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雏鸡听觉脑干中质膜钙ATP酶2的特定区域调节

Compartment-specific regulation of plasma membrane calcium ATPase type 2 in the chick auditory brainstem.

作者信息

Wang Yuan, Cunningham Dale E, Tempel Bruce L, Rubel Edwin W

机构信息

Virginia Merrill Bloedel Hearing Research Center, Department of Otolaryngology-Head and Neck Surgery, University of Washington School of Medicine, Seattle, Washington 98195, USA.

出版信息

J Comp Neurol. 2009 Jun 20;514(6):624-40. doi: 10.1002/cne.22045.

Abstract

Calcium signaling plays a role in synaptic regulation of dendritic structure, usually on the time scale of hours or days. Here we use immunocytochemistry to examine changes in expression of plasma membrane calcium ATPase type 2 (PMCA2), a high-affinity calcium efflux protein, in the chick nucleus laminaris (NL) following manipulations of synaptic inputs. Dendrites of NL neurons segregate into dorsal and ventral domains, receiving excitatory input from the ipsilateral and contralateral ears, respectively, via nucleus magnocellularis (NM). Deprivation of the contralateral projection from NM to NL leads to rapid retraction of ventral, but not the dorsal, dendrites of NL neurons. Immunocytochemistry revealed symmetric distribution of PMCA2 in two neuropil regions of normally innervated NL. Electron microscopy confirmed that PMCA2 localizes in both NM terminals and NL dendrites. As early as 30 minutes after transection of the contralateral projection from NM to NL or unilateral cochlea removal, significant decreases in PMCA2 immunoreactivity were seen in the deprived neuropil of NL compared with the other neuropil that continued to receive normal input. The rapid decrease correlated with reductions in the immunoreactivity for microtubule-associated protein 2, which affects cytoskeleton stabilization. These results suggest that PMCA2 is regulated independently in ventral and dorsal NL dendrites and/or their inputs from NM in a way that is correlated with presynaptic activity. This provides a potential mechanism by which deprivation can change calcium transport that, in turn, may be important for rapid, compartment-specific dendritic remodeling.

摘要

钙信号传导在树突结构的突触调节中发挥作用,通常作用时间尺度为数小时或数天。在这里,我们使用免疫细胞化学方法来检测在对突触输入进行操作后,鸡层状核(NL)中质膜钙ATP酶2型(PMCA2,一种高亲和力钙外流蛋白)的表达变化。NL神经元的树突分为背侧和腹侧区域,分别通过大细胞神经核(NM)接收来自同侧和对侧耳朵的兴奋性输入。剥夺从NM到NL的对侧投射会导致NL神经元腹侧树突迅速回缩,但背侧树突不会。免疫细胞化学显示,在正常支配的NL的两个神经毡区域中,PMCA2呈对称分布。电子显微镜证实PMCA2定位于NM终末和NL树突中。早在切断从NM到NL的对侧投射或单侧摘除耳蜗后30分钟,与继续接受正常输入的另一个神经毡相比,在NL的被剥夺神经毡中就观察到PMCA2免疫反应性显著降低。这种快速降低与微管相关蛋白2的免疫反应性降低相关,微管相关蛋白2影响细胞骨架的稳定性。这些结果表明,PMCA2在腹侧和背侧NL树突和/或它们来自NM的输入中以与突触前活动相关的方式被独立调节。这提供了一种潜在机制,通过该机制剥夺可以改变钙转运,而钙转运反过来可能对快速的、特定区域的树突重塑很重要。

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