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与相邻Sp1和富含AT元件结合的因子之间的互斥相互作用调节胰岛素瘤细胞中胃泌素基因的转录。

Mutually exclusive interactions between factors binding to adjacent Sp1 and AT-rich elements regulate gastrin gene transcription in insulinoma cells.

作者信息

Chung D C, Brand S J, Tillotson L G

机构信息

Gastrointestinal Unit, Massachusetts General Hospital, Boston 02114, USA.

出版信息

J Biol Chem. 1995 Apr 14;270(15):8829-36. doi: 10.1074/jbc.270.15.8829.

DOI:10.1074/jbc.270.15.8829
PMID:7721790
Abstract

The gastrin gene is transiently expressed in fetal pancreatic islets during islet neogenesis but then switched off after birth when islet cells become fully differentiated. Previous studies identified a cis-regulatory sequence between -109 and -75 in the human gastrin promoter which binds islet cell-specific activators and a nonspecific repressor and thus may act as a molecular switch. The present study identified another cis-regulatory sequence (-163ACACTAAATGAAAGGGCGGGGCAG-140) which bound two islet nuclear proteins in a mutually exclusive manner, as defined by gel shift competition, methylation interference, and DNase I foot-printing assays. The general transactivator Sp1 recognized the downstream GGGCGGGG sequence, but Sp1 binding was prevented when another islet factor bound to the adjacent AT-rich sequence (CTAAATGA). This gastrin AT-rich element is nearly identical to the binding site (ATAAATGA) for the islet-specific transcription factor beta TF-1. However, the gastrin AT-binding factor appeared to differ from beta TF-1 in its gel mobility shift pattern. Transfections of rat insulinoma cells revealed that mutations which blocked binding to the AT-rich element but allowed Sp1 binding up-regulated transcriptional activity. These results suggest that the gastrin AT-binding factor blocks transactivation by Sp1 and may have a role in the repression of gastrin transcription seen at the end of islet differentiation.

摘要

胃泌素基因在胰岛新生过程中于胎儿胰腺胰岛中短暂表达,但在出生后胰岛细胞完全分化时关闭。先前的研究在人胃泌素启动子中鉴定出一个位于-109至-75之间的顺式调控序列,该序列结合胰岛细胞特异性激活因子和一种非特异性阻遏物,因此可能充当分子开关。本研究鉴定出另一个顺式调控序列(-163ACACTAAATGAAAGGGCGGGGCAG-140),通过凝胶迁移竞争、甲基化干扰和DNase I足迹分析确定,该序列以互斥方式结合两种胰岛核蛋白。通用反式激活因子Sp1识别下游的GGGCGGGG序列,但当另一种胰岛因子与相邻富含AT的序列(CTAAATGA)结合时,Sp1的结合受到阻止。这种胃泌素富含AT的元件与胰岛特异性转录因子βTF-1的结合位点(ATAAATGA)几乎相同。然而,胃泌素AT结合因子在凝胶迁移率变动模式上似乎与βTF-1不同。大鼠胰岛素瘤细胞的转染显示,阻断与富含AT元件的结合但允许Sp1结合的突变上调了转录活性。这些结果表明,胃泌素AT结合因子阻断Sp1的反式激活作用,可能在胰岛分化末期所见的胃泌素转录抑制中起作用。

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Mutually exclusive interactions between factors binding to adjacent Sp1 and AT-rich elements regulate gastrin gene transcription in insulinoma cells.与相邻Sp1和富含AT元件结合的因子之间的互斥相互作用调节胰岛素瘤细胞中胃泌素基因的转录。
J Biol Chem. 1995 Apr 14;270(15):8829-36. doi: 10.1074/jbc.270.15.8829.
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