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穿通通路横断后齿状回颗粒细胞树突中NMDAR1蛋白和mRNA的亚细胞差异调节。

Differential subcellular regulation of NMDAR1 protein and mRNA in dendrites of dentate gyrus granule cells after perforant path transection.

作者信息

Gazzaley A H, Benson D L, Huntley G W, Morrison J H

机构信息

Fishberg Research Center for Neurobiology, Mount Sinai School of Medicine, New York, New York 10029, USA.

出版信息

J Neurosci. 1997 Mar 15;17(6):2006-17. doi: 10.1523/JNEUROSCI.17-06-02006.1997.

Abstract

Unilateral transection of the excitatory perforant path results in the acute deafferentation of a segregated zone on the distal dendrites of hippocampal dentate gyrus granule cells (i.e., outer molecular layer), followed by sprouting, reactive synaptogenesis, and a return of physiological and behavioral function. To investigate cellular mechanisms underlying NMDA receptor plasticity in response to such extensive synaptic reorganization, we quantitatively evaluated changes in intensity levels of NMDAR1 immunofluorescence and NMDAR1 mRNA hybridization within subcellular compartments of dentate gyrus granule cells 2, 5, and 9 d after perforant path lesions. There were no significant changes in either measure at 2 d postlesion. However, at 5 and 9 d postlesion, during the period of axonal sprouting and synaptogenesis, there was an increase in NMDAR1 immunolabeling that was restricted to the dendritic segments of the denervated outer molecular layer and the granule cell somata. In contrast, NMDAR1 mRNA levels at 5 and 9 d postlesion increased throughout the full extent of the molecular layer, including both denervated and nondenervated segments of granule cell dendrites. These findings reveal that NMDAR1 mRNA is one of a limited population of mRNAs that is transported into dendrites and further suggest that in response to terminal proliferation and sprouting, increased mRNA transport occurs throughout the full dendritic extent, whereas increased local protein synthesis is restricted to denervated regions of the dendrites whose afferent activity is perturbed. These results begin to elucidate the dynamic postsynaptic subcellular regulation of receptor subunits associated with synaptic plasticity after denervation.

摘要

兴奋性穿通通路的单侧横断导致海马齿状回颗粒细胞远端树突(即外分子层)上一个分离区域的急性传入神经阻滞,随后是发芽、反应性突触形成以及生理和行为功能的恢复。为了研究在这种广泛的突触重组过程中NMDA受体可塑性的细胞机制,我们定量评估了穿通通路损伤后2、5和9天齿状回颗粒细胞亚细胞区室中NMDAR1免疫荧光强度水平和NMDAR1 mRNA杂交的变化。损伤后2天,这两种测量均无显著变化。然而,在损伤后5天和9天,在轴突发芽和突触形成期间,NMDAR1免疫标记增加,且仅限于去神经支配的外分子层的树突段和颗粒细胞胞体。相比之下,损伤后5天和9天,NMDAR1 mRNA水平在分子层的整个范围内均增加,包括颗粒细胞树突的去神经支配和未去神经支配段。这些发现表明,NMDAR1 mRNA是被转运到树突中的有限数量的mRNA之一,并且进一步表明,响应终末增殖和发芽,在整个树突范围内发生mRNA转运增加,而局部蛋白质合成增加仅限于其传入活动受到干扰的树突的去神经支配区域。这些结果开始阐明去神经支配后与突触可塑性相关的受体亚基的动态突触后亚细胞调节。

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