C. A. Lindgren: Grinnell College, Department of Biology, 1116 8th Ave., Grinnell College, Grinnell, IA 50112, USA.
J Physiol. 2013 Oct 1;591(19):4749-64. doi: 10.1113/jphysiol.2013.256727. Epub 2013 Jul 1.
Previous work has demonstrated that activation of muscarinic acetylcholine receptors at the lizard neuromuscular junction (NMJ) induces a biphasic modulation of evoked neurotransmitter release: an initial depression followed by a delayed enhancement. The depression is mediated by the release of the endocannabinoid 2-arachidonylglycerol (2-AG) from the muscle and its binding to cannabinoid type 1 receptors on the motor nerve terminal. The work presented here suggests that the delayed enhancement of neurotransmitter release is mediated by cyclooxygenase-2 (COX-2) as it converts 2-AG to the glycerol ester of prostaglandin E2 (PGE2-G). Using immunofluorescence, COX-2 was detected in the perisynaptic Schwann cells (PSCs) surrounding the NMJ. Pretreatment with either of the selective COX-2 inhibitors, nimesulide or DuP 697, prevents the delayed increase in endplate potential (EPP) amplitude normally produced by muscarine. In keeping with its putative role as a mediator of the delayed muscarinic effect, PGE2-G enhances evoked neurotransmitter release. Specifically, PGE2-G increases the amplitude of EPPs without altering that of spontaneous miniature EPPs. As shown previously for the muscarinic effect, the enhancement of evoked neurotransmitter release by PGE2-G depends on nitric oxide (NO) as the response is abolished by application of either N(G)-nitro-l-arginine methyl ester (l-NAME), an inhibitor of NO synthesis, or carboxy-PTIO, a chelator of NO. Intriguingly, the enhancement is not prevented by AH6809, a prostaglandin receptor antagonist, but is blocked by capsazepine, a TRPV1 and TRPM8 receptor antagonist. Taken together, these results suggest that the conversion of 2-AG to PGE2-G by COX-2 underlies the muscarine-induced enhancement of neurotransmitter release at the vertebrate NMJ.
先前的工作已经表明,在蜥蜴神经肌肉接点(NMJ)处激活毒蕈碱乙酰胆碱受体可引起诱发神经递质释放的双相调制:初始抑制随后延迟增强。这种抑制是由肌肉中内源性大麻素 2-花生四烯酰甘油(2-AG)的释放及其与运动神经末梢上的大麻素 1 型受体结合介导的。本文提出的工作表明,神经递质释放的延迟增强是由环氧化酶-2(COX-2)介导的,因为它将 2-AG 转化为前列腺素 E2 的甘油酯(PGE2-G)。通过免疫荧光,在围绕 NMJ 的突触旁施万细胞(PSCs)中检测到 COX-2。用选择性 COX-2 抑制剂尼美舒利或 DuP 697 预处理可防止通常由毒蕈碱产生的终板电位(EPP)幅度的延迟增加。与作为延迟毒蕈碱效应的介质的假定作用一致,PGE2-G 增强了诱发的神经递质释放。具体而言,PGE2-G 增加了 EPP 的幅度,而不改变自发微小 EPP 的幅度。如先前对毒蕈碱效应所示,PGE2-G 增强诱发的神经递质释放取决于一氧化氮(NO),因为应用 NO 合成抑制剂 N(G)-硝基-l-精氨酸甲酯(l-NAME)或 NO 螯合剂羧基-PTIO 会消除反应。有趣的是,AH6809,一种前列腺素受体拮抗剂,不能阻止增强作用,但辣椒素,一种 TRPV1 和 TRPM8 受体拮抗剂,可以阻止增强作用。总之,这些结果表明,COX-2 将 2-AG 转化为 PGE2-G 是脊椎动物 NMJ 中毒蕈碱诱导的神经递质释放增强的基础。