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AMPA受体翻转和摆动变体的亚型特异性早期运输

Isoform-specific early trafficking of AMPA receptor flip and flop variants.

作者信息

Coleman Sarah K, Möykkynen Tommi, Cai Chunlin, von Ossowski Lotta, Kuismanen Esa, Korpi Esa R, Keinänen Kari

机构信息

Department of Biological and Environmental Sciences, Division of Biochemistry, Viikki Biocenter, University of Helsinki, FIN-00014 Helsinki, Finland.

出版信息

J Neurosci. 2006 Oct 25;26(43):11220-9. doi: 10.1523/JNEUROSCI.2301-06.2006.

Abstract

Flip and flop splice variants of AMPA receptor subunits are expressed in distinct but partly overlapping patterns and impart different desensitization kinetics to cognate receptor channels. In the absence of specific antibodies, isoform-specific differences in trafficking or localization of native flip and flop subunits remain uncharacterized. We report that in several transfected cell lines, transport of homomeric glutamate receptor (GluR)-D(flop) receptors is largely blocked at the endoplasmic reticulum (ER) exit, whereas GluR-D(flip) undergoes complex glycosylation and reaches the plasma membrane at >10x higher levels than GluR-D(flop), as determined by immunofluorescence, patch-clamp recordings and biochemical assays. The transport difference between flip and flop is independent of activity, is primarily determined by amino acid residue 780 (Leu in flop, Val in flip), and is manifested even in the secretion of the soluble ligand-binding domain, suggesting it is independent of oligomerization. Coexpression with stargazin or with the flip isoform rescues the surface expression of GluR-D(flop) near to the level exhibited by GluR-D(flip). Our results demonstrate that the extracellular flip/flop region, via interactions with ER luminal splice form-specific protein(s), plays a hitherto unappreciated and important role in AMPA-receptor trafficking.

摘要

AMPA受体亚基的翻转和摆动剪接变体以不同但部分重叠的模式表达,并赋予同源受体通道不同的脱敏动力学。在缺乏特异性抗体的情况下,天然翻转和摆动亚基在运输或定位方面的亚型特异性差异仍未得到表征。我们报告,在几种转染细胞系中,同源谷氨酸受体(GluR)-D(摆动)受体的运输在内质网(ER)出口处基本受阻,而GluR-D(翻转)经历复杂的糖基化,并以比GluR-D(摆动)高10倍以上的水平到达质膜,这通过免疫荧光、膜片钳记录和生化分析确定。翻转和摆动之间的运输差异与活性无关,主要由氨基酸残基780(摆动中为亮氨酸,翻转中为缬氨酸)决定,甚至在可溶性配体结合域的分泌中也有体现,表明它与寡聚化无关。与stargazin或翻转亚型共表达可使GluR-D(摆动)的表面表达恢复到接近GluR-D(翻转)所显示的水平。我们的结果表明,细胞外翻转/摆动区域通过与内质网腔剪接形式特异性蛋白相互作用,在AMPA受体运输中发挥了迄今未被认识到的重要作用。

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