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Inside-out Ca2+ signalling prompted by STIM1 conformational switch

机译:STIM1构象转换提示由内而外的Ca2 +信号传导

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Store-operated Ca2+ entry mediated by STIM1 and ORAI1 constitutes one of the major Ca2+ entry routes in mammalian cells. The molecular choreography of STIM1-ORAI1 coupling is initiated by endoplasmic reticulum (ER) Ca2+ store depletion with subsequent oligomerization of the STIM1 ER-luminal domain, followed by its redistribution towards the plasma membrane to gate ORAI1 channels. The mechanistic underpinnings of this inside-out Ca2+ signalling were largely undefined. By taking advantage of a unique gain-of-function mutation within the STIM1 transmembrane domain (STIM1-TM), here we show that local rearrangement, rather than alteration in the oligomeric state of STIM1-TM, prompts conformational changes in the cytosolic juxtamembrane coiled-coil region. Importantly, we further identify critical residues within the cytoplasmic domain of STIM1 (STIM1-CT) that entail autoinhibition. On the basis of these findings, we propose a model in which STIM1-TM reorganization switches STIM1-CT into an extended conformation, thereby projecting the ORAI-activating domain to gate ORAI1 channels.
机译:由STIM1和ORAI1介导的商店操纵的Ca2 +进入途径是哺乳动物细胞中主要的Ca2 +进入途径之一。 STIM1-ORAI1偶联的分子编排是由内质网(ER)Ca2 +存储耗竭和随后STIM1 ER-管腔结构域的寡聚化,随后向质膜的重新分布到门ORAI1通道的引发而开始的。这种由内而外的Ca2 +信号传导的机制基础尚未明确。通过利用STIM1跨膜结构域(STIM1-TM)内独特的功能获得突变,我们在这里显示局部重排而不是STIM1-TM寡聚状态的改变提示盘绕的胞质近膜构象变化-线圈区域。重要的是,我们进一步确定STIM1(STIM1-CT)的胞质结构域内的关键残基,这些残基需要自动抑制。基于这些发现,我们提出了一个模型,其中STIM1-TM重组将STIM1-CT转换为扩展构象,从而将ORAI激活域投影到门ORAI1通道。

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