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豚鼠输尿管平滑肌细胞中钠钙交换介导的细胞内钙离子浓度变化

Alterations in [Ca2+]i mediated by sodium-calcium exchange in smooth muscle cells isolated from the guinea-pig ureter.

作者信息

Aaronson P I, Benham C D

机构信息

Department of Pharmacology, St George's Hospital Medical School, London.

出版信息

J Physiol. 1989 Sep;416:1-18. doi: 10.1113/jphysiol.1989.sp017745.

Abstract
  1. Sodium-calcium exchange was studied in single enzymatically isolated cells of the guinea-pig ureter using the Ca2(+)-sensitive fluorescent dye Indo-1 to monitor the intracellular Ca2+ concentration ([Ca2+]i). Patch pipettes containing Indo-1 were used to introduce the dye into cells, to set the intracellular Na+ concentration ([Na+]i) and control the membrane potential during experiments. 2. With [Na+]i set at 11-12 mM and a membrane potential of -60 or -70 mV, brief depolarization of ureter cells elicited typical voltage-gated inward currents associated with rapid increases in [Ca2+]i which showed a bell-shaped potential dependence. If Ca2+ currents were blocked with nifedipine, depolarization led to slower rises in [Ca2+]i. The rates and amplitudes of these increased monotonically with progressively larger depolarizations up to +120 mV. 3. The nifedipine-resistant rises in [Ca2+]i elicited by depolarization were potentiated when the extracellular sodium concentration ([Na+]o) was reduced. Basal levels of [Ca2+]i also increased as [Na+]o was reduced, although the dependence of this effect on [Na+]o was smaller than would be predicted if [Ca2+]i was set only by a Na(+)-Ca2+ exchange process. 4. The nifedipine-insensitive rises in [Ca2+]i elicited by depolarization were potentiated at higher basal levels of [Ca2+]i. 5. The ability of cells to reduce [Ca2+]i rapidly following Ca2+ loading during voltage-gated transients was markedly inhibited if the Na+ concentration gradient was reversed, but was little affected if the Na+ gradient was decreased by 25 or 50%. Recovery from a Ca2+ load caused by reversal of the Na+ gradient could be induced by removal of Cao2+ in the continuing absence of Nao+, indicating the importance of a Na(+)-independent [Ca2+]i-lowering system. 6. The results demonstrate that Na(+)-Ca2+ exchange can modulate [Ca2+]i when [Na+]i and the membrane potential are set at or near their physiological levels in these smooth muscle cells. [Ca2+]i does not, however, appear to be markedly sensitive to the Na+ concentration gradient under the conditions employed for these experiments, suggesting that a Na(+)-independent Ca2+ extrusion system is mainly responsible for regulating [Ca2+]i under normal conditions.
摘要
  1. 使用对Ca2+敏感的荧光染料Indo-1监测豚鼠输尿管单个酶分离细胞内的Ca2+浓度([Ca2+]i),研究钠钙交换。含有Indo-1的膜片吸管用于将染料引入细胞,设定细胞内Na+浓度([Na+]i)并在实验过程中控制膜电位。2. 当[Na+]i设定为11 - 12 mM且膜电位为 - 60或 - 70 mV时,输尿管细胞的短暂去极化引发典型的电压门控内向电流,伴随着[Ca2+]i的快速增加,呈现钟形电位依赖性。如果用硝苯地平阻断Ca2+电流,去极化会导致[Ca2+]i上升较慢。这些上升的速率和幅度随着去极化程度逐渐增大直至 + 120 mV而单调增加。3. 当细胞外钠浓度([Na+]o)降低时,去极化引起的对硝苯地平不敏感的[Ca2+]i上升增强。随着[Na+]o降低,[Ca2+]i的基础水平也增加,尽管这种效应对[Na+]o的依赖性小于如果[Ca2+]i仅由Na(+)-Ca2+交换过程设定时的预测值。4. 在较高的[Ca2+]i基础水平下,去极化引起的对硝苯地平不敏感的[Ca2+]i上升增强。5. 如果Na+浓度梯度反转,在电压门控瞬变期间Ca2+加载后细胞快速降低[Ca2+]i的能力会受到显著抑制,但如果Na+梯度降低25%或50%则影响较小。在持续不存在Nao+的情况下,通过去除Cao2+可诱导由Na+梯度反转引起的Ca2+负荷的恢复,这表明存在一个不依赖Na+的[Ca2+]i降低系统的重要性。6. 结果表明,在这些平滑肌细胞中,当[Na+]i和膜电位设定在或接近其生理水平时,Na(+)-Ca2+交换可调节[Ca2+]i。然而,在这些实验所采用的条件下,[Ca2+]i似乎对Na+浓度梯度不敏感,这表明在正常情况下,一个不依赖Na+的Ca2+排出系统主要负责调节[Ca2+]i。

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