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N-甲基-D-天冬氨酸激活大鼠海马锥体细胞中的电压依赖性钙电导。

N-methyl aspartate activates voltage-dependent calcium conductance in rat hippocampal pyramidal cells.

作者信息

Dingledine R

出版信息

J Physiol. 1983 Oct;343:385-405. doi: 10.1113/jphysiol.1983.sp014899.

Abstract

The depolarizing actions of N-methyl-DL-aspartate (NMA) and L-glutamate on pyramidal neurones were compared in a hippocampal slice preparation. Tetrodotoxin (1 microM) was added to the perfusion solution to suppress regenerative Na conductances. Depolarization evoked by ionophoretic application of NMA triggered slow, high-threshold regenerative spikes. These are considered to be Ca spikes since the amplitude and rate of rise could be reduced by verapamil, D-600, Co2+ and Mn2+, and increased by Ba2+. Multiple Ca-spike thresholds could be demonstrated in the same cell. In contrast, depolarizations evoked by L-glutamate only rarely triggered Ca-spikes. The minimum latency to the onset of depolarization evoked by NMA was less than 20 ms. The latency and amplitude of NMA-evoked responses were highly dependent on the position of the ionophoretic pipette; movements of the pipette by as little as 10-50 micron could markedly change the size of the response. Spatially separate hot spots for NMA and glutamate were not found. Depolarizations evoked by small to moderate ionophoretic currents of NMA were usually associated with an apparent rise in input resistance, as tested by the response to transmembrane current pulses. Ionophoresis of L-glutamate, or high NMA doses, however, usually caused a fall in input resistance. Both the depolarization and the conductance change evoked by NMA were highly voltage-dependent within the approximate range -50 to -80 mV; they could be increased by modest depolarization and reduced by hyperpolarization of the membrane. No reversal potential could be demonstrated in the hyperpolarizing direction. Rather, the NMA response approached zero asymptotically at sufficiently hyperpolarized membrane potentials. Subthreshold depolarizations and conductance changes elicited by NMA could be blocked by Co2+, Mn2+ and Cd2+, and reduced by D-600 and verapamil. These Ca2+ antagonists had little or no effect on resting membrane potential or input resistance, or on responses to L-glutamate. Ba2+ increased the amplitude of subthreshold NMA responses. Intracellular injection of Cs+ plus tetraethylammonium caused cells to fire large, prolonged (up to 15 s) Ca spikes, presumably because most K+ conductances were blocked. Under these conditions the effect of NMA was unchanged or enhanced. Raising [K+]o to 10.5 mM (from the normal 3.5 mM) caused a depolarization and fall in input resistance, but did not change the amplitude or voltage dependence of the NMA response. Reducing [Na+]o caused an initial increase, then usually a delayed decrease in the amplitude of the NMA response.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

在海马脑片标本中比较了N-甲基-DL-天冬氨酸(NMA)和L-谷氨酸对锥体细胞的去极化作用。将河豚毒素(1微摩尔)加入灌流液中以抑制再生性钠电导。通过离子电泳施加NMA引起的去极化触发了缓慢的、高阈值的再生性动作电位。这些被认为是钙动作电位,因为其幅度和上升速率可被维拉帕米、D-600、Co2+和Mn2+降低,并被Ba2+增加。在同一细胞中可显示多个钙动作电位阈值。相比之下,L-谷氨酸引起的去极化很少触发钙动作电位。NMA引起的去极化开始的最短潜伏期小于20毫秒。NMA诱发反应的潜伏期和幅度高度依赖于离子电泳微电极的位置;微电极移动仅10 - 50微米就能显著改变反应的大小。未发现NMA和谷氨酸在空间上分离的热点。如通过对跨膜电流脉冲的反应所测试的,由小到中等离子电泳电流的NMA引起的去极化通常与输入电阻的明显增加相关。然而,L-谷氨酸的离子电泳或高剂量的NMA通常会导致输入电阻下降。NMA引起的去极化和电导变化在约-50至-80毫伏的范围内高度依赖于电压;它们可通过适度去极化增加,通过膜的超极化降低。在超极化方向未显示反转电位。相反,在足够超极化的膜电位下,NMA反应渐近地接近零。NMA引起的阈下去极化和电导变化可被Co2+、Mn2+和Cd2+阻断,并被D-600和维拉帕米降低。这些钙拮抗剂对静息膜电位或输入电阻或对L-谷氨酸的反应几乎没有影响。Ba2+增加了阈下NMA反应的幅度。细胞内注射Cs+加四乙铵导致细胞发放大的、持续时间长(长达15秒)的钙动作电位,推测是因为大多数钾电导被阻断。在这些条件下,NMA的作用未改变或增强。将[K+]o从正常的3.5毫摩尔提高到10.5毫摩尔导致去极化和输入电阻下降,但未改变NMA反应的幅度或电压依赖性。降低[Na+]o导致NMA反应幅度先增加,然后通常延迟下降。(摘要截短于400字)

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