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内皮细胞中组织因子启动子的调控。NF-κB、AP-1和Sp1样转录因子的结合。

Regulation of the tissue factor promoter in endothelial cells. Binding of NF kappa B-, AP-1-, and Sp1-like transcription factors.

作者信息

Moll T, Czyz M, Holzmüller H, Hofer-Warbinek R, Wagner E, Winkler H, Bach F H, Hofer E

机构信息

Department of Transplantation Immunology, Vienna International Research Cooperation Center, Vienna, Austria.

出版信息

J Biol Chem. 1995 Feb 24;270(8):3849-57. doi: 10.1074/jbc.270.8.3849.

DOI:10.1074/jbc.270.8.3849
PMID:7876129
Abstract

Tissue factor is up-regulated on endothelial cells and monocytes in response to cytokines and endotoxin and is the main trigger of the extrinsic pathway of the coagulation cascade. We have isolated the porcine tissue factor gene and studied the regulation of the promoter, which has not been investigated previously in endothelial cells. Comparison of the promoter sequences with the respective human and murine genes reveals short stretches of homology, which encompass potential binding sites for AP-1, NF kappa B, and Sp1 transcription factors. Using DNase I footprinting, we detect binding of nuclear factors to these promoter elements. Transfection experiments demonstrate that a 300-base pair fragment containing the conserved elements can mediate induced transcription and that the NF kappa B-like element is essential. In accordance, electrophoretic mobility shift assays show a strong increase in the binding of factors to the NF kappa B-like site following induction. We further provide evidence that RelA (p65), c-Rel, and possibly novel polypeptides bind to the tissue factor NF kappa B element. In addition, we show constitutive binding of members of the Fos/Jun and Sp1 families to the AP-1 and Sp1 sites, respectively. We propose a concerted action of AP-1-, NF kappa B-, and Sp1-like factors in transcription from the tissue factor promoter in endothelial cells.

摘要

组织因子在内皮细胞和单核细胞上因细胞因子和内毒素而上调,是凝血级联反应外源性途径的主要触发因素。我们已分离出猪组织因子基因,并研究了其启动子的调控,此前尚未在内皮细胞中对此进行过研究。将该启动子序列与相应的人类和小鼠基因进行比较,发现了短片段的同源性,其中包括AP-1、核因子κB和Sp1转录因子的潜在结合位点。使用DNA酶I足迹法,我们检测到核因子与这些启动子元件的结合。转染实验表明,一个包含保守元件的300个碱基对的片段可以介导诱导转录,并且核因子κB样元件至关重要。相应地,电泳迁移率变动分析显示,诱导后因子与核因子κB样位点的结合显著增加。我们进一步提供证据表明,RelA(p65)、c-Rel以及可能的新多肽与组织因子核因子κB元件结合。此外,我们分别显示了Fos/Jun家族成员和Sp1家族成员与AP-1位点和Sp1位点的组成性结合。我们提出,AP-1、核因子κB和Sp1样因子在内皮细胞中组织因子启动子的转录过程中协同发挥作用。

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