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仅含F-box结构域蛋白2(Fbxo2)的缺失会破坏特定N-甲基-D-天冬氨酸受体亚基的水平和定位,并促进异常的突触连接。

Loss of F-box only protein 2 (Fbxo2) disrupts levels and localization of select NMDA receptor subunits, and promotes aberrant synaptic connectivity.

作者信息

Atkin Graham, Moore Shannon, Lu Yuan, Nelson Rick F, Tipper Nathan, Rajpal Gautam, Hunt Jack, Tennant William, Hell Johannes W, Murphy Geoffrey G, Paulson Henry

机构信息

Department of Neurology.

Molecular and Behavioral Neuroscience Institute, and.

出版信息

J Neurosci. 2015 Apr 15;35(15):6165-78. doi: 10.1523/JNEUROSCI.3013-14.2015.

Abstract

NMDA receptors (NMDARs) play an essential role in some forms of synaptic plasticity, learning, and memory. Therefore, these receptors are highly regulated with respect to their localization, activation, and abundance both within and on the surface of mammalian neurons. Fundamental questions remain, however, regarding how this complex regulation is achieved. Using cell-based models and F-box Only Protein 2 (Fbxo2) knock-out mice, we found that the ubiquitin ligase substrate adaptor protein Fbxo2, previously reported to facilitate the degradation of the NMDAR subunit GluN1 in vitro, also functions to regulate GluN1 and GluN2A subunit levels in the adult mouse brain. In contrast, GluN2B subunit levels are not affected by the loss of Fbxo2. The loss of Fbxo2 results in greater surface localization of GluN1 and GluN2A, together with increases in the synaptic markers PSD-95 and Vglut1. These synaptic changes do not manifest as neurophysiological differences or alterations in dendritic spine density in Fbxo2 knock-out mice, but result instead in increased axo-dendritic shaft synapses. Together, these findings suggest that Fbxo2 controls the abundance and localization of specific NMDAR subunits in the brain and may influence synapse formation and maintenance.

摘要

N-甲基-D-天冬氨酸受体(NMDARs)在某些形式的突触可塑性、学习和记忆中起着至关重要的作用。因此,这些受体在哺乳动物神经元内部和表面的定位、激活及丰度方面受到高度调控。然而,关于这种复杂调控是如何实现的,仍存在一些基本问题。利用基于细胞的模型和仅含F盒蛋白2(Fbxo2)基因敲除小鼠,我们发现泛素连接酶底物衔接蛋白Fbxo2,此前报道其在体外可促进NMDAR亚基GluN1的降解,在成年小鼠大脑中也具有调控GluN1和GluN2A亚基水平的功能。相比之下,GluN2B亚基水平不受Fbxo2缺失的影响。Fbxo2的缺失导致GluN1和GluN2A在细胞表面的定位增加,同时突触标记物PSD-95和Vglut1也增加。这些突触变化在Fbxo2基因敲除小鼠中并未表现为神经生理学差异或树突棘密度的改变,而是导致轴突-树突干突触增加。总之,这些发现表明Fbxo2控制着大脑中特定NMDAR亚基的丰度和定位,并可能影响突触的形成和维持。

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