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Orai proteins interact with TRPC channels and confer responsiveness to store depletion

机译:Orai蛋白与TRPC通道相互作用并赋予响应能力以存储耗尽

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The TRPC (C-type transient receptor potential) class of ion channels has been hypothesized to participate in store-operated Ca~(2+) entry (SOCE). Recently, however, STIM1 and Orai1 proteins have been proposed to form SOCE channels. Whether TRPCs participate in SOCE that is dependent on or regulated by Orai has not been explored. Here we show that Orai1 physically interacts with the N and C termini of TRPC3 and TRPC6, and that in cells overexpressing either TRPC3 or TRPC6 in a store-depletion insensitive manner, these TRPCs become sensitive to store depletion upon expression of an exogenous Orai. Thus, Orai-1, -2, and -3 enhanced thapsi-gargin-induced calcium entry by 50-150% in cells stably overexpressing either TRPC3 or TRPC6. Orai1 expression had no significant effect on endogenous, thapsigargin-induced calcium entry in wild-type cells (HEK-293, COS1), in HEK cells expressing a thapsigargin-sensitive variant of TRPC3 (TRPC3a), or in HEK cells overexpressing another membrane protein, V1aR. Single-channel cation currents present in membrane patches of TRPC3-overexpressing cells were suppressed by expression of Orai1. We propose that Orai proteins by interacting with TRPCs act as regulatory subunits that confer STIM1-mediated store depletion sensitivity to these channels.
机译:假设离子通道的TRPC(C型瞬态受体电位)类别参与了存储操作的Ca〜(2+)条目(SOCE)。然而,最近,已经提出了STIM1和Orai1蛋白形成SOCE通道。尚未探讨TRPC是否参与依赖Orai或由Orai监管的SOCE。在这里,我们显示Orai1与TRPC3和TRPC6的N和C末端发生物理相互作用,并且在过度表达TRPC3或TRPC6的细胞中,以存储耗尽不敏感的方式,这些TRPC在表达外源Orai后变得对存储耗尽敏感。因此,在稳定过量表达TRPC3或TRPC6的细胞中,Orai-1,-2和-3使thapsi-gargin诱导的钙进入增加了50-150%。 Orai1的表达对野生型细胞(HEK-293,COS1),表达thapsigargin敏感的TRPC3变体(TRPC3a)的HEK细胞或过表达另一种膜蛋白的HEK细胞中内生的毒胡萝卜素诱导的钙进入均无明显影响,V1aR。 Orai1的表达抑制了TRPC3过表达细胞的膜片中存在的单通道阳离子电流。我们建议Orai蛋白通过与TRPCs相互作用作为调节亚基,赋予STIM1介导的存储耗尽敏感性这些通道。

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