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N-甲基-D-天冬氨酸受体亚基家族的分子特征

Molecular characterization of the family of the N-methyl-D-aspartate receptor subunits.

作者信息

Ishii T, Moriyoshi K, Sugihara H, Sakurada K, Kadotani H, Yokoi M, Akazawa C, Shigemoto R, Mizuno N, Masu M

机构信息

Institute for Immunology, Kyoto University Faculty of Medicine, Japan.

出版信息

J Biol Chem. 1993 Feb 5;268(4):2836-43.

PMID:8428958
Abstract

cDNA clones for four different N-methyl-D-aspartate (NMDA) receptor subunits (NMDAR2A-NMDAR2D) were isolated through polymerase chain reactions followed by molecular screening of a rat brain cDNA library. These subunits are only about 15% identical with the key subunit of the NMDA receptor (NMDAR1) but are highly homologous (approximately 50% homology) with one another. They also commonly possess large hydrophilic domains at both amino- and carboxyl-terminal sides of the four putative transmembrane segments. NMDAR2A and NMDAR2C expressed individually in Xenopus oocytes showed no electrophysiological response to agonists. However, these subunits in combined expression with NMDAR1 markedly potentiated the NMDAR1 activity and produced functional variability in the affinity of agonists, the effectiveness of antagonists, and the sensitivity to Mg2+ blockade. Thus, NMDAR1 is essential for the function of the NMDA receptor, and multiple NMDAR2 subunits potentiate and differentiate the function of the NMDA receptor by forming different heteromeric configurations with NMDAR1. Northern blotting and in situ hybridization analyses revealed that the expressions of individual mRNAs for the NMDAR2 subunits overlap in some brain regions but are also specialized in many other regions. This investigation demonstrates the anatomical and functional differences of the NMDAR2 subunits, which provide the molecular basis for the functional diversity of the NMDA receptor.

摘要

通过聚合酶链反应,随后对大鼠脑cDNA文库进行分子筛选,分离出了四种不同的N-甲基-D-天冬氨酸(NMDA)受体亚基(NMDAR2A-NMDAR2D)的cDNA克隆。这些亚基与NMDA受体的关键亚基(NMDAR1)仅有约15%的同一性,但彼此之间具有高度同源性(约50%的同源性)。它们在四个假定的跨膜片段的氨基和羧基末端通常也都具有大的亲水区。在非洲爪蟾卵母细胞中单独表达的NMDAR2A和NMDAR2C对激动剂无电生理反应。然而,这些亚基与NMDAR1联合表达时,显著增强了NMDAR1的活性,并在激动剂亲和力、拮抗剂效力以及对Mg2+阻断的敏感性方面产生了功能变异性。因此,NMDAR1对NMDA受体的功能至关重要,多个NMDAR2亚基通过与NMDAR1形成不同的异聚体构型来增强和区分NMDA受体的功能。Northern印迹和原位杂交分析显示,NMDAR2亚基各自的mRNA表达在一些脑区有重叠,但在许多其他区域也具有特异性。这项研究证明了NMDAR2亚基的解剖学和功能差异,为NMDA受体的功能多样性提供了分子基础。

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