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Capacitative Ca2+ Entry Is Closely Linked to the Filling State of Internal Ca2+ Stores: A Study Using Simultaneous Measurements of ICRAC and Intraluminal [Ca2+]

机译:电容性Ca2 +进入与内部Ca2 +存储的填充状态紧密相关:一项使用ICRAC和腔内[Ca2 +]同时测量的研究

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摘要

ICRAC (the best characterized Ca2+ current activated by store depletion) was monitored concurrently for the first time with [Ca2+] changes in internal stores. To establish the quantitative and kinetic relationship between these two parameters, we have developed a novel means to clamp [Ca2+] within stores of intact cells at any level. The advantage of this approach, which is based on the membrane-permeant low-affinity Ca2+ chelator N,N,N′,N′-tetrakis (2-pyridylmethyl)ethylene diamine (TPEN), is that [Ca2+] within the ER can be lowered and restored to its original level within 10–15 s without modifications of Ca2+ pumps or release channels. Using these new tools, we demonstrate here that Ca2+ release–activated Ca2+ current (ICRAC) is activated (a) solely by reduction of free [Ca2+] within the ER and (b) by any measurable decrease in [Ca2+]ER. We also demonstrate that the intrinsic kinetics of inactivation are relatively slow and possibly dependent on soluble factors that are lost during the whole-cell recording.
机译:首次同时通过内部存储中的[Ca2 +]变化对ICRAC(通过存储耗尽激活的最有特征的Ca2 +电流)进行了监视。为了建立这两个参数之间的定量和动力学关系,我们开发了一种新颖的方法来将[Ca2 +]夹在任何水平的完整细胞中。这种方法的优势是基于膜渗透性低亲和力的Ca2 +螯合剂N,N,N',N'-四(2-吡啶甲基)乙二胺(TPEN),它可以使ER内的[Ca2 +]无需修改Ca2 +泵或释放通道,即可在10-15 s内将其降低并恢复到原始水平。使用这些新工具,我们在此处证明了Ca2 +释放激活的Ca2 +电流(ICRAC)被激活(a)仅通过减少ER中的游离[Ca2 +]和(b)通过[Ca2 +] ER的任何可测量的降低来激活。我们还证明灭活的内在动力学相对较慢,可能取决于全细胞记录过程中丢失的可溶性因子。

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