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STIM1 中的一个基本序列通过与 Orai1 的 C 端酸性卷曲螺旋相互作用促进 Ca2+内流。

A basic sequence in STIM1 promotes Ca2+ influx by interacting with the C-terminal acidic coiled coil of Orai1.

机构信息

Department of Chemistry and Chemical Biology, Cornell University, Ithaca, New York 14853, USA.

出版信息

Biochemistry. 2010 Feb 16;49(6):1067-71. doi: 10.1021/bi901936q.

Abstract

Store-operated Ca(2+) entry (SOCE) is a ubiquitous signaling process in eukaryotic cells in which the endoplasmic reticulum (ER)-localized Ca(2+) sensor, STIM1, activates the plasma membrane-localized Ca(2+) release-activated Ca(2+) (CRAC) channel, Orai1, in response to emptying of ER Ca(2+) stores. In efforts to understand this activation mechanism, we recently identified an acidic coiled-coil region in the C-terminus of Orai1 that contributes to physical association between these two proteins, as measured by fluorescence resonance energy transfer, and is necessary for Ca(2+) influx, as measured by an intracellular Ca(2+) indicator. Here, we present evidence that a positively charged sequence of STIM1 in its CRAC channel activating domain, human residues 384-386, is necessary for activation of SOCE, most likely because this sequence interacts directly with the acidic coiled coil of Orai1 to gate Ca(2+) influx. We find that mutation to remove positive charges in these residues in STIM1 prevents its stimulated association with wild-type Orai1. However, association does occur between this mutant STIM1 and Orai1 that is mutated to remove negative charges in its C-terminal coiled coil, indicating that other structural features are sufficient for this interaction. Despite this physical association, we find that thapsigargin fails to activate SOCE following coexpression of mutant STIM1 with either wild type or mutant Orai1, implicating STIM1 residues 384-386 in transmission of the Ca(2+) gating signal to Orai1 following store depletion.

摘要

钙库操纵性钙内流(SOCE)是真核细胞中普遍存在的信号转导过程,其中内质网(ER)定位的钙传感器 STIM1 响应 ER Ca2+ 储存耗尽,激活质膜定位的 Ca2+ 释放激活的 Ca2+(CRAC)通道 Orai1。为了理解这种激活机制,我们最近在 Orai1 的 C 末端鉴定出一个酸性卷曲螺旋区域,该区域通过荧光共振能量转移测量,有助于这两种蛋白质之间的物理相互作用,并对 Ca2+ 内流(通过细胞内 Ca2+指示剂测量)是必需的。在这里,我们提供的证据表明,STIM1 的 CRAC 通道激活结构域中的一个带正电荷的序列,人类残基 384-386,对于 SOCE 的激活是必需的,很可能是因为该序列直接与 Orai1 的酸性卷曲螺旋相互作用以门控 Ca2+ 内流。我们发现,在 STIM1 中这些残基的正电荷被突变以去除时,会阻止其与野生型 Orai1 的受刺激的相互作用。然而,这种突变 STIM1 确实与 Orai1 发生相互作用,而 Orai1 的 C 末端卷曲螺旋中的负电荷被突变去除,表明其他结构特征足以进行这种相互作用。尽管存在这种物理相互作用,但我们发现,在用突变 STIM1 共表达时,他莫昔芬不能激活 SOCE,无论是野生型还是突变型 Orai1,这表明 STIM1 残基 384-386 在 ER 耗尽后将 Ca2+ 门控信号传递给 Orai1 。

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