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Slac2-a/黑素亲和素的类突触结合蛋白样蛋白(Slp)同源结构域1是与Rab27A的GTP依赖性特异性结合的关键决定因素。

Synaptotagmin-like protein (Slp) homology domain 1 of Slac2-a/melanophilin is a critical determinant of GTP-dependent specific binding to Rab27A.

作者信息

Fukuda Mitsunori

机构信息

Fukuda Initiative Research Unit, RIKEN (Institute of Physical and Chemical Research), 2-1 Hirosawa, Wako, Saitama 351-0198, Japan.

出版信息

J Biol Chem. 2002 Oct 18;277(42):40118-24. doi: 10.1074/jbc.M205765200. Epub 2002 Aug 19.

DOI:10.1074/jbc.M205765200
PMID:12189142
Abstract

The N-terminal synaptotagmin-like protein (Slp) homology domain (SHD) of the Slp and Slac2 families has recently been identified as a specific Rab27A-binding domain (Kuroda, T. S., Fukuda, M., Ariga, H., and Mikoshiba, K. (2002) J. Biol. Chem. 277, 9212-9218; Fukuda, M., Kuroda, T. S., and Mikoshiba, K. (2002) J. Biol. Chem. 277, 12432-12436). The SHD consists of two conserved alpha-helical regions (SHD1 and SHD2) that are often separated by two zinc finger motifs. However, the structural basis of Rab27A recognition by the SHD (i.e. involvement of each region (SHD1, zinc finger motifs, and SHD2) in Rab27A recognition and critical residue(s) for Rab27A/SHD interaction) had never been elucidated. In this study, systematic deletion analysis and Ala-based site-directed mutagenesis showed that SHD1 of Slac2-a/melanophilin alone is both necessary and sufficient for high affinity specific recognition of the GTP-bound form of Rab27A. By contrast, the zinc finger motifs and SHD2 are not an autonomous Rab27A-binding site and seem to be important for stabilization of the structure of the SHD or higher affinity Rab27A binding. In addition, chimeric analysis of Rab3A and Rab27A showed that the specific sequence of the switch II region of Rab27 isoforms (especially Leu-84, Phe-88, and Asp-91 of Rab27A), which is not conserved in the Rab3 or Rab8 isoforms, is essential for recognition by the Slac2-a SHD. Based on these findings, I propose that SHD1 of the Slp and Slac2 families be referred to as RBD27 (Rab-binding domain specific for Rab27 isoforms).

摘要

最近,Slp和Slac2家族的N端类突触结合蛋白(Slp)同源结构域(SHD)被确定为一个特定的Rab27A结合结构域(黑田,T.S.,福田,M.,有贺,H.,和三木茂,K.(2002年)《生物化学杂志》277,9212 - 9218;福田,M.,黑田,T.S.,和三木茂,K.(2002年)《生物化学杂志》277,12432 - 12436)。SHD由两个保守的α螺旋区域(SHD1和SHD2)组成,它们常被两个锌指基序隔开。然而,SHD识别Rab27A的结构基础(即每个区域(SHD1、锌指基序和SHD2)在Rab27A识别中的作用以及Rab27A/SHD相互作用的关键残基)从未得到阐明。在本研究中,系统的缺失分析和基于丙氨酸的定点诱变表明,单独的Slac2 - a/亲黑素的SHD1对于高亲和力特异性识别GTP结合形式的Rab27A既必要又充分。相比之下,锌指基序和SHD2不是一个自主的Rab27A结合位点,似乎对SHD结构的稳定或更高亲和力的Rab27A结合很重要。此外,Rab3A和Rab27A的嵌合分析表明,Rab27亚型开关II区域的特定序列(特别是Rab27A的Leu - 84、Phe - 88和Asp - 91)在Rab3或Rab8亚型中不保守,对于Slac2 - a SHD的识别至关重要。基于这些发现,我提议将Slp和Slac2家族的SHD1称为RBD27(对Rab27亚型特异的Rab结合结构域)。

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