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CA3 和 CA1 之间的成对刺激改变了大鼠海马 CA3 的兴奋性。

Paired stimulation between CA3 and CA1 alters excitability of CA3 in the rat hippocampus.

机构信息

Department of Physiology, National Defense Medical College, Tokorozawa, Japan.

出版信息

Neurosci Lett. 2013 Feb 8;534:182-7. doi: 10.1016/j.neulet.2012.11.058. Epub 2012 Dec 20.

Abstract

It is generally accepted that the extent of plasticity is localized to the region around synapses and post-synaptic intracellular signaling cascades. We investigated the presence of long-range retrograde plasticity associated with excitability at pre-synaptic neurons (CA3) and regulated by the firing of post-synaptic neurons (CA1). We used acute hippocampus slices from transgenic rats expressing channelrhodopsin-2 (ChR2) in both CA1 and CA3 neurons. We employed a parallel photostimulation technique, which enabled robust and independent evocation of action potentials in either CA3 or CA1 neurons. Optically evoked CA3 firings were paired either with CA1 simultaneous firings or with CA1 suppression after the prolonged stimulation. Pre-synaptic excitability was monitored by measuring the optically-evoked firing rate (Opt-FR). We found that the Opt-FR of CA3 neurons was long-term up-regulated as a result of synchronous pre- and post-synaptic pairing stimulation, but down-regulated by the pre-synaptic stimulation during post-synaptic suppression. Both pairing-dependent up-regulation and down-regulation were retarded by NMDA receptor blocking or colchicine preincubation. This finding suggest that CA3 excitability is regulated by CA1 neuron activity at the time of CA3 firing.

摘要

人们普遍认为,可塑性的程度局限于突触周围区域和突触后细胞内信号级联。我们研究了与兴奋相关的长程逆行可塑性的存在,这种可塑性与前突触神经元(CA3)有关,并且受到后突触神经元(CA1)的发射调节。我们使用急性海马脑片,其中 CA1 和 CA3 神经元都表达通道视紫红质-2(ChR2)。我们采用平行光刺激技术,能够在 CA3 或 CA1 神经元中产生强大而独立的动作电位。用光激发 CA3 放电与 CA1 同时放电或长时间刺激后的 CA1 抑制配对。通过测量光激发的放电率(Opt-FR)来监测前突触兴奋性。我们发现,由于同步的前突触和后突触配对刺激,CA3 神经元的 Opt-FR 被长期上调,但在后突触抑制期间,前突触刺激会下调。NMDA 受体阻断或秋水仙碱预孵育均会延迟配对依赖性的上调和下调。这一发现表明,CA3 兴奋性受 CA1 神经元在 CA3 放电时的活动调节。

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