培养的大鼠骨髓细胞中低电压激活的Ca2+通道电流的电压依赖性增强。

Voltage-dependent potentiation of low-voltage-activated Ca2+ channel currents in cultured rat bone marrow cells.

作者信息

Publicover S J, Preston M R, El Haj A J

机构信息

School of Biological Sciences, University of Birmingham, Edgbaston, UK.

出版信息

J Physiol. 1995 Dec 15;489 ( Pt 3)(Pt 3):649-61. doi: 10.1113/jphysiol.1995.sp021080.

DOI:10.1113/jphysiol.1995.sp021080

PMID:8788931

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1156836/

Abstract

The whole-cell patch-clamp technique was used to study Ca2+ channel currents in stromal cells of 7-10 day dexamethasone-treated and control rat bone marrow cultures. In saline containing either 108 mM Ba2+ or a 2.5 mM Ca(2+)-1 mM Mg2+ mixture, most cells expressed both fast-inactivating, low-voltage-activated (LVA) and slow-inactivating, high-voltage-activated (HVA) currents. 2. Repeated application of 400 ms voltage steps to 60 mV above the holding potential (Vh, -90 mV in Ca(2+)-Mg2+ mixture and -60 mV in Ba2+) at a frequency > or = 0.1 Hz resulted in a potentiation of the LVA component of the 2nd and subsequent currents. 3. LVA current potentiation was examined using a two-pulse (prepulse-test pulse) method. Prepulses to Vh + 150 mV induced an 80-100% increase in the amplitude of the LVA component of Ca2+ channel currents in saline containing either Ba2+ or Ca(2+)-Mg2+. This effect was also seen in non-dexamethasone-treated cultures. 4. Potentiation was not modified by omission of ATP and GTP from the pipette saline, and was not inhibited by extracellular application of the broad spectrum kinase inhibitors H-7 or RK252-a. 5. Potentiation was dependent on the amplitude and duration of the prepulse. Using the standard protocol, the threshold for potentiation was approximately Vh + 45 mV and saturation occurred at Vh + 150-180 mV. Further increases in prepulse amplitude did not modify potentiation. With a prepulse to +10 mV (Ba2+ saline) potentiation was half-maximal with a prepulse duration of 250-300 ms duration and saturated at 750-1000 ms. 6. Peak potentiation occurred 1-2 s after the prepulse. The time for total decay of potentiation varied from 10 to 90 s. 7. Voltage dependency of prepulse-induced potentiation did not resemble that of inactivation induced by similar prepulses. 8. Current kinetics, I-V relationship and sensitivity to blockade by Ni2+ and diphenylhydantoin of prepulse-recruited current resembled those of control LVA current. 9. The amplitude of prepulse-recruited current was positively correlated with control LVA current amplitude. 10. LVA currents supported regenerative potentials under current clamp. Repeated activation reduced spike latency. 11. It is suggested that current potentiation may be recruited physiologically, possibly in association with activation of stretch-sensitive channels, causing enhanced activation of HVA Ca2+ currents.

摘要

采用全细胞膜片钳技术研究地塞米松处理7 - 10天的大鼠骨髓培养物及对照骨髓培养物中基质细胞的Ca2+通道电流。在含有108 mM Ba2+或2.5 mM Ca(2+)-1 mM Mg2+混合物的盐溶液中，大多数细胞同时表达快速失活的低电压激活（LVA）电流和缓慢失活的高电压激活（HVA）电流。2. 以≥0.1 Hz的频率，将400 ms的电压阶跃重复施加到比静息电位（Vh，在Ca(2+)-Mg2+混合物中为 - 90 mV，在Ba2+中为 - 60 mV）高60 mV处，导致第二个及后续电流的LVA成分增强。3. 使用双脉冲（预脉冲 - 测试脉冲）方法检测LVA电流增强。在含有Ba2+或Ca(2+)-Mg2+的盐溶液中，预脉冲至Vh + 150 mV可使Ca2+通道电流的LVA成分幅度增加80 - 100%。在未用地塞米松处理的培养物中也观察到这种效应。4. 从移液管盐溶液中省略ATP和GTP不会改变增强作用，并且细胞外应用广谱激酶抑制剂H - 7或RK252 - a也不会抑制增强作用。5. 增强作用取决于预脉冲的幅度和持续时间。使用标准方案，增强作用的阈值约为Vh + 45 mV，在Vh + 150 - 180 mV时达到饱和。预脉冲幅度进一步增加不会改变增强作用。在Ba2+盐溶液中，预脉冲至 + 10 mV时，增强作用在预脉冲持续时间为250 - 300 ms时达到半最大值，并在750 - 1000 ms时达到饱和。6. 峰值增强作用在预脉冲后1 - 2 s出现。增强作用完全衰减的时间从10到90 s不等。7. 预脉冲诱导的增强作用的电压依赖性与类似预脉冲诱导的失活的电压依赖性不同。8. 预脉冲募集电流的电流动力学、I - V关系以及对Ni2+和苯妥英钠阻断的敏感性与对照LVA电流相似。9. 预脉冲募集电流的幅度与对照LVA电流幅度呈正相关。10. 在电流钳制下，LVA电流支持再生电位。重复激活可缩短动作电位潜伏期。11. 提示电流增强作用可能在生理情况下被募集，可能与牵张敏感通道的激活有关，从而导致HVA Ca2+电流的激活增强。