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NKx转录因子家族成员甲状腺转录因子1和心肌特异性同源盒蛋白(CSX)对小鼠克拉拉细胞特异性蛋白(mCC10)基因的转录调控

Transcriptional regulation of a mouse Clara cell-specific protein (mCC10) gene by the NKx transcription factor family members thyroid transciption factor 1 and cardiac muscle-specific homeobox protein (CSX).

作者信息

Ray M K, Chen C Y, Schwartz R J, DeMayo F J

机构信息

Department of Cell Biology, Baylor College of Medicine, Houston, Texas 77030, USA.

出版信息

Mol Cell Biol. 1996 May;16(5):2056-64. doi: 10.1128/MCB.16.5.2056.

Abstract

This report defines the elements between bp -800 and -166 that regulate the quantitative level of mouse CC10 (mCC10) transcription in the lungs. The elements in this promoter domain are the response elements for the NKx2.1 homeobox protein, thyroid transcription factor 1 (TTF1). DNase I footprint analysis identified five binding sites for TTF1 between bp -800 and - 166. These sites are located at bp -344 to -335, - 282 to -273, -268 to -263, -258 to -249, and - 199 to - 190. In addition to these enhancer elements, two TTF1 binding sites were identified in the proximal promoter region (bp - 166 to + 1), at bp -74 to -69 and -49 to -39. An identical footprint of the mCC10 promoter region was also observed with another member of the NKx family, NKx 2.5, the cardiac muscle-specific homeobox protein (CSX). Deletion and linker-scanner mutational analyses of the TTF1 binding sites in the mCC10 distal promoter region with transient cotransfection into CV1 cells with either TTF1 or CSX identified the site located between bp -282 and -273 as the major regulator of CC10 expression, with minor regulation by sites at bp -344 to -335 and -258 to -249. The importance of the NKx binding site at bp -282 to -273 was verified in vivo. Transgenic mice generated with the human growth hormone gene fused to 800 bp of the mCC10 promoter containing a mutation in the TTF1 binding site at bp -282 to -273 showed a reduction in transgene expression equal to that of the mice generated with only 166 bp of 5'-flanking DNA. This report emphasizes the importance of TTF1 or related factors as major regulators of pulmonary gene expression and demonstrates the potential of NKx proteins to bind and activate heterologous target genes.

摘要

本报告确定了bp -800至-166之间调控小鼠肺组织中CC10(mCC10)转录定量水平的元件。该启动子区域中的元件是NKx2.1同源框蛋白(甲状腺转录因子1,TTF1)的反应元件。DNA酶I足迹分析确定了bp -800至-166之间TTF1的五个结合位点。这些位点位于bp -344至-335、-282至-273、-268至-263、-258至-249以及-199至-190处。除了这些增强子元件外,在近端启动子区域(bp -166至+1)还确定了两个TTF1结合位点,分别位于bp -74至-69和-49至-39处。NKx家族的另一个成员NKx 2.5(心肌特异性同源框蛋白,CSX)对mCC10启动子区域也有相同的足迹。通过将mCC10远端启动子区域中TTF1结合位点进行缺失和连接子扫描突变分析,并与TTF1或CSX一起瞬时共转染到CV1细胞中,确定位于bp -282至-273之间的位点是CC10表达的主要调节因子,bp -344至-335和-258至-249处的位点起次要调节作用。bp -282至-273处NKx结合位点在体内的重要性得到了验证。用人生长激素基因与mCC10启动子的800 bp融合构建转基因小鼠,该启动子在bp -282至-273处的TTF1结合位点发生突变,结果显示转基因表达降低,与仅用5'侧翼DNA的166 bp构建的小鼠相同。本报告强调了TTF1或相关因子作为肺基因表达主要调节因子的重要性,并证明了NKx蛋白结合和激活异源靶基因的潜力。

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