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钙离子和N - 乙基马来酰亚胺敏感因子对早期内体上SNARE复合体的拆解有不同的调节作用。

Ca2+ and N-ethylmaleimide-sensitive factor differentially regulate disassembly of SNARE complexes on early endosomes.

作者信息

Yan Qing, Sun Wei, McNew James A, Vida Thomas A, Bean Andrew J

机构信息

Department of Neurobiology and Anatomy, University of Texas Medical School, Houston, Texas 77030, USA.

出版信息

J Biol Chem. 2004 Apr 30;279(18):18270-6. doi: 10.1074/jbc.M400093200. Epub 2004 Feb 9.

DOI:10.1074/jbc.M400093200
PMID:14769786
Abstract

The endosome-associated protein Hrs inhibits the homotypic fusion of early endosomes. A helical region of Hrs containing a Q-SNARE motif mediates this effect as well as its endosomal membrane association via SNAP-25, an endosomal receptor for Hrs. Hrs inhibits formation of an early endosomal SNARE complex by displacing VAMP-2 from the complex, suggesting a mechanism by which Hrs inhibits early endosome fusion. We examined the regulation of endosomal SNARE complexes to probe how Hrs may function as a negative regulator. We show that although NSF dissociates the VAMP-2.SNAP-25.syntaxin 13 complex, it has no effect on the Hrs-containing complex. Whereas Ca(2+) dissociates the Hrs-containing complex but not the VAMP-2-containing SNARE complex. This is the first demonstration of differential regulation of R/Q-SNARE and all Q-SNARE-containing SNARE complexes. Ca(2+) also reverses the Hrs-induced inhibition of early endosome fusion in a tetanus toxin-sensitive manner and removes Hrs from early endosomal membranes. Moreover, Hrs inhibition of endosome fusion and its endosomal localization are sensitive to bafilomycin, implying a role for luminal Ca(2+). Thus, Hrs may bind a SNARE protein on early endosomal membranes negatively regulating trans-SNARE pairing and endosomal fusion. The release of Ca(2+) from the endosome lumen dissociates Hrs, allowing a VAMP-2-containing complex to form enabling fusion.

摘要

内体相关蛋白Hrs抑制早期内体的同型融合。Hrs的一个含有Q-SNARE基序的螺旋区域介导了这种效应以及它通过SNAP-25(一种Hrs的内体受体)与内体膜的结合。Hrs通过从复合物中取代VAMP-2来抑制早期内体SNARE复合物的形成,这提示了一种Hrs抑制早期内体融合的机制。我们研究了内体SNARE复合物的调控,以探究Hrs如何作为负调节因子发挥作用。我们发现,虽然NSF可使VAMP-2.SNAP-25.syntaxin 13复合物解离,但对含有Hrs的复合物没有影响。而Ca(2+)可使含有Hrs的复合物解离,但对含有VAMP-2的SNARE复合物没有影响。这是首次证明R/Q-SNARE和所有含Q-SNARE的SNARE复合物存在差异调控。Ca(2+)还以破伤风毒素敏感的方式逆转了Hrs诱导的早期内体融合抑制,并将Hrs从早期内体膜上移除。此外,Hrs对内体融合的抑制及其在内体中的定位对巴弗洛霉素敏感,这暗示了腔内Ca(2+)的作用。因此,Hrs可能与早期内体膜上的一种SNARE蛋白结合,负向调节跨SNARE配对和内体融合。内体腔内Ca(2+)的释放使Hrs解离,从而允许形成含VAMP-2的复合物以实现融合。

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Ca2+ and N-ethylmaleimide-sensitive factor differentially regulate disassembly of SNARE complexes on early endosomes.钙离子和N - 乙基马来酰亚胺敏感因子对早期内体上SNARE复合体的拆解有不同的调节作用。
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