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转录因子Nrf1的一种新型剪接变体与TNFα启动子相互作用并刺激转录。

A novel splice variant of the transcription factor Nrf1 interacts with the TNFalpha promoter and stimulates transcription.

作者信息

Prieschl E E, Novotny V, Csonga R, Jaksche D, Elbe-Bürger A, Thumb W, Auer M, Stingl G, Baumruker T

机构信息

Department of Immunology, Novartis Research Institute, Brunner Strasse 59, A-1235 Vienna, Austria.

出版信息

Nucleic Acids Res. 1998 May 15;26(10):2291-7. doi: 10.1093/nar/26.10.2291.

Abstract

Common signaling chains of various receptor families, despite some similarities, are able to provoke quite different cellular responses. This suggests that they are linked to different cascades and transcription factors, dependent on the context of the ligand binding moiety and the cell type. The ITAM (immunoreceptor tyrosine-based activation motif) containing gamma chain of the FcepsilonRI, FcgammaRI, FcgammaRIII and the T-cell receptor is one of these shared signaling molecules. Here, we show that in the context of the FcgammaRIII, the gamma chain activates the transcription factor Nrf1 or a closely related protein that specifically interacts with the extended kappa3 site in the TNFalpha promoter. A novel splice variant of Nrf1 with a 411 bp deletion of the serine-rich region, resulting in an overall structure reminiscent of the BTB and CNC homology (Bach) proteins, was isolated from the corresponding DC18 cells. In a gel shift analysis, this bacterially expressed splice variant binds to the TNFalpha promoter site after in vitro phosphorylation by casein kinase II (CKII). In addition, cotransfection studies demonstrate that this splice variant mediates induced transcription at the TNFalpha promoter after stimulation/activation in a heterologous system.

摘要

各种受体家族的常见信号链尽管存在一些相似之处,但能够引发截然不同的细胞反应。这表明它们与不同的级联反应和转录因子相关联,这取决于配体结合部分的背景和细胞类型。含有免疫受体酪氨酸激活基序(ITAM)的FcepsilonRI、FcgammaRI、FcgammaRIII的γ链以及T细胞受体就是这些共享的信号分子之一。在此,我们表明,在FcgammaRIII的背景下,γ链激活转录因子Nrf1或一种与TNFα启动子中延伸的κ3位点特异性相互作用的密切相关蛋白。从相应的DC18细胞中分离出一种Nrf1的新型剪接变体,其富含丝氨酸区域缺失411 bp,导致整体结构让人联想到BTB和CNC同源(Bach)蛋白。在凝胶迁移分析中,这种细菌表达的剪接变体在经酪蛋白激酶II(CKII)体外磷酸化后与TNFα启动子位点结合。此外,共转染研究表明,这种剪接变体在异源系统中刺激/激活后介导TNFα启动子处的诱导转录。

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