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N-甲基-D-天冬氨酸受体亚基基因NMDAR1近端5'-侧翼区域的功能分析

Functional analysis of the proximal 5'-flanking region of the N-methyl-D-aspartate receptor subunit gene, NMDAR1.

作者信息

Bai G, Kusiak J W

机构信息

Molecular Neurobiology Unit, NIA, National Institutes of Health, Baltimore, Maryland 21224, USA.

出版信息

J Biol Chem. 1995 Mar 31;270(13):7737-44. doi: 10.1074/jbc.270.13.7737.

DOI:10.1074/jbc.270.13.7737
PMID:7706322
Abstract

The NMDAR1 receptor subunit is a common subunit of N-methyl-D-aspartate receptors. We have previously characterized 3 kilobases (kb) of 5'-flanking sequence of the NMDAR1 gene and now report on the ability of this region to direct transcription of a reporter gene and on its interaction with nuclear proteins. The sequence 356 base pairs (bp) 5' of the first nucleotide of codon 1 was sufficient to express a luciferase reporter gene in rat PC12 pheochromocytoma cells. Additional sequences upstream of nucleotide -356 influenced the activity approximately 2-fold. A labeled 112-bp fragment (position -356 to -245) formed six complexes (C1A and -B, C2A and -B, and C3A and -B), grouped as three double bands, with nuclear extracts from PC12 cells. Competition with Sp1 oligonucleotides abolished formation of C2A and -B and C3A and -B complexes. Sp1 antibody recognized the C3A complex in supershift experiments. Prior immunoprecipitation of nuclear extracts with Sp1 antibody abolished formation CA2 and -B and C3A and -B complexes. Purified Sp1 protein alone did not form a C3A complex but potentiated its formation when PC12 nuclear extract was added. A GC-rich sequence in this fragment was protected from DNase I digestion by nuclear extract. These results suggest that a 356-bp sequence comprises the NMDAR1 basal promoter, and that NMDAR1 gene expression may be regulated by Sp1-like nuclear factors.

摘要

NMDAR1受体亚基是N-甲基-D-天冬氨酸受体的一个常见亚基。我们之前已对NMDAR1基因5'侧翼序列的3千碱基(kb)进行了特征分析,现在报告该区域指导报告基因转录的能力及其与核蛋白的相互作用。密码子1第一个核苷酸上游356个碱基对(bp)的序列足以在大鼠PC12嗜铬细胞瘤细胞中表达荧光素酶报告基因。核苷酸-356上游的其他序列使活性增加了约2倍。一个标记的112 bp片段(位置-356至-245)与PC12细胞的核提取物形成了六个复合物(C1A和-B、C2A和-B以及C3A和-B),分为三个双链带。与Sp1寡核苷酸竞争可消除C2A和-B以及C3A和-B复合物的形成。在超迁移实验中,Sp1抗体识别C3A复合物。先用Sp1抗体对核提取物进行免疫沉淀可消除CA2和-B以及C3A和-B复合物的形成。单独的纯化Sp1蛋白不会形成C3A复合物,但加入PC12核提取物时会增强其形成。该片段中富含GC的序列受到核提取物对DNase I消化的保护。这些结果表明,一个356 bp的序列构成了NMDAR1基础启动子,并且NMDAR1基因表达可能受Sp1样核因子调控。

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