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定量分析ATP门控P2X7受体中的钙离子电流和通透性。

Quantifying Ca2+ current and permeability in ATP-gated P2X7 receptors.

作者信息

Liang Xin, Samways Damien S K, Wolf Kyle, Bowles Elizabeth A, Richards Jennifer P, Bruno Jonathan, Dutertre Sébastien, DiPaolo Richard J, Egan Terrance M

机构信息

From the Department of Pharmacological and Physiological Science and Center for Neuroscience, and.

the Department of Biology, Clarkson University, Potsdam, New York 13699, and.

出版信息

J Biol Chem. 2015 Mar 20;290(12):7930-42. doi: 10.1074/jbc.M114.627810. Epub 2015 Feb 2.

Abstract

ATP-gated P2X7 receptors are prominently expressed in inflammatory cells and play a key role in the immune response. A major consequence of receptor activation is the regulated influx of Ca(2+) through the self-contained cation non-selective channel. Although the physiological importance of the resulting rise in intracellular Ca(2+) is universally acknowledged, the biophysics of the Ca(2+) flux responsible for the effects are poorly understood, largely because traditional methods of measuring Ca(2+) permeability are difficult to apply to P2X7 receptors. Here we use an alternative approach, called dye-overload patch-clamp photometry, to quantify the agonist-gated Ca(2+) flux of recombinant P2X7 receptors of dog, guinea pig, human, monkey, mouse, rat, and zebrafish. We find that the magnitude of the Ca(2+) component of the ATP-gated current depends on the species of origin, the splice variant, and the concentration of the purinergic agonist. We also measured a significant contribution of Ca(2+) to the agonist-gated current of the native P2X7Rs of mouse and human immune cells. Our results provide cross-species quantitative measures of the Ca(2+) current of the P2X7 receptor for the first time, and suggest that the cytoplasmic N terminus plays a meaningful role in regulating the flow of Ca(2+) through the channel.

摘要

三磷酸腺苷(ATP)门控的P2X7受体在炎症细胞中大量表达,并在免疫反应中起关键作用。受体激活的一个主要后果是通过其自身包含的非选择性阳离子通道调节钙离子(Ca(2+))内流。尽管细胞内Ca(2+)浓度升高的生理重要性已得到普遍认可,但对产生这些效应的Ca(2+)通量的生物物理学了解甚少,这主要是因为传统的测量Ca(2+)通透性的方法难以应用于P2X7受体。在此,我们采用一种称为染料过载膜片钳光度法的替代方法,来量化犬、豚鼠、人、猴、小鼠、大鼠和斑马鱼重组P2X7受体的激动剂门控Ca(2+)通量。我们发现,ATP门控电流中Ca(2+)成分的大小取决于受体的来源物种、剪接变体以及嘌呤能激动剂的浓度。我们还测量了Ca(2+)对小鼠和人类免疫细胞天然P2X7受体激动剂门控电流的显著贡献。我们的结果首次提供了跨物种的P2X7受体Ca(2+)电流的定量测量,并表明胞质N末端在调节Ca(2+)通过通道的流动中发挥了重要作用。

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