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细胞内钙离子激活了从人肠系膜动脉分离出的平滑肌细胞中的一个低电导氯通道。

Intracellular calcium ions activate a low-conductance chloride channel in smooth-muscle cells isolated from human mesenteric artery.

作者信息

Klöckner U

机构信息

Department of Physiology, University of Köln, Germany.

出版信息

Pflugers Arch. 1993 Aug;424(3-4):231-7. doi: 10.1007/BF00384347.

Abstract

Calcium-activated chloride currents were studied by the patch-clamp technique in vascular smooth muscle cells (VSMC) isolated from human mesenteric arteries. Bath application of 20 mM caffeine caused the cell membrane to depolarize by a calcium-activated inward current that peaked to -654 +/- 230 pA (holding potential -50 mV). Cell-attached, at the same time inwardly directed single-channel currents were detected with an amplitude of -0.22 pA. In open-cell-attached patches channel activity was triggered by elevating [Ca2+]i to 10 microM. At -60 mV the mean amplitude of the current was -0.24 pA and the mean open time of the channels was 28 ms. Plotting the amplitude of the current versus the test potential yielded a single-channel conductance of 2.8 +/- 0.5 pS. The currents disappeared when [Cl-] was reduced from 150 mM to 5 mM at the cytosolic side of the inside-out patch at a holding potential of -60 mV (calculated reversal potential -58 mV) suggesting that the calcium-activated current was a chloride current. This suggests that, in human mesenteric VSMC, elevation of [Ca2+]i activates a low-conductance chloride channel, which may mediate the agonist-induced depolarization of the cell membrane.

摘要

采用膜片钳技术研究了从人肠系膜动脉分离的血管平滑肌细胞(VSMC)中的钙激活氯电流。浴槽中加入20 mM咖啡因可使细胞膜因钙激活内向电流而去极化,该电流峰值达到-654±230 pA(钳制电位-50 mV)。在细胞贴附式记录中,同时检测到内向单通道电流,幅度为-0.22 pA。在破膜片贴附式记录中,通过将[Ca2+]i升高至10 μM触发通道活动。在-60 mV时,电流的平均幅度为-0.24 pA,通道的平均开放时间为28 ms。绘制电流幅度与测试电位的关系图得出单通道电导为2.8±0.5 pS。在-60 mV的钳制电位下(计算得出的反转电位为-58 mV),当内面向外膜片的胞质侧[Cl-]从150 mM降至5 mM时,电流消失,这表明钙激活电流是氯电流。这表明,在人肠系膜VSMC中,[Ca2+]i升高激活了一个低电导氯通道,该通道可能介导激动剂诱导的细胞膜去极化。

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