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一种活性钠钾ATP酶的表达,其α亚基缺乏所有二十三个天然半胱氨酸残基。

Expression of an active Na,K-ATPase with an alpha-subunit lacking all twenty-three native cysteine residues.

作者信息

Hu Y K, Eisses J F, Kaplan J H

机构信息

Department of Biochemistry and Molecular Biology, Oregon Health Sciences University, Portland, Oregon 97201-3098, USA.

出版信息

J Biol Chem. 2000 Sep 29;275(39):30734-9. doi: 10.1074/jbc.M003737200.

Abstract

We have constructed a mutant Na,K-ATPase alpha1-subunit with all native cysteine residues replaced. Using the baculovirus system, this cysteine-less alpha1-subunit and wild-type beta1-subunit were expressed in High Five cells. After 3 days of infection, cells were fractionated, and endoplasmic reticulum, Golgi apparatus, and plasma membranes were isolated. The molecular activity of the cysteine-less mutant in the plasma membranes was close to the wild-type protein (8223 min(-)(1) versus 6655 min(-)(1)). Cation and ATP activation of Na,K-ATPase activities revealed that replacing all 23 cysteines resulted in only a 50% reduction of K(m) for Na(+), a 2-fold increase in K(m) for K(+), and no changes in K(m) for ATP. The distribution of alpha-subunits among the membranes showed a high percentage of cysteine-less protein in the endoplasmic reticulum and Golgi apparatus compared with the wild-type protein. Furthermore, the cellular stability of the alphabeta assembly appeared reduced in the cysteine-less mutant. Cells harvested after more than 3 days of infection showed extensive degradation of the cysteine-less alpha-subunit, which is not observed with the wild-type enzyme. Thus the Na,K-ATPase contains no cysteine residues that are critical for function, but the folding and/or assembly pathway of this enzyme is affected by total cysteine substitution.

摘要

我们构建了一个将所有天然半胱氨酸残基都替换掉的突变型钠钾ATP酶α1亚基。利用杆状病毒系统,在High Five细胞中表达了这种不含半胱氨酸的α1亚基和野生型β1亚基。感染3天后,对细胞进行分级分离,分离出内质网、高尔基体和质膜。质膜中不含半胱氨酸的突变体的分子活性接近野生型蛋白(分别为8223 min⁻¹和6655 min⁻¹)。钠钾ATP酶活性对阳离子和ATP的激活作用表明,将所有23个半胱氨酸替换后,仅使Na⁺的米氏常数(Km)降低50%,使K⁺的Km增加2倍,而ATP的Km没有变化。膜间α亚基的分布显示,与野生型蛋白相比,内质网和高尔基体中不含半胱氨酸的蛋白比例较高。此外,不含半胱氨酸的突变体中αβ组装体的细胞稳定性似乎降低。感染超过3天后收获的细胞显示,不含半胱氨酸的α亚基出现广泛降解,而野生型酶则未观察到这种情况。因此,钠钾ATP酶不包含对功能至关重要的半胱氨酸残基,但该酶的折叠和/或组装途径会受到半胱氨酸完全替换的影响。

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