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海马体中钙诱导的长时程增强效应。

Calcium-induced long-term potentiation in the hippocampus.

作者信息

Turner R W, Baimbridge K G, Miller J J

出版信息

Neuroscience. 1982 Jun;7(6):1411-6. doi: 10.1016/0306-4522(82)90254-8.

Abstract

The effect of a transient increase in extracellular calcium concentration on the Schaffer collateral-commissural evoked excitatory postsynaptic potential and population spike responses of CAI pyramidal neurons was investigated using the rat in vitro hippocampal slice preparation. Brief exposure of slices (5-10 min) to twice the normal concentration of calcium (4 mM) induced a marked potentiation of both the excitatory postsynaptic potential and population spike that could persist for at least 3 h. No long-term changes were observed in either the presynaptic fiber volley of antidromically evoked CAI population spike, indicating that the potentiation could not be attributed to an increase in the number of fibers activated or a generalized increase in cellular excitability. The response of CAI pyramidal neurons to the iontophoretic application of L-glutamate in the apical dendritic zone was also unaffected after exposure to high calcium perfusate, suggesting a lack of alteration in membrane excitability or receptor sensitivity restricted to the region of synaptic input. In addition, total intracellular calcium content of individual slices, measured by atomic absorption spectrophotometry, was significantly increased for at least 1 h following return to the control medium. These data indicate that brief exposure of in vitro hippocampal slices to a high extracellular calcium concentration results in a long-term increase in synaptic efficacy which is similar in many respects to long-term potentiation induced by tetanic stimulation of hippocampal excitatory afferents. The results further suggest that the mechanisms underlying calcium-induced long-term potentiation may reside in presynaptic components and involve an enhanced transmitter release.

摘要

采用大鼠离体海马脑片标本,研究细胞外钙浓度短暂升高对Schaffer侧支-连合诱发的CA1锥体神经元兴奋性突触后电位和群体峰电位反应的影响。将脑片短暂暴露(5 - 10分钟)于两倍正常浓度的钙(4 mM)中,可诱导兴奋性突触后电位和群体峰电位显著增强,且这种增强可持续至少3小时。在逆向诱发CA1群体峰电位的突触前纤维峰电位方面未观察到长期变化,这表明这种增强不能归因于激活纤维数量的增加或细胞兴奋性的普遍提高。暴露于高钙灌流液后,CA1锥体神经元对顶端树突区离子导入L - 谷氨酸的反应也未受影响,这表明在突触输入区域,膜兴奋性或受体敏感性没有改变。此外,通过原子吸收分光光度法测量,单个脑片的总细胞内钙含量在回到对照培养基后至少1小时内显著增加。这些数据表明,将离体海马脑片短暂暴露于高细胞外钙浓度会导致突触效能长期增加,这在许多方面与海马兴奋性传入纤维强直刺激诱导的长时程增强相似。结果进一步表明,钙诱导的长时程增强的机制可能存在于突触前成分中,并涉及递质释放增强。

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