去极化诱发的钙离子释放发生在一种非兴奋性细胞——大鼠巨核细胞中。
Depolarization-evoked Ca2+ release in a non-excitable cell, the rat megakaryocyte.
作者信息
Mahaut-Smith M P, Hussain J F, Mason M J
机构信息
Department of Physiology, University of Cambridge, Downing Street, Cambridge CB2 3EG, UK.
出版信息
J Physiol. 1999 Mar 1;515 ( Pt 2)(Pt 2):385-90. doi: 10.1111/j.1469-7793.1999.385ac.x.
Abstract
- The effect of membrane potential on [Ca2+]i in rat megakaryocytes was studied using simultaneous whole-cell patch clamp and fura-2 fluorescence recordings. 2. Depolarization from -75 to 0 mV had no effect on [Ca2+]i in unstimulated cells, but evoked one or more spikes of Ca2+ increase (peak increase: 714 +/- 95 nM) during activation of metabotropic purinoceptors by 1 microM ADP. 3. The depolarization-evoked Ca2+ increase was present in Ca2+-free medium and also following removal of Na+. Thus depolarization mobilizes Ca2+ from an intracellular store without a requirement for altered Na+-Ca2+ exchange activity. 4. Intracellular dialysis with heparin blocked the depolarization-evoked Ca2+ increase, indicating a role for functional IP3 receptors. 5. Under current clamp, ADP caused the membrane potential to fluctuate between -43 +/- 1 and -76 +/- 1 mV. Under voltage clamp, depolarization from -75 to -45 mV evoked a transient [Ca2+]i increase (398 +/- 91 nM) during exposure to ADP. 6. We conclude that during stimulation of metabotropic purinoceptors, membrane depolarization over the physiological range can stimulate Ca2+ release from intracellular stores in the rat megakaryocyte, a non-excitable cell type. This may represent an important mechanism by which electrogenic influences can control patterns of [Ca2+]i increase.
摘要
- 采用全细胞膜片钳和fura-2荧光同步记录技术,研究了膜电位对大鼠巨核细胞胞内钙离子浓度([Ca2+]i)的影响。2. 从-75 mV去极化到0 mV对未受刺激细胞的[Ca2+]i无影响,但在1 μM ADP激活代谢型嘌呤受体时,可诱发一次或多次钙离子浓度升高峰(峰值升高:714±95 nM)。3. 在无钙培养基中以及去除钠离子后,去极化诱发的钙离子浓度升高依然存在。因此,去极化可从细胞内储存库中动员钙离子,而无需改变钠钙交换活性。4. 用肝素进行细胞内透析可阻断去极化诱发的钙离子浓度升高,表明功能性肌醇三磷酸(IP3)受体发挥了作用。5. 在电流钳模式下,ADP使膜电位在-43±1 mV和-76±1 mV之间波动。在电压钳模式下,从-75 mV去极化到-45 mV在暴露于ADP期间诱发了短暂的[Ca2+]i升高(398±91 nM)。6. 我们得出结论,在代谢型嘌呤受体受刺激期间,生理范围内的膜去极化可刺激大鼠巨核细胞(一种非兴奋性细胞类型)从细胞内储存库释放钙离子。这可能代表了一种重要机制,通过该机制电源性影响可控制[Ca2+]i升高模式。
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