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REGULATION OF RAT DOPAMINE β-HYDROXYLASE GENE TRANSCRIPTION BY EARLY GROWTH RESPONSE GENE 1 (EGR1)

机译:早期生长反应基因1(EGR1)对大鼠多巴胺β-羟化酶基因转录的调控

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摘要

Egr1, a transcription factor rapidly induced by various stimuli including stress, can elevate transcription of genes for the catecholamine biosynthetic enzymes TH and PNMT. To examine if Egr1 also regulates dopamine β-hydroxylase (DBH) gene expression, PC12 cells were transfected with expression vector for full length or truncated inactive Egr1 and various DBH promoter-driven luciferase constructs. While Egr1 elevated TH promoter activity, DBH promoter activity was reduced. The reduction occurred as early as 4 h and reached maximal inhibition 16–40 h after transfection. Egr1 also reduced the expression of endogenous DBH mRNA and the induction of DBH promoter activity by cAMP. These effects were not observed with truncated Egr1 lacking the DNA binding domain. The first 247, but not 200, nucleotides of DBH promoter are sufficient for this suppression. Several putative Egr1 motifs were identified, and mutagenesis showed that the motif at −227/−224 is required. Binding of Egr1 to this region of the DBH promoter was verified by chromatin immunoprecipitation and electrophoretic mobility shift assays. This study demonstrates that DBH promoter contains at least one functional Egr1 motif; and indicates, for the first time, that Egr1 can play an inhibitory role in regulation of DBH gene transcription.
机译:Egr1是一种由多种刺激(包括压力)迅速诱导的转录因子,可以提高儿茶酚胺生物合成酶TH和PNMT的基因转录。为了检查Egr1是否也调节多巴胺β-羟化酶(DBH)基因表达,将PC12细胞用表达载体转染了全长或截短的非活性Egr1和各种DBH启动子驱动的荧光素酶构建体。虽然Egr1提高TH启动子活性,但DBH启动子活性降低。减少最早在4 h发生,转染后16–40 h达到最大抑制。 Egr1还减少了内源性DBH mRNA的表达以及cAMP对DBH启动子活性的诱导。对于缺少DNA结合域的截短的Egr1,未观察到这些效果。 DBH启动子的前247个而不是200个核苷酸足以进行这种抑制。鉴定了几个推定的Egr1基序,诱变表明在-227 / -224位基序是必需的。 Egr1结合到DBH启动子的这一区域已通过染色质免疫沉淀和电泳迁移率变动分析进行了验证。这项研究表明,DBH启动子包含至少一个功能性的Egr1基序。并首次表明Egr1在调节DBH基因转录中起抑制作用。

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