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豚鼠心脏细胞中通过T型Ca2+通道的生理离子通量的宏观和整体特性。

Macroscopic and unitary properties of physiological ion flux through T-type Ca2+ channels in guinea-pig heart cells.

作者信息

Balke C W, Rose W C, Marban E, Wier W G

机构信息

University of Maryland, School of Medicine, Department of Physiology, Baltimore 21201.

出版信息

J Physiol. 1992 Oct;456:247-65. doi: 10.1113/jphysiol.1992.sp019335.

Abstract
  1. We sought to distinguish two types of Ca2+ channel in guinea-pig ventricular cells (T-type and L-type) and to characterize their respective gating and permeation properties when Ca2+ (1-10 mM) is the charge carrier, as is the case physiologically. 2. Na+ was removed from both the external and internal solutions to eliminate currents through Na+ channels and Na(+)-Ca2+ exchange. Major differences in the voltage dependence of steady-state inactivation were exploited to separate the two Ca2+ current components. 3. From a holding potential of -50 mV, only L-type channels were available to open with depolarization. When holding at -90 mV, T-type channels contributed an additional rapidly inactivating component superimposed upon the L-type current. Only the L-type channels thus identified were sensitive to the dihydropyridine Ca2+ channel blocker nitrendipine. 4. T-type currents, measured by taking the difference between the currents elicited from a holding potential of -90 mV and those elicited from -50 mV, peaked within 10 ms and decayed completely within 50-100 ms. 5. Macroscopic T-type currents were largest during depolarizing pulses between -40 and -30 mV (peak current density of 0.62 +/- 0.21 nA nF-1) and decreased at more positive potentials, becoming unmeasurably small above 0 mV. 6. Unitary currents recorded with similar ionic conditions and voltage protocols exhibited a single-channel conductance of 4-5 pS in 10 mM Ca2+. Ensemble average currents through a single channel reproduced accurately the time course of whole-cell T-type current. Permeation properties could not explain the absence of macroscopic T-type currents at positive test potentials, which must therefore be attributable to gating. 7. Convolution analysis was employed to clarify the single-channel basis of the rapidly decaying current waveform of T-type channels. The latencies to first opening and reopening, which reflect activation and deactivation, influenced the waveform most strikingly. Open times were sufficiently brief that they contributed little to shaping the average current. Thus, macroscopic inactivation largely reflects rate-limiting activation events. 8. The unitary current amplitudes and peak open probabilities measured for single T-type channels, when compared to the average macroscopic T-type current density, predict 10.6 functional channels per picofarad, or approximately 1700 T-type channels per typical ventricular myocyte.
摘要
  1. 我们试图区分豚鼠心室肌细胞中的两种钙通道(T型和L型),并在生理情况下钙离子(1 - 10 mM)作为电荷载体时,描述它们各自的门控和通透特性。2. 从细胞外液和细胞内液中去除钠离子,以消除通过钠通道和钠钙交换产生的电流。利用稳态失活电压依赖性的主要差异来分离两种钙电流成分。3. 从 - 50 mV的钳制电位开始,去极化时只有L型通道可被激活开放。当钳制在 - 90 mV时,T型通道在L型电流上叠加了一个额外的快速失活成分。如此鉴定出的只有L型通道对二氢吡啶类钙通道阻滞剂尼群地平敏感。4. T型电流通过测量从 - 90 mV钳制电位诱发的电流与从 - 50 mV钳制电位诱发的电流之间的差值来测定,在10 ms内达到峰值,并在50 - 100 ms内完全衰减。5. 宏观T型电流在 - 40至 - 30 mV的去极化脉冲期间最大(峰值电流密度为0.62±0.21 nA nF⁻¹),在更正的电位下减小,在0 mV以上变得小到无法测量。6. 在相似的离子条件和电压方案下记录的单通道电流,在10 mM钙离子中显示单通道电导为4 - 5 pS。通过单个通道的整体平均电流准确地再现了全细胞T型电流的时间进程。通透特性无法解释在正测试电位下宏观T型电流的缺失,因此这一定归因于门控。7. 采用卷积分析来阐明T型通道快速衰减电流波形的单通道基础。首次开放和重新开放的延迟反映了激活和失活,对波形影响最为显著。开放时间足够短暂,对平均电流的形成贡献不大。因此,宏观失活在很大程度上反映了限速激活事件。8. 将单个T型通道测量的单通道电流幅度和峰值开放概率与平均宏观T型电流密度相比,预测每皮法有10.6个功能通道,或每个典型心室肌细胞约有1700个T型通道。

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