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鉴定出突触SNARE复合体的一个最小核心,其足以进行可逆组装和解聚。

Identification of a minimal core of the synaptic SNARE complex sufficient for reversible assembly and disassembly.

作者信息

Fasshauer D, Eliason W K, Brünger A T, Jahn R

机构信息

Department of Neurobiology, Max-Planck-Institute for Biophysical Chemistry, Göttingen, Germany.

出版信息

Biochemistry. 1998 Jul 21;37(29):10354-62. doi: 10.1021/bi980542h.

DOI:10.1021/bi980542h
PMID:9671503
Abstract

Assembly of the three neuronal membrane proteins synaptobrevin, syntaxin, and SNAP-25 is thought to be one of the key steps in mediating exocytosis of synaptic vesicles. In vivo and in vitro, these proteins form a tight complex. Assembly is associated with a large increase in alpha-helical content, suggesting that major structural and conformational changes are associated with the assembly reaction. Limited proteolysis by trypsin, chymotrypsin, and proteinase K of the ternary complex formed from recombinant proteins lacking their membrane anchors revealed a SDS-resistant minimal core. The components of this core complex were purified and characterized by N-terminal sequencing and mass spectrometry. They include a slightly shortened synaptobrevin fragment, C- and N-terminal fragments of SNAP-25, and a C-terminal fragment of syntaxin that is slightly larger than the previously characterized H3 domain. Recombinant proteins corresponding to these fragments are sufficient for assembly and disassembly. In addition, each of the two SNAP-25 fragments can individually form complexes with syntaxin and synaptobrevin, suggesting that they both contribute to the assembly of the SNARE complex. Upon complex assembly, a large increase in alpha-helical content is observed along with a significantly increased melting temperature (Tm). Like the full-length complex, the minimal complex tends to form an oligomeric species; global analysis of equilibrium ultracentrifugation data suggests a monomer-trimer equilibrium exists. These conserved biophysical properties may thus be of fundamental importance in the mechanism of membrane fusion.

摘要

三种神经元膜蛋白突触小泡蛋白、 syntaxin和SNAP - 25的组装被认为是介导突触小泡胞吐作用的关键步骤之一。在体内和体外,这些蛋白形成紧密复合物。组装与α - 螺旋含量的大幅增加相关,表明主要的结构和构象变化与组装反应有关。用胰蛋白酶、胰凝乳蛋白酶和蛋白酶K对缺乏膜锚定结构的重组蛋白形成的三元复合物进行有限的蛋白水解,揭示了一种抗SDS的最小核心。通过N端测序和质谱对该核心复合物的成分进行了纯化和表征。它们包括一个稍微缩短的突触小泡蛋白片段、SNAP - 25的C端和N端片段,以及一个比先前表征的H3结构域稍大的syntaxin C端片段。与这些片段相对应的重组蛋白足以进行组装和拆卸。此外,两个SNAP - 25片段中的每一个都可以单独与syntaxin和突触小泡蛋白形成复合物,这表明它们都对SNARE复合物的组装有贡献。在复合物组装时,观察到α - 螺旋含量大幅增加,同时解链温度(Tm)显著升高。与全长复合物一样,最小复合物倾向于形成寡聚体;平衡超速离心数据的整体分析表明存在单体 - 三聚体平衡。因此,这些保守的生物物理性质可能在膜融合机制中具有根本重要性。

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