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I 型代谢型谷氨酸受体在不同小鼠纹状体神经元中的相反作用

Contrasting actions of group I metabotropic glutamate receptors in distinct mouse striatal neurones.

作者信息

Partridge John G, Lewin Amanda E, Yasko Jessica R, Vicini Stefano

机构信息

Department of Pharmacology and Physiology, Georgetown University School of Medicine, Washington, DC, 20007, USA Interdisciplinary Program in Neuroscience, Georgetown University School of Medicine, Washington, DC, 20007, USA

Department of Pharmacology and Physiology, Georgetown University School of Medicine, Washington, DC, 20007, USA.

出版信息

J Physiol. 2014 Jul 1;592(13):2721-33. doi: 10.1113/jphysiol.2014.272773. Epub 2014 Apr 7.

Abstract

In mouse striatum, metabotropic glutamate receptor (mGluR) activation leads to several modulatory effects in synaptic transmission. These effects range from dampening of glutamate release from excitatory terminals to depolarization of divergent classes of interneurones. We compared the action of group I mGluR activation on several populations of striatal neurones using a combination of genetic identification, electrophysiology, and Ca(2+) imaging techniques. Patch-clamp recordings from spiny projection neurones (SPNs) and various interneurone populations demonstrated that the group I mGluR agonist (RS)-3,5-dihydroxyphenylglycine (DHPG) robustly depolarizes several interneurone classes that form GABAergic synapses onto SPNs. We further utilized the genetic reporter mouse strain Ai38, which expresses the calcium indicator protein GCaMP3 in a Cre-dependent manner. Breeding Ai38 mice with various neurone selective, promoter-driven Cre recombinase mice resulted in GCaMP3 expression in defined cell populations in striatum. Consistent with our electrophysiological findings, group I agonist applications increased intracellular levels of calcium ([Ca(2+)]i) in all interneurone populations tested. We also found that acute DHPG application evoked a transient, rapid increase in [Ca(2+)]i from only a small percentage of identifiable SPNs. Surprisingly, this fast [Ca(2+)]i response exhibited a robust enhancement or sensitization, in a calcium-dependent fashion. Following several procedures to increase [Ca(2+)]i, the vast majority of SPNs responded with rapid changes in [Ca(2+)]i to mGluR agonists in a time-dependent fashion. These findings extend our understanding on group I mGluR influence of striatal output via powerful, local GABAergic connections in addition to [Ca(2+)]i dynamics that impact on activity or spike-timing-dependent forms of synaptic plasticity.

摘要

在小鼠纹状体中,代谢型谷氨酸受体(mGluR)的激活会对突触传递产生多种调节作用。这些作用范围从抑制兴奋性终末释放谷氨酸到使不同类型的中间神经元去极化。我们结合基因鉴定、电生理学和Ca(2+)成像技术,比较了I组mGluR激活对纹状体神经元多个群体的作用。对棘状投射神经元(SPN)和各种中间神经元群体进行膜片钳记录表明,I组mGluR激动剂(RS)-3,5-二羟基苯甘氨酸(DHPG)能强烈使几种在SPN上形成GABA能突触的中间神经元类型去极化。我们进一步利用基因报告小鼠品系Ai38,其以Cre依赖的方式表达钙指示剂蛋白GCaMP3。将Ai38小鼠与各种神经元选择性、启动子驱动的Cre重组酶小鼠杂交,导致GCaMP3在纹状体特定细胞群体中表达。与我们的电生理学发现一致,应用I组激动剂会使所有测试的中间神经元群体中的细胞内钙水平([Ca(2+)]i)升高。我们还发现,急性应用DHPG仅能使一小部分可识别的SPN的[Ca(2+)]i出现短暂、快速升高。令人惊讶的是,这种快速的[Ca(2+)]i反应以钙依赖的方式表现出强烈的增强或敏化。在采取多种增加[Ca(2+)]i的方法后,绝大多数SPN会以时间依赖的方式对mGluR激动剂产生[Ca(2+)]i的快速变化反应。这些发现扩展了我们对I组mGluR通过强大的局部GABA能连接影响纹状体输出的理解,此外还涉及影响活动或突触可塑性的尖峰时间依赖性形式的[Ca(2+)]i动态变化。

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