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通过两种不同且互补的交联方法探索信号序列与大肠杆菌信号识别颗粒(SRP)之间的相互作用。

Exploring the interactions between signal sequences and E. coli SRP by two distinct and complementary crosslinking methods.

作者信息

Clérico Eugenia M, Szymańska Aneta, Gierasch Lila M

机构信息

Department of Biochemistry & Molecular Biology, University of Massachusetts, Amherst MA 01003, U.S.A.

出版信息

Biopolymers. 2009;92(3):201-11. doi: 10.1002/bip.21181.

DOI:10.1002/bip.21181
PMID:19280642
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2896254/
Abstract

Photoaffinity crosslinking comprises a group of invaluable techniques used to investigate in detail a binding interaction between two polypeptides. As the diverse photo crosslinking techniques available display inherent differences, the method of choice will provide specific information about a particular system under study. We used two complementary crosslinking approaches: photo-induced crosslinking of unmodified proteins (PICUP) and benzophenone-mediated (BPM) crosslinking to extensively examine the interaction between the signal recognition particle (SRP) and signal sequences. Signal peptide binding by SRP presents a central puzzle in the protein targeting process because signal sequences must be recognized with fidelity but lack strict primary structural homology. The concurrent use of PICUP and BPM crosslinking to link signal peptides to E. coli SRP allowed us to explore the crosslinking pattern resulting from using different crosslinking chemistries, varying the position of the photoprobe in the hydrophobic core of the signal sequence, and shifting the crosslinking reactive group away from the signal peptide backbone. By PICUP, signal peptides crosslinked exclusively to the NG domain of the SRP protein Ffh, regardless of the position of the reactive residue. Benzophenone-modified amino acids preferentially crosslinked the signal peptide to the C-terminal (M) domain of Ffh. We conclude that signal peptide binding is largely mediated by the M domain. Importantly, our data also indicate intimate, at least transient, contacts between the hydrophobic core of the signal peptide and the NG domain. These results reopen the possibility of a direct involvement of the NG domain in signal sequence recognition.

摘要

光亲和交联包括一组用于详细研究两种多肽之间结合相互作用的宝贵技术。由于现有的多种光交联技术存在固有差异,所选择的方法将提供有关所研究特定系统的特定信息。我们使用了两种互补的交联方法:未修饰蛋白质的光诱导交联(PICUP)和二苯甲酮介导的(BPM)交联,以广泛研究信号识别颗粒(SRP)与信号序列之间的相互作用。SRP对信号肽的结合是蛋白质靶向过程中的一个核心难题,因为信号序列必须被准确识别,但缺乏严格的一级结构同源性。同时使用PICUP和BPM交联将信号肽与大肠杆菌SRP连接起来,使我们能够探索使用不同交联化学、改变光探针在信号序列疏水核心中的位置以及将交联反应基团从信号肽主链上移开所产生的交联模式。通过PICUP,信号肽仅与SRP蛋白Ffh的NG结构域交联,而与反应性残基的位置无关。二苯甲酮修饰的氨基酸优先将信号肽与Ffh的C末端(M)结构域交联。我们得出结论,信号肽结合主要由M结构域介导。重要的是,我们的数据还表明信号肽的疏水核心与NG结构域之间存在紧密的,至少是短暂的接触。这些结果重新开启了NG结构域直接参与信号序列识别的可能性。

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