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突触前延迟整流钾电流对鱿鱼巨大突触递质释放的调节

Regulation of transmitter release at the squid giant synapse by presynaptic delayed rectifier potassium current.

作者信息

Augustine G J

机构信息

Department of Biological Sciences, University of Southern California, Los Angeles 90089-2520.

出版信息

J Physiol. 1990 Dec;431:343-64. doi: 10.1113/jphysiol.1990.sp018333.

Abstract
  1. The three-microelectrode voltage clamp technique and pharmacological agents were used to examine the properties and functions of potassium currents in squid giant presynaptic terminals. 2. Outward currents consisted of two components: a slow component which activated over hundreds of milliseconds and was blocked by extracellular application of tetraethylammonium (TEA) ions and a more rapidly activating component which was relatively insensitive to extracellular TEA. 3. The more rapid component was studied in isolation by treating presynaptic terminals with extracellular TEA, as well as tetrodotoxin (to block sodium channel currents) and manganese (to block calcium channel currents). The magnitude of this current component was 1-2 mA cm-2 at 0 mV. Rates of activation and deactivation were voltage dependent and little evidence of inactivation was seen for depolarizations less than several seconds in duration. 4. The reversal potential of the current was -70 to -80 mV in normal saline and became more positive with elevated extracellular potassium concentrations, suggesting that potassium is the primary permeant ion. Accumulation of extracellular potassium appeared to be marked during depolarizations that produced significant activation of the current. 5. Extracellular application of 3,4-diaminopyridine (DAP) blocked the current with an apparent dissociation constant of 7 microM at 0 mV. Intracellular applications of DAP and TEA also were effective in reducing this current. These treatments, but not extracellular TEA application, broadened presynaptic action potentials and increased the magnitude and time-to-peak of postsynaptic currents elicited by the broadened presynaptic action potentials. Postsynaptic currents were a sensitive and linear function of action potential duration; a 30% increase in action potential duration increased postsynaptic current amplitude by 190%. 6. Estimation of the magnitude and time course of the presynaptic calcium current, based on previous measurements of calcium channel gating, indicated that action potential broadening produces a large increase in calcium current magnitude. These calculations predict that a 30% increase in presynaptic action potential duration will increase the peak amplitude of the calcium current by approximately 170% and the total amount of calcium entry by approximately 230%. This implies a linear relationship between transmitter release and calcium entry during an action potential and can be explained by assuming that calcium co-operatively triggers release within intracellular domains that do not overlap.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 采用三微电极电压钳技术和药理学试剂来研究枪乌贼巨大突触前终末钾电流的特性和功能。2. 外向电流由两个成分组成:一个缓慢成分,其在数百毫秒内激活,可被细胞外施加的四乙铵(TEA)离子阻断;另一个激活更快的成分,对细胞外TEA相对不敏感。3. 通过用细胞外TEA以及河豚毒素(以阻断钠通道电流)和锰(以阻断钙通道电流)处理突触前终末,对更快的成分进行了单独研究。在0 mV时,该电流成分的大小为1 - 2 mA/cm²。激活和失活速率依赖于电压,对于持续时间小于几秒的去极化,几乎没有失活的迹象。4. 在正常盐溶液中,电流的反转电位为 - 70至 - 80 mV,随着细胞外钾浓度升高而变得更正,表明钾是主要的通透离子。在产生该电流显著激活的去极化过程中,细胞外钾的积累似乎很明显。5. 细胞外施加3,4 - 二氨基吡啶(DAP)以7 microM的表观解离常数在0 mV时阻断该电流。细胞内施加DAP和TEA也有效地降低了该电流。这些处理,但不是细胞外施加TEA,拓宽了突触前动作电位,并增加了由拓宽的突触前动作电位引发的突触后电流的幅度和峰值时间。突触后电流是动作电位持续时间的敏感且线性函数;动作电位持续时间增加30%会使突触后电流幅度增加190%。6. 根据先前对钙通道门控的测量来估计突触前钙电流的大小和时间进程,表明动作电位拓宽会使钙电流大小大幅增加。这些计算预测,突触前动作电位持续时间增加30%将使钙电流的峰值幅度增加约170%,钙内流总量增加约230%。这意味着在动作电位期间递质释放与钙内流之间存在线性关系,并且可以通过假设钙在不重叠的细胞内区域协同触发释放来解释。(摘要截取自400字)

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