normal molar activity, all the partial reactions, and the ability to catalyze ATP-dependent Na+/K+ exchange after reconstitution into proteoliposomes. Comparison of steady-state kinetics of the hydrolytic activities of recombinant and native enzymes showed that (a) ATP and Na+ plots of Na+-ATPase were the same in the two preparations; (b) apparent K+ affinity of K+-phosphatase of recombinant enzyme was lower than that of kidney enzyme; and (c) for Na+/K+- ATPase activity, apparent K+ affinity of recombinant enzyme was lower, and its apparent Na+ and ATP affinities were higher than those of kidney enzyme. The two enzymes had similar ADP- and K+-sensitive phosphointermediates, identical affinities for ouabain, and similar ligand sensitivities of dissociation rates of ouabain-enzyme complexes. Evidently, the recombinant enzyme has reduced affinity at cytoplasmic K+ sites, but no changes at multiple Na+, ATP, and ouabain binding sites. Likely causes of this selective change include altered glycosylation state of beta and interactions among active and inactive recombinant enzymes. The present results provide the necessary database for the appropriate use of an expression system in structure-function studies on canine alpha1,beta1 isoform of Na+/K+-ATPase, and indicate the need for similar studies on recombinant Na+/K+-ATPases obtained in other expression systems.

摘要

目前可用的表达系统中获得的少量不纯重组酶的性质信息匮乏,以及在新环境中表达是否会改变这种膜酶的各种催化活性尚不确定,这阻碍了关于Na⁺/K⁺-ATP酶结构与其反应机制关系的诱变研究进展。因此,我们的目的是详细比较广泛研究的犬肾Na⁺/K⁺-ATP酶与其在杆状病毒感染的Sf-9细胞中表达的α1、β1亚基的性质。发现重组酶的活性部分含有10%-20%表达的α亚基,在重构到蛋白脂质体后具有正常的摩尔活性、所有部分反应以及催化ATP依赖的Na⁺/K⁺交换的能力。重组酶和天然酶水解活性的稳态动力学比较表明:(a)两种制剂中Na⁺-ATP酶的ATP和Na⁺曲线相同;(b)重组酶的K⁺-磷酸酶的表观K⁺亲和力低于肾酶;(c)对于Na⁺/K⁺-ATP酶活性,重组酶的表观K⁺亲和力较低,其表观Na⁺和ATP亲和力高于肾酶。这两种酶具有相似的对ADP和K⁺敏感的磷酸中间产物、对哇巴因的相同亲和力以及哇巴因-酶复合物解离速率的相似配体敏感性。显然,重组酶在细胞质K⁺位点的亲和力降低,但在多个Na⁺、ATP和哇巴因结合位点没有变化。这种选择性变化的可能原因包括β糖基化状态的改变以及活性和非活性重组酶之间的相互作用。目前的结果为在犬Na⁺/K⁺-ATP酶α1、β1同工型的结构-功能研究中适当使用表达系统提供了必要的数据库,并表明需要对在其他表达系统中获得的重组Na⁺/K⁺-ATP酶进行类似研究。

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