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通过代谢型谷氨酸受体激活在僧帽细胞的初级树突中 T 型钙通道的突触激活。

Synaptic activation of T-type Ca2+ channels via mGluR activation in the primary dendrite of mitral cells.

机构信息

Department of Biology, University of Victoria, Victoria, British Columbia, Canada.

出版信息

J Neurophysiol. 2010 May;103(5):2557-69. doi: 10.1152/jn.00796.2009. Epub 2010 Jan 13.

Abstract

Mitral cells are the primary output of the olfactory bulb, projecting to many higher brain areas. Understanding how mitral cells process and transmit information is key to understanding olfactory perception. Mitral dendrites possess high densities of voltage-gated channels, are able to initiate and propagate orthodromic and antidromic action potentials, and release neurotransmitter. We show that mitral cells also possess a low-voltage-activated T-type Ca(2+) current. Immunohistochemistry shows strong Cav3.3 labeling in the primary dendrite and apical tuft with weaker staining in basal dendrites and no staining in somata. A low-voltage-activated Ca(2+) current activates from -68 mV, is blocked by 500 microM Ni(2+) and 50 microM NNC 55-0396, but is insensitive to 50 microM Ni(2+) and 500 microM isradipine. 2-photon Ca(2+) imaging shows that T channels are functionally expressed in the primary dendrite where their activity determines the resting [Ca(2+)] and are responsible for subthreshold voltage-dependent Ca(2+) changes previously observed in vivo. Application of the group 1 mGluR agonist dihydroxyphenylglycine (DHPG) (50 microM) robustly upregulates T-channel current in the primary and apical tuft dendrite. Olfactory nerve stimulation generates a long-lasting depolarization, and we show that mGluRs recruit T channels to contribute approximately 36% of the voltage integral of this depolarization. The long-lasting depolarization results in sustained firing and block of T channels decreased action potential firing by 84.1 +/- 4.6%. Therefore upregulation of T channels by mGluRs is required for prolonged firing in response to olfactory nerve input.

摘要

僧帽细胞是嗅球的主要输出细胞,投射到许多高级脑区。了解僧帽细胞如何处理和传递信息是理解嗅觉感知的关键。僧帽细胞树突具有高密度的电压门控通道,能够发起和传播顺向和逆向动作电位,并释放神经递质。我们发现,僧帽细胞还具有一种低电压激活的 T 型钙电流。免疫组织化学显示,Cav3.3 在主树突和顶树突中强烈标记,在基底树突中标记较弱,在胞体中无标记。一种低电压激活的 Ca(2+)电流从-68 mV 激活,被 500 microM Ni(2+)和 50 microM NNC 55-0396 阻断,但对 50 microM Ni(2+)和 500 microM 异搏定不敏感。双光子 Ca(2+)成像显示,T 通道在主树突中功能性表达,其活性决定了静息 [Ca(2+)],并负责先前在体内观察到的亚阈值电压依赖性 Ca(2+)变化。应用组 1 mGluR 激动剂二羟苯甘氨酸 (DHPG) (50 microM) 可显著增强主树突和顶树突的 T 通道电流。嗅神经刺激产生持久的去极化,我们发现 mGluRs 募集 T 通道,贡献约 36%的这种去极化的电压积分。持久的去极化导致持续的放电,而 T 通道的阻断使动作电位的放电减少 84.1 +/- 4.6%。因此,mGluRs 对 T 通道的上调是对嗅神经输入产生持久放电所必需的。

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