Fukudome Yuko, Ohno-Shosaku Takako, Matsui Minoru, Omori Yuko, Fukaya Masahiro, Tsubokawa Hiroshi, Taketo Makoto M, Watanabe Masahiko, Manabe Toshiya, Kano Masanobu
Department of Cellular Neurophysiology, Graduate School of Medical Science, Kanazawa University, 13-1 Takara-machi, Kanazawa 920-8640, Japan.
Eur J Neurosci. 2004 May;19(10):2682-92. doi: 10.1111/j.0953-816X.2004.03384.x.
The cholinergic system in the CNS plays important roles in higher brain functions, primarily through muscarinic acetylcholine receptors. At cellular levels, muscarinic activation produces various effects including modulation of synaptic transmission. Here we report that muscarinic activation suppresses hippocampal inhibitory transmission through two distinct mechanisms, namely a cannabinoid-dependent and cannabinoid-independent mechanism. We made paired whole-cell recordings from cultured hippocampal neurons of rats and mice, and monitored inhibitory postsynaptic currents (IPSCs). When cannabinoid receptor type 1 (CB1) was blocked, oxotremorine M (oxo-M), a muscarinic agonist, suppressed IPSCs in a subset of neuron pairs. This suppression was associated with an increase in paired-pulse ratio, blocked by the M(2)-preferring antagonist gallamine, and was totally absent in neuron pairs from M(2)-knockout mice. When CB1 receptors were not blocked, oxo-M suppressed IPSCs in a gallamine-resistant manner in cannabinoid-sensitive pairs. This suppression was associated with an increase in paired-pulse ratio, blocked by the CB1 antagonist AM281, and was completely eliminated in neuron pairs from M(1)/M(3)-compound-knockout mice. Our immunohistochemical examination showed that M(2) and CB1 receptors were present at inhibitory presynaptic terminals of mostly different origins. These results indicate that two distinct mechanisms mediate the muscarinic suppression. In a subset of synapses, activation of M(2) receptors at presynaptic terminals suppresses GABA release directly. In contrast, in a different subset of synapses, activation of M(1)/M(3) receptors causes endocannabinoid production and subsequent suppression of GABA release by activating presynaptic CB1 receptors. Thus, the muscarinic system can influence hippocampal functions by controlling different subsets of inhibitory synapses through the two distinct mechanisms.
中枢神经系统中的胆碱能系统在高级脑功能中发挥重要作用,主要通过毒蕈碱型乙酰胆碱受体。在细胞水平上,毒蕈碱激活产生多种效应,包括对突触传递的调节。在此我们报告,毒蕈碱激活通过两种不同机制抑制海马体抑制性传递,即大麻素依赖性机制和大麻素非依赖性机制。我们对大鼠和小鼠培养的海马神经元进行了配对全细胞记录,并监测抑制性突触后电流(IPSCs)。当1型大麻素受体(CB1)被阻断时,毒蕈碱激动剂氧化震颤素M(oxo-M)在一部分神经元对中抑制了IPSCs。这种抑制与配对脉冲比率的增加相关,被偏好M(2)的拮抗剂加拉明阻断,并且在M(2)基因敲除小鼠的神经元对中完全不存在。当CB1受体未被阻断时,oxo-M在对大麻素敏感的神经元对中以加拉明抗性方式抑制IPSCs。这种抑制与配对脉冲比率的增加相关,被CB1拮抗剂AM281阻断,并且在M(1)/M(3)复合基因敲除小鼠的神经元对中完全消除。我们的免疫组织化学检查表明,M(2)和CB1受体存在于大多数不同来源的抑制性突触前终末。这些结果表明,两种不同机制介导了毒蕈碱抑制作用。在一部分突触中,突触前终末的M(2)受体激活直接抑制γ-氨基丁酸(GABA)释放。相反,在另一部分不同的突触中,M(1)/M(3)受体激活导致内源性大麻素产生,并通过激活突触前CB1受体随后抑制GABA释放。因此,毒蕈碱系统可通过这两种不同机制控制抑制性突触的不同子集来影响海马体功能。
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