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L-Aspartic acid induces a region of negative slope conductance in the current-voltage relationship of cultured spinal cord neurons.L-天冬氨酸在培养的脊髓神经元的电流-电压关系中诱导出一个负斜率电导区域。
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The dissociative anaesthetics, ketamine and phencyclidine, selectively reduce excitation of central mammalian neurones by N-methyl-aspartate.分离麻醉药氯胺酮和苯环己哌啶可选择性降低N-甲基天冬氨酸对中枢哺乳动物神经元的兴奋作用。
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Excitatory amino acids in synaptic transmission in the Schaffer collateral-commissural pathway of the rat hippocampus.兴奋性氨基酸在大鼠海马体的Schaffer侧支-连合通路突触传递中的作用
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培养的小鼠中枢神经元上由N-甲基-D-天冬氨酸受体介导的缓慢兴奋性突触后电流。

Slow excitatory postsynaptic currents mediated by N-methyl-D-aspartate receptors on cultured mouse central neurones.

作者信息

Forsythe I D, Westbrook G L

机构信息

Laboratory of Developmental Neurobiology, NICHD, Bethesda, MD 20892.

出版信息

J Physiol. 1988 Feb;396:515-33. doi: 10.1113/jphysiol.1988.sp016975.

DOI:10.1113/jphysiol.1988.sp016975
PMID:2900892
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1192058/
Abstract
  1. Monosynaptic excitatory postsynaptic potentials (EPSPs) evoked between pairs of cultured neurones from either hippocampus or spinal cord were examined using the tight-seal whole-cell recording technique. 2. Using the selective N-methyl-D-aspartate (NMDA)-receptor antagonist, 2-amino-5-phosphonovaleric acid (APV), two components of the EPSP could be resolved in cultures from both brain regions. The APV-sensitive (slow) component had the same latency, but a much slower time-to-peak and longer duration than the APV-resistant (fast) component. Other NMDA antagonists such as ketamine also selectively blocked the slow component of the EPSP. 3. In Mg2+-free medium, the dual-component EPSP had a duration lasting up to 500 ms, greatly exceeding the membrane time constant of the postsynaptic neurone, suggesting that persistent activation of NMDA receptors was responsible for the long duration of the APV-sensitive component. 4. Under voltage clamp the excitatory postsynaptic currents (EPSCs) also showed fast and slow components, both of which had a reversal potential near 0 mV in physiological saline. The synaptic current could be fitted with a sum of two exponentials with a decay time constant for the slow EPSC near 80 ms. The slow current contributed approximately 50% of the total charge transfer during the EPSC. 5. In Mg2+-containing medium, the peak of the fast component was voltage insensitive, whereas the synaptic current measured at a latency of 10-50 ms was voltage dependent with a region of negative slope conductance at membrane potentials hyperpolarized to -30 mV. 6. Raising [Ca2+]o from 1 to 20 mM resulted in a shift of the reversal potential of the APV-sensitive component from near 0 mV to + 10 mV, but the reversal potential of the fast component remained near 0 mV. This suggests that conductances with different ionic permeability underlie the two components of the EPSC and that the slow component is highly permeable to Ca2+ as well as to monovalent cations. 7. Our results demonstrate that two functionally distinct excitatory amino acid receptor channels are simultaneously activated by transmitter release from a single presynaptic neurone. The conductance mechanism underlying the slow component of the EPSP displays the voltage dependence and Ca2+ permeability expected for NMDA-receptor channels. We suggest that the available conductance generating the slow EPSP may be sufficient, even at low firing rates, to influence excitability on both a short-term and more long-lasting basis.
摘要
  1. 使用紧密密封的全细胞记录技术,检测了从海马体或脊髓培养的神经元对之间诱发的单突触兴奋性突触后电位(EPSP)。2. 使用选择性N-甲基-D-天冬氨酸(NMDA)受体拮抗剂2-氨基-5-磷酸戊酸(APV),在来自两个脑区的培养物中都可以分辨出EPSP的两个成分。APV敏感(慢)成分具有相同的潜伏期,但与APV抗性(快)成分相比,其峰值时间要慢得多,持续时间更长。其他NMDA拮抗剂如氯胺酮也选择性地阻断了EPSP的慢成分。3. 在无镁培养基中,双成分EPSP的持续时间长达500毫秒,大大超过了突触后神经元的膜时间常数,这表明NMDA受体的持续激活是APV敏感成分持续时间长的原因。4. 在电压钳制下,兴奋性突触后电流(EPSC)也显示出快成分和慢成分,在生理盐水中,两者的反转电位都接近0 mV。突触电流可以用两个指数之和来拟合,慢EPSC的衰减时间常数接近80毫秒。慢电流在EPSC期间贡献了约50%的总电荷转移。5. 在含镁培养基中,快成分的峰值对电压不敏感,而在10 - 50毫秒潜伏期测量的突触电流对电压敏感,在膜电位超极化到 - 30 mV时存在负斜率电导区域。6. 将细胞外[Ca2+]从1 mM提高到20 mM,导致APV敏感成分的反转电位从接近0 mV移至 + 10 mV,但快成分的反转电位仍接近0 mV。这表明EPSC的两个成分具有不同离子通透性的电导,并且慢成分对Ca2+以及单价阳离子具有高度通透性。7. 我们的结果表明,两个功能不同的兴奋性氨基酸受体通道同时被单个突触前神经元释放的递质激活。EPSP慢成分的电导机制表现出NMDA受体通道预期的电压依赖性和Ca2+通透性。我们认为,即使在低发放率下,产生慢EPSP的可用电导可能足以在短期和更持久的基础上影响兴奋性。