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细胞外钾、镁和钙浓度变化对大鼠海马脑片CA1区和齿状回突触传递的影响。

Effects of changes in extracellular potassium, magnesium and calcium concentration on synaptic transmission in area CA1 and the dentate gyrus of rat hippocampal slices.

作者信息

Rausche G, Igelmund P, Heinemann U

机构信息

Institut für Neurophysiologie, Zentrum für Physiologie und Pathophysiologie, Universität, zu Köln, Federal Republic of Germany.

出版信息

Pflugers Arch. 1990 Feb;415(5):588-93. doi: 10.1007/BF02583510.

Abstract

The dependence of stimulus-induced synaptic potentials on changes of extracellular ionic concentrations of potassium ([K+]o 3, 5, 8 mM), magnesium ([Mg2+]o 2, 4, 8 mM) and calcium [Ca2+]o (2 mM and continuous lowering by washing with Ca2(+)-free solutions) was investigated in area CA1 and dentate gyrus of rat hippocampal slices. Field potentials (fps), [K+]o and [Ca2+]o were measured with double-barreled ion selective/reference microelectrodes. Paired pulse stimulation (interval 50-ms) was applied either to the lateral perforant path or to the Schaffer collaterals. Elevation of [K+]o from 5 to 8 mM and of [Mg2+]o from 2 to 8 mM depressed the rise of excitatory postsynaptic potentials, as well as the amplitude of population spikes. With elevation of [K+]o, the effect was stronger in the dentate gyrus, while with elevation of [Mg2+]o, the reduction was more pronounced in area CA1. During washout of Ca2+, synaptic potentials became reduced and finally depressed. The [Ca2+]o at which synaptic transmission was blocked increased with higher [Mg2+]o and decreased with a change of [K+]o from 3 to 5 mM, whereas with an elevation of [K+]o from 5 to 8 mM, it rose in area CA1 but was reduced in dentate gyrus. All ionic changes also affected frequency habituation and potentiation in paired pulse experiments. In dentate gyrus, frequency habituation was reversed to frequency potentiation with moderate lowering of [Ca2+]o and with elevation of [Mg2+]o and [K+]o. In contrast, in area CA1 frequency potentiation was reduced upon elevation of [K+]o.

摘要

在大鼠海马切片的CA1区和齿状回中,研究了刺激诱导的突触电位对细胞外钾离子浓度([K+]o分别为3、5、8 mM)、镁离子浓度([Mg2+]o分别为2、4、8 mM)和钙离子浓度[Ca2+]o(2 mM,并通过用无钙溶液冲洗持续降低)变化的依赖性。用场电位(fps)、[K+]o和[Ca2+]o的双管离子选择性/参比微电极进行测量。对侧穿通通路或Schaffer侧支施加配对脉冲刺激(间隔50毫秒)。将[K+]o从5 mM升高到8 mM以及将[Mg2+]o从2 mM升高到8 mM会抑制兴奋性突触后电位的上升以及群体峰电位的幅度。随着[K+]o升高,齿状回中的效应更强,而随着[Mg2+]o升高,CA1区的降低更明显。在冲洗掉Ca2+的过程中,突触电位降低并最终受到抑制。阻断突触传递时的[Ca2+]o随着[Mg2+]o升高而增加,随着[K+]o从3 mM变为5 mM而降低,而随着[K+]o从5 mM升高到8 mM,它在CA1区升高但在齿状回中降低。所有离子变化也影响配对脉冲实验中的频率习惯化和增强。在齿状回中,随着[Ca2+]o适度降低以及[Mg2+]o和[K+]o升高,频率习惯化转变为频率增强。相反,在CA1区,随着[K+]o升高,频率增强降低。

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