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精胺对大鼠培养海马神经元N-甲基-D-天冬氨酸受体反应的多种作用

Multiple effects of spermine on N-methyl-D-aspartic acid receptor responses of rat cultured hippocampal neurones.

作者信息

Benveniste M, Mayer M L

机构信息

Laboratory of Cellular and Molecular Neurophysiology, NICHD, National Institutes of Health, Bethesda, MD 20892.

出版信息

J Physiol. 1993 May;464:131-63. doi: 10.1113/jphysiol.1993.sp019627.

Abstract
  1. The modulation by polyamines of responses to N-methyl-D-aspartic acid (NMDA) was studied using a rapid perfusion system and whole-cell voltage-clamp recording from rat hippocampal neurons in dissociated culture. 2. Concentration jump responses to 100 microM NMDA in the presence of 10 microM glycine revealed potentiation by 3 mM spermine at a membrane potential of +60 mV, but depression at -120 mV; the degree of potentiation at +60 mV was variable from cell to cell while marked depression at -120 mV was observed in all cells. The depression of responses to NMDA by spermine was highly voltage dependent (z delta = 1.17) with an apparent equilibrium dissociation constant for block at 0 mV of 27 mM. 3. Analysis of spermine dose-potentiation curves for responses recorded at +60 mV in the presence of 10 microM glycine revealed a half-maximal effect at 125 microM. Under the same conditions, but at -60 mV, analysis of spermine-evoked depression was performed for cells with less than 5% potentiation at +60 mV, and revealed half-maximal inhibition at 344 microM. 4. Dose-response analysis for the glycine-sensitive activation of NMDA receptors at +60 mV revealed a 3.5-fold increase in apparent affinity for glycine in the presence of 1 mM spermine. This increase in affinity for glycine was accompanied by a 3.3-fold decrease in the rate of development of glycine-sensitive desensitization, and a 2.4-fold decrease in the rate of dissociation of glycine from NMDA receptors, while the rate constant for dissociation of NMDA was not reduced. 5. In the presence of non-saturating concentrations of glycine, spermine-induced potentiation at +60 mV developed with two exponential components: a slow glycine-sensitive component, the amplitude and time constant of which decreased with increasing glycine concentration (30 nM glycine, amplitude = 80.2 +/- 5.1%, tau = 780 +/- 79 ms; 3 microM glycine, amplitude = 22.6 +/- 7.1%, tau = 45 +/- 13 ms), and a faster component (tau < 20 ms at all concentrations of glycine), the amplitude of which varied from cell to cell, and which became larger with increase in concentration of glycine. When responses to the application of spermine were measured in the presence 10 microM L-alanine instead of 100 nM glycine, the slow component of potentiation was absent.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 运用快速灌注系统以及对解离培养的大鼠海马神经元进行全细胞电压钳记录的方法,研究了多胺对N-甲基-D-天冬氨酸(NMDA)反应的调节作用。2. 在存在10 μM甘氨酸的情况下,对100 μM NMDA的浓度阶跃反应显示,在膜电位为+60 mV时,3 mM精胺可使其增强,但在-120 mV时则为抑制;+60 mV时的增强程度在细胞间存在差异,而在-120 mV时所有细胞均观察到明显抑制。精胺对NMDA反应的抑制高度依赖电压(zδ = 1.17),在0 mV时阻断的表观平衡解离常数为27 mM。3. 对在存在10 μM甘氨酸时于+60 mV记录的反应进行精胺剂量增强曲线分析,结果显示在125 μM时达到半数最大效应。在相同条件下,但在-60 mV时,对在+60 mV时增强小于5%的细胞进行精胺诱发抑制分析,结果显示在344 μM时达到半数最大抑制。4. 在+60 mV时对NMDA受体甘氨酸敏感激活的剂量反应分析显示,在存在1 mM精胺的情况下,对甘氨酸的表观亲和力增加了3.5倍。对甘氨酸亲和力的这种增加伴随着甘氨酸敏感脱敏发展速率降低3.3倍,以及甘氨酸从NMDA受体解离速率降低2.4倍,而NMDA解离的速率常数未降低。5. 在存在非饱和浓度甘氨酸的情况下,精胺在+60 mV时诱发的增强有两个指数成分:一个缓慢的甘氨酸敏感成分,其幅度和时间常数随甘氨酸浓度增加而降低(30 nM甘氨酸,幅度 = 80.2 ± 5.1%,τ = 780 ± 79 ms;3 μM甘氨酸,幅度 = 22.6 ± 7.1%,τ = 45 ± 13 ms),以及一个较快成分(在所有甘氨酸浓度下τ < 20 ms),其幅度在细胞间有所不同,且随甘氨酸浓度增加而变大。当在存在10 μM L-丙氨酸而非100 nM甘氨酸的情况下测量对精胺应用的反应时,增强的缓慢成分不存在。(摘要截断于400字)

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