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鉴定人类心肌肌钙蛋白I基因启动子表达所需的顺式作用DNA元件。

Identification of cis-acting DNA elements required for expression of the human cardiac troponin I gene promoter.

作者信息

Bhavsar P K, Dellow K A, Yacoub M H, Brand N J, Barton P J

机构信息

National Heart and Lung Institute, Imperial College School of Medicine, Dovehouse Street, London, SW3 6LY, UK.

出版信息

J Mol Cell Cardiol. 2000 Jan;32(1):95-108. doi: 10.1006/jmcc.1999.1058.

DOI:10.1006/jmcc.1999.1058
PMID:10652194
Abstract

The human cardiac troponin I (TnIc) gene exhibits both cardiac-specific and developmentally regulated expression. The structure and expression of this gene as well as the identification of putative regulatory elements have been described previously. This study shows that a minimal promoter containing 98 bp of sequence is sufficient to drive transcription in neonatal rat cardiac myocytes. This region contains several putative cis -regulatory elements including an Initiator element surrounding the start site of transcription, an A/T-rich (TATA/MEF-2) element, two GATA elements and a cytosine-rich region containing overlapping CACC box and Sp1 elements. Using electrophoretic mobility shift assays (EMSAs) this study demonstrates the binding of MEF-2, Oct-1, and recombinant TBP to the A/T-rich element and of GATA-4 to both GATA elements. The CACC/Sp element binds the zinc finger transcription factors Sp1 and Sp3 in addition to an unidentified complex present in neonatal rat cardiac myocytes. Mutation of each of these sites has a deleterious effect on promoter activity as assayed by transient transfection into cardiac myocytes. The data suggest that transcriptional activity of the human TnIc gene can be driven by a compact promoter region and that within this region GATA, MEF-2 Sp1 and CACC box-binding factors are required for optimal activity. Furthermore, a comparison with data obtained for identical elements in the promoters of rodent TnIc genes identifies differences between species which may be of consequence for species-specific promoter function.

摘要

人类心肌肌钙蛋白I(TnIc)基因表现出心脏特异性和发育调控性表达。该基因的结构与表达以及假定调控元件的鉴定先前已有描述。本研究表明,一个包含98个碱基对序列的最小启动子足以驱动新生大鼠心肌细胞中的转录。该区域包含几个假定的顺式调控元件,包括围绕转录起始位点的起始元件、一个富含A/T的(TATA/MEF-2)元件、两个GATA元件以及一个富含胞嘧啶的区域,该区域包含重叠的CACC框和Sp1元件。利用电泳迁移率变动分析(EMSA),本研究证明了MEF-2、Oct-1和重组TBP与富含A/T的元件结合,以及GATA-4与两个GATA元件结合。CACC/Sp元件除了与新生大鼠心肌细胞中存在的一种未鉴定复合物结合外,还与锌指转录因子Sp1和Sp3结合。通过瞬时转染心肌细胞进行检测,这些位点中的每一个发生突变都会对启动子活性产生有害影响。数据表明,人类TnIc基因的转录活性可由一个紧凑的启动子区域驱动,并且在该区域内,GATA、MEF-2、Sp1和CACC框结合因子是实现最佳活性所必需的。此外,与啮齿动物TnIc基因启动子中相同元件所获得的数据进行比较,确定了物种之间的差异,这些差异可能对物种特异性启动子功能具有重要意义。

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