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CYP2C8 以二聚体的形式存在于天然膜中。

CYP2C8 exists as a dimer in natural membranes.

机构信息

Department of Molecular and Integrative Physiology and the College of Medicine, University of Illinois at Urbana-Champaign, Urbana, Illinois, USA.

出版信息

Drug Metab Dispos. 2010 Nov;38(11):1976-83. doi: 10.1124/dmd.110.034942. Epub 2010 Aug 10.

Abstract

CYP2C8 with a modified N-terminal sequence (2C8H) crystallizes as a dimer, but it is not known whether native CYP2C8 exists as a dimer in natural membranes. We have examined the organization of 2C8H and CYP2C8 expressed in bacterial membranes and mammalian endoplasmic reticulum membranes, respectively, by cysteine scanning and cross-linking or oxidation of sulfhydryl groups. In both forms of CYP2C8, cross-linked dimers were observed that were eliminated by mutation of Cys-24 in the linker region. Introduction of individual cysteines in the N-terminal 21-amino acid membrane-spanning signal anchor resulted in a pattern of cross-linking consistent with an α-helical structure for the signal anchor. In the linker region, cross-linking was observed for cysteine substituted at residues 22, 23, or 24, just before three Arg residues, indicating close apposition of the two linker sequences despite the neighboring positive charges. Introduction into the F-G loop region of cysteine pairs optimally located for cross-linking based on the crystal structure resulted in cross-linked dimers in the Cys-24 mutant. Deletion of the signal anchor sequence eliminated cross-linking mediated by Cys-24 or by cysteines introduced in the F-G loop regions, indicating that the signal anchor interaction is required for stable dimer formation. These results indicate that the signal anchor sequence and the F-G loop region form interfaces for CYP2C8 intermolecular interactions in natural membranes.

摘要

CYP2C8 带有修饰的 N 端序列(2C8H)形成二聚体,但尚不清楚天然膜中的 CYP2C8 是否以二聚体形式存在。我们通过半胱氨酸扫描和巯基的交联或氧化,分别研究了细菌膜中表达的 2C8H 和 CYP2C8 的结构,以及内质网膜中表达的 2C8H 和 CYP2C8。在这两种形式的 CYP2C8 中,观察到交联的二聚体,通过连接区中 Cys-24 的突变可以消除这些二聚体。在 N 端 21 个氨基酸跨膜信号锚的疏水区引入单个半胱氨酸,导致交联模式与信号锚的α螺旋结构一致。在连接区,在紧邻三个 Arg 残基之前的残基 22、23 或 24 处取代半胱氨酸时,观察到交联,表明尽管存在相邻的正电荷,但两个连接序列的紧密接近。根据晶体结构,将最优定位用于交联的半胱氨酸对引入 F-G 环区域,导致 Cys-24 突变体中的交联二聚体。信号锚序列的缺失消除了 Cys-24 或 F-G 环区域中引入的半胱氨酸介导的交联,表明信号锚相互作用是稳定二聚体形成所必需的。这些结果表明,信号锚序列和 F-G 环区域在天然膜中形成 CYP2C8 分子间相互作用的界面。

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