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一个包含疏水和亲水序列的氨基末端结构域将信号识别颗粒受体α亚基与内质网膜上的β亚基结合。

An amino-terminal domain containing hydrophobic and hydrophilic sequences binds the signal recognition particle receptor alpha subunit to the beta subunit on the endoplasmic reticulum membrane.

作者信息

Young J C, Ursini J, Legate K R, Miller J D, Walter P, Andrews D W

机构信息

Department of Biochemistry, McMaster University, Hamilton, Ontario, Canada.

出版信息

J Biol Chem. 1995 Jun 30;270(26):15650-7. doi: 10.1074/jbc.270.26.15650.

DOI:10.1074/jbc.270.26.15650
PMID:7797564
Abstract

The signal recognition particle receptor consists of two subunits of 72 kDa (SR alpha) and 30 kDa (SR beta). Assembly of SR alpha on the endoplasmic reticulum membrane can occur independent of the signal recognition particle-mediated translocation pathway. To identify the sequences within SR alpha necessary for membrane binding, a series of amino-terminal and internal deletion mutants was constructed and translated in a cell-free system. In addition, nascent SR alpha polypeptides of varying lengths were generated by cycloheximide treatment of translation reactions. Microsome binding assays performed on these polypeptides revealed a membrane binding domain consisting of the amino-terminal 140 residues of SR alpha. This domain includes the two hydrophobic sequences originally proposed to bind to membranes and a highly charged region not previously implicated in membrane assembly. Furthermore, the domain forms a protease-resistant folding unit that after proteolysis can target and anchor onto microsomes. Extraction of microsomal SR alpha at high pH supplemented with 1 M NaSCN suggests that SR alpha and the membrane binding domain are not integrated in the endoplasmic reticulum membrane. The membrane binding domain is also the major site of tight binding with SR beta, suggesting that SR beta plays a role in the membrane assembly of SR alpha.

摘要

信号识别颗粒受体由72 kDa(SRα)和30 kDa(SRβ)的两个亚基组成。SRα在内质网膜上的组装可以独立于信号识别颗粒介导的转运途径发生。为了鉴定SRα中与膜结合所需的序列,构建了一系列氨基末端和内部缺失突变体,并在无细胞系统中进行翻译。此外,通过对翻译反应进行环己酰亚胺处理,产生了不同长度的新生SRα多肽。对这些多肽进行的微粒体结合试验揭示了一个由SRα的氨基末端140个残基组成的膜结合结构域。该结构域包括最初提出与膜结合的两个疏水序列和一个以前未涉及膜组装的高度带电区域。此外,该结构域形成一个抗蛋白酶的折叠单元,在蛋白水解后可以靶向并锚定到微粒体上。在补充有1 M NaSCN的高pH值下提取微粒体SRα表明,SRα和膜结合结构域没有整合在内质网膜中。膜结合结构域也是与SRβ紧密结合的主要位点,表明SRβ在SRα的膜组装中起作用。

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