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丝氨酸880磷酸化的GluR2在海马神经元中的稳定突触保留。

Stable synaptic retention of serine-880-phosphorylated GluR2 in hippocampal neurons.

作者信息

States Bradley A, Khatri Latika, Ziff Edward B

机构信息

Department of Biochemistry, NYU School of Medicine, NY, USA.

出版信息

Mol Cell Neurosci. 2008 Jun;38(2):189-202. doi: 10.1016/j.mcn.2008.02.003. Epub 2008 Mar 4.

Abstract

Phosphorylation of S880 within the GluR2 C-terminus has been reported to promote endocytosis of AMPA receptors (AMPARs) by preventing GluR2 interaction with the putative synaptic anchoring proteins GRIP and ABP. It is not yet established however, whether S880 phosphorylation induces removal of AMPARs from synaptic sites, and the trafficking of phosphorylated GluR2 subunits with surface and endocytosed GluR2 has not been directly compared within the same intact neurons. Here we show that phosphorylation of GluR2 subunits by PKC activated with phorbol esters is compartmentally restricted to receptors located at the cell surface. Endogenous AMPARs containing S880-phosphorylated GluR2 remained highly synaptic and colocalized with postsynaptic markers to the same extent as AMPARs which did not contain S880-phosphorylated GluR2. Moreover, following S880 phosphorylation, exogenous GluR2 homomers were found specifically at the cell surface and did not co-traffic with the internalized endosomal GluR2 population. We also show that GluR2 is endogenously phosphorylated by a constitutively active kinase pharmacologically related to PKC, and this phosphorylation is opposed by the protein phosphatase PP1. Our results demonstrate a population of hippocampal AMPARs which do not require interaction with GRIP/ABP for synaptic anchorage.

摘要

据报道,谷氨酸受体2(GluR2)C末端的S880磷酸化通过阻止GluR2与假定的突触锚定蛋白GRIP和ABP相互作用,促进α-氨基-3-羟基-5-甲基-4-异恶唑丙酸受体(AMPARs)的内吞作用。然而,S880磷酸化是否会诱导AMPARs从突触位点移除尚未确定,并且在同一完整神经元内,尚未直接比较磷酸化的GluR2亚基与表面和内吞的GluR2的运输情况。在这里,我们表明,佛波酯激活的蛋白激酶C(PKC)对GluR2亚基的磷酸化在区域上仅限于位于细胞表面的受体。含有S880磷酸化GluR2的内源性AMPARs仍高度定位于突触,并且与突触后标记物共定位的程度与不含S880磷酸化GluR2的AMPARs相同。此外,在S880磷酸化后,外源性GluR2同聚体特异性地出现在细胞表面,并且不与内化的内体GluR2群体共同运输。我们还表明,GluR2被一种与PKC药理学相关的组成型活性激酶内源性磷酸化,并且这种磷酸化被蛋白磷酸酶PP1所拮抗。我们的结果表明,海马体中的一群AMPARs在突触锚定方面不需要与GRIP/ABP相互作用。

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