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N-聚糖在AMPA受体配体结合结构域中的功能作用表征。

Characterization of the functional role of the N-glycans in the AMPA receptor ligand-binding domain.

作者信息

Pasternack Arja, Coleman Sarah K, Féthière James, Madden Dean R, LeCaer Jean-Pierre, Rossier Jean, Pasternack Michael, Keinänen Kari

机构信息

Viikki Biocenter, Department of Biosciences (Division of Biochemistry), Viikinkaari 5D, FIN-00014 University of Helsinki, Finland.

出版信息

J Neurochem. 2003 Mar;84(5):1184-92. doi: 10.1046/j.1471-4159.2003.01611.x.

DOI:10.1046/j.1471-4159.2003.01611.x
PMID:12603841
Abstract

The ligand-binding domains of AMPA receptor subunits carry two conserved N-glycosylation sites. In order to gain insight into the functional role of the corresponding N-glycans, we examined how the elimination of glycosylation at these sites (N407 and N414) affects the ligand-binding characteristics, structural stability, cell-surface expression, and channel properties of homomeric GluR-D (GluR4) receptor and its soluble ligand-binding domain (S1S2). GluR-D S1S2 protein expressed as a secreted protein in insect cells was found to be glycosylated at N407 and N414. No major differences in the ligand-binding properties were observed between the 'wild-type' S1S2 and non-glycosylated N407D/N414Q double mutant, or between S1S2 proteins expressed in the presence or absence of tunicamycin, an inhibitor of N-glycosylation. Purified glycosylated and non-glycosylated S1S2 proteins also showed similar thermostabilities as determined by CD spectroscopy. Full-length homomeric GluR-D receptor with N407D/N414Q mutation was expressed on the surface of HEK293 cells like the wild-type GluR-D. In outside-out patches, GluR-D and the N407D/N414Q mutant produced similar rapidly desensitizing current responses to glutamate and AMPA. We therefore report that the two conserved ligand-binding domain glycans do not play any major role in receptor-ligand interactions, do not impart a stabilizing effect on the ligand-binding domain, and are not critical for the formation and surface localization of homomeric GluR-D AMPA receptors in HEK293 cells.

摘要

AMPA受体亚基的配体结合结构域带有两个保守的N-糖基化位点。为了深入了解相应N-聚糖的功能作用,我们研究了消除这些位点(N407和N414)的糖基化如何影响同聚体GluR-D(GluR4)受体及其可溶性配体结合结构域(S1S2)的配体结合特性、结构稳定性、细胞表面表达和通道特性。在昆虫细胞中作为分泌蛋白表达的GluR-D S1S2蛋白在N407和N414处被糖基化。在“野生型”S1S2与非糖基化的N407D/N414Q双突变体之间,或在存在或不存在N-糖基化抑制剂衣霉素的情况下表达的S1S2蛋白之间,未观察到配体结合特性的主要差异。通过圆二色光谱法测定,纯化的糖基化和非糖基化S1S2蛋白也表现出相似的热稳定性。具有N407D/N414Q突变的全长同聚体GluR-D受体像野生型GluR-D一样在HEK293细胞表面表达。在外翻膜片上,GluR-D和N407D/N414Q突变体对谷氨酸和AMPA产生了相似的快速脱敏电流反应。因此,我们报道这两个保守的配体结合结构域聚糖在受体-配体相互作用中不发挥任何主要作用,对配体结合结构域没有稳定作用,并且对于HEK293细胞中同聚体GluR-D AMPA受体的形成和表面定位也不是关键的。

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