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大鼠海马CA1区和齿状回的内嗅皮层输入:电流源密度研究

Entorhinal inputs to hippocampal CA1 and dentate gyrus in the rat: a current-source-density study.

作者信息

Leung L S, Roth L, Canning K J

机构信息

Department of Physiology and Clinical Neurological Sciences, University of Western Ontario, London, Canada.

出版信息

J Neurophysiol. 1995 Jun;73(6):2392-403. doi: 10.1152/jn.1995.73.6.2392.

Abstract
  1. Laminar profiles of the average evoked potentials and current-source-density analysis were used to study the input provided by the medial perforant path (PP) to the hippocampus in the urethan-anesthetized rat. 2. Stimulation of the PP activated an early latency sink in the middle molecular layer of the dentate gyrus (DG) and in the stratum lacunosum-moleculare in CA1. The DG current sink was generated by excitatory synaptic currents activated by the PP on dentate granule cells. In the normal rat, the peak current sink in the DG was typically five times greater than that of CA1. However, the CA1 sink could be distinguished from the DG sink in several ways: 1) it peaked when the DG sink was subsiding; 2) it showed paired-pulse facilitation, whereas the DG sink did not; and 3) in rats in which the DG was lesioned by local colchicine injection, the DG sink was reduced much more than the CA1 sink. 3. The PP afferents to CA1 required a slightly higher stimulus threshold (> 100 microA) for activation than those projecting to the DG granule cells (< 30 microA). The onset latency of the early CA1 sink (2.5 +/- 0.2 ms, mean +/- SE) was also slightly longer than that of the DG sink (1.7 +/- 0.1 ms), suggesting that the axons of entorhinal layer III cells that project to CA1 have a slightly lower conduction velocity than the axons of the layer II cells that project to the DG. 4. The short-latency current sink activated by the PP in the distal dendritic layers of CA1 was likely provided by excitatory currents at the distal apical dendrites of CA1 pyramidal cells. The accompanying current source was mainly confined to stratum radiatum and appeared not to involve the cell body layer. Thus the electrotonic current spread may not be effective enough to depolarize the cell body or axon hillock. Contribution of interneurons to the above source-sink profile is possible, with the provision that these interneurons must have dendritic processes that span strata radiatum and lacunosum moleculare. 5. Extracellular field recordings provided no evidence that PP evoked a short-latency (< 9 ms) CA1-generated population spike, even with the use of micropipettes filled with mM bicuculline. Similarly, unit recordings in CA1 revealed only long-latency (9-17 ms) unit firing after PP stimulation, corresponding to a late, di/trisynaptic excitation of CA1 via the Schaffer collaterals.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 采用平均诱发电位的层流剖面图和电流源密度分析,研究在乌拉坦麻醉的大鼠中,内侧穿通通路(PP)向海马提供的输入。2. 刺激PP可激活齿状回(DG)中层分子层以及CA1区的腔隙-分子层中一个潜伏期较早的电流汇。DG区的电流汇是由PP对齿状颗粒细胞激活的兴奋性突触电流产生的。在正常大鼠中,DG区的电流汇峰值通常比CA1区大五倍。然而,CA1区的电流汇可通过以下几种方式与DG区的电流汇区分开来:1)当DG区的电流汇消退时它达到峰值;2)它表现出双脉冲易化,而DG区的电流汇则没有;3)在通过局部注射秋水仙碱使DG区受损的大鼠中,DG区的电流汇比CA1区的电流汇减少得更多。3. 投射到CA1区的PP传入纤维激活所需的刺激阈值(>100微安)略高于投射到DG颗粒细胞的传入纤维(<30微安)。早期CA1区电流汇的起始潜伏期(2.5±0.2毫秒,平均值±标准误)也略长于DG区电流汇的起始潜伏期(1.7±0.1毫秒),这表明投射到CA1区的内嗅皮层III层细胞的轴突传导速度略低于投射到DG区的II层细胞的轴突传导速度。4. PP在CA1区远端树突层激活的短潜伏期电流汇可能是由CA1锥体细胞远端顶端树突处的兴奋性电流提供的。伴随的电流源主要局限于辐射层,似乎不涉及细胞体层。因此,电紧张性电流传播可能不足以使细胞体或轴突丘去极化。中间神经元对上述源-汇剖面图有贡献是可能的,前提是这些中间神经元必须有跨越辐射层和腔隙-分子层的树突过程。5. 细胞外场记录没有提供证据表明PP能诱发短潜伏期(<9毫秒)的由CA1区产生的群体锋电位,即使使用充满毫摩尔浓度荷包牡丹碱的微电极也未发现。同样,CA1区的单位记录显示,PP刺激后仅出现长潜伏期(9 - 17毫秒)的单位放电,这对应于通过谢弗侧支对CA1区的晚期、二/三突触兴奋。(摘要截断于400字)

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