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首页> 外文期刊>The Plant Cell >A Novel Calcium Binding Site in the Slow Vacuolar Cation Channel TPC1 Senses Luminal Calcium Levels
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A Novel Calcium Binding Site in the Slow Vacuolar Cation Channel TPC1 Senses Luminal Calcium Levels

机译:TPC1在缓慢的液泡阳离子通道中的新型钙结合位点感知发光钙水平。

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摘要

Cytosolic calcium homeostasis is pivotal for intracellular signaling and requires sensing of calcium concentrations in the cytosol and accessible stores. Numerous Ca2+ binding sites have been characterized in cytosolic proteins. However, little is known about Ca2+ binding inside organelles, like the vacuole. The slow vacuolar (SV) channel, encoded by Arabidopsis thaliana TPC1, is regulated by luminal Ca2+. However, the D454/fou2 mutation in TPC1 eliminates vacuolar calcium sensitivity and increases store calcium content. In a search for the luminal calcium binding site, structure modeling indicated a possible coordination site formed by residues Glu-450, Asp-454, Glu-456, and Glu-457 on the luminal side of TPC1. Each Glu residue was replaced by Gln, the modified genes were transiently expressed in loss-of-TPC1-function protoplasts, and SV channel responses to luminal calcium were recorded by patch clamp. SV channels lacking any of the four negatively charged residues appeared altered in calcium sensitivity of channel gating. Our results indicate that Glu-450 and Asp-454 are directly involved in Ca2+ binding, whereas Glu-456 and Glu-457 are probably involved in connecting the luminal Ca2+ binding site to the channel gate. This novel vacuolar calcium binding site represents a potential tool to address calcium storage in plants.
机译:胞质钙稳态对于细胞内信号传导至关重要,并且需要感测细胞溶质和可及存储中钙的浓度。在胞质蛋白中已鉴定出许多Ca2 +结合位点。但是,关于液泡内部的Ca 2+结合的了解很少。由拟南芥TPC1编码的慢液泡(SV)通道受腔Ca2 +调控。但是,TPC1中的D454 / fou2突变消除了液泡钙敏感性,并增加了储钙量。在寻找腔内钙结合位点的过程中,结构建模表明可能是由TPC1腔侧Glu-450,Asp-454,Glu-456和Glu-457残基形成的配位点。每个Glu残基都被Gln取代,修饰的基因在TPC1功能缺失的原生质体中瞬时表达,并通过膜片钳记录了对腔内钙的SV通道反应。缺少四个带负电残基的SV通道似乎改变了通道门控的钙敏感性。我们的结果表明,Glu-450和Asp-454直接参与Ca2 +结合,而Glu-456和Glu-457可能参与将腔内Ca2 +结合位点连接至通道门。这个新的液泡钙结合位点代表了解决植物中钙储存的潜在工具。

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