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豚鼠胃窦单个平滑肌细胞膜电流的特性分析。

Characterization of membrane currents in single smooth muscle cells from the guinea-pig gastric antrum.

作者信息

Noack T, Deitmer P, Lammel E

机构信息

Department of Physiology, Philipps University, Marburg, FRG.

出版信息

J Physiol. 1992;451:387-417. doi: 10.1113/jphysiol.1992.sp019170.

Abstract
  1. Smooth muscle cells, enzymatically isolated from the antrum of the guinea-pig stomach, were voltage clamped at room temperature using the whole-cell patch clamp technique. In physiological salt solution (PSS), step depolarization from a holding potential of -90 mV elicited inward calcium current (ICa) followed and superimposed by outward potassium current. 2. Outward current was divided into components depending on the presence of extracellular Ca2+ and others which were not activated as a result of Ca2+ influx. Ca(2+)-dependent components were (1) a fast transient component most likely representing Ca(2+)-activated K+ current (IK(Ca)) immediately triggered by the initial peak of ICa and (2) spontaneous transient outward currents (STOCs) apparently reflecting synchronized opening of IK(Ca) channels by cyclic release of Ca2+ from intracellular stores. Ca2+ influx-independent outward current could be divided into two main components: (1) a transient component (I(to)) showing voltage-dependent activation and inactivation and (2) a non-inactivating component (Ini). 3. I(to) activated with a threshold around -30 mV, was fully available at -90 mV and completely inactivated at -10 mV. The time course of both activation and inactivation of I(to) at different potentials could be described by single exponential functions. Time constants of activation decreased from 35 ms at -10 mV to 10 ms at +40 mV. The time constant of inactivation was about 2 s and only weakly voltage dependent. Time constants for exponentially developing recovery from inactivation of I(to) ranged from 0.1 s at -100 mV to 10 s at -30 mV. I(to) was insensitive to 4-aminopyridine (4-AP, 5 mmol/l), slightly sensitive to tetraethylammonium (TEA, 10 mmol/l), but substantially inhibited by caffeine (10 mmol/l) and Cd2+ (5 mmol/l). Estimates of the single-channel conductance by current fluctuation analysis indicated a small value of about 2.5 pS. 4. The action of TEA on current elicited from a holding potential of -10 mV indicated a major contribution to Ini of a distinct component (Ini,K) that was completely blocked by this substance at a concentration of 10 mmol/l. Ini was almost unaffected by 4-AP (5 mmol/l) and caffeine (10 mmol/l), but strongly suppressed by Cd2+ (5 mmol/l). Current fluctuation analysis of Ini,K gave a value for the single-channel conductance of about 60 pS. 5. Ca2+ inward current was studied in PSS ([Ca2+]o = 2.5 mmol/l) using pipette solution in which K+ was replaced by Cs+ to suppress outward K+ currents.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 采用全细胞膜片钳技术,在室温下对从豚鼠胃窦部酶解分离出的平滑肌细胞进行电压钳制。在生理盐溶液(PSS)中,从 -90 mV 的钳制电位进行阶跃去极化,可引发内向钙电流(ICa),随后有外向钾电流叠加在其上。2. 外向电流根据细胞外 Ca2+ 的存在情况分为不同成分,以及其他不因 Ca2+ 内流而激活的成分。依赖 Ca2+ 的成分有:(1)一个快速瞬变成分,很可能代表由 ICa 的初始峰值立即触发的 Ca2+ 激活钾电流(IK(Ca));(2)自发瞬态外向电流(STOCs),显然反映了细胞内钙库中 Ca2+ 的周期性释放使 IK(Ca) 通道同步开放。不依赖 Ca2+ 内流的外向电流可分为两个主要成分:(1)一个瞬变成分(I(to)),表现出电压依赖性激活和失活;(2)一个非失活成分(Ini)。3. I(to) 在约 -30 mV 的阈值下激活,在 -90 mV 时完全可用,在 -10 mV 时完全失活。I(to) 在不同电位下的激活和失活时间进程可用单指数函数描述。激活时间常数从 -10 mV 时的 35 ms 降至 +40 mV 时的 10 ms。失活时间常数约为 2 s,且仅对电压有微弱依赖性。I(to) 从失活状态指数性恢复的时间常数范围从 -100 mV 时的 0.1 s 到 -30 mV 时的 10 s。I(to) 对 4 - 氨基吡啶(4 - AP, 5 mmol/l)不敏感,对四乙铵(TEA, 10 mmol/l)稍有敏感,但被咖啡因(10 mmol/l)和 Cd2+(5 mmol/l)显著抑制。通过电流波动分析对单通道电导的估计表明其值约为 2.5 pS。4. TEA 对从 -10 mV 的钳制电位引发的电流的作用表明,一种独特成分(Ini,K)对 Ini 有主要贡献,该成分在 10 mmol/l 的浓度下被这种物质完全阻断。Ini 几乎不受 4 - AP(5 mmol/l)和咖啡因(10 mmol/l)影响,但被 Cd2+(5 mmol/l)强烈抑制。对 Ini,K 的电流波动分析得出单通道电导值约为 60 pS。5. 在 PSS([Ca2+]o = 2.5 mmol/l)中,使用用 Cs+ 替代 K+ 的移液管溶液来抑制外向 K+ 电流,研究 Ca2+ 内向电流。(摘要截取自 400 字)

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