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双链RNA激活NF-κB与人β-干扰素启动子中一个可诱导元件的结合。

Double-stranded RNA activates binding of NF-kappa B to an inducible element in the human beta-interferon promoter.

作者信息

Visvanathan K V, Goodbourn S

机构信息

Gene Expression Laboratory, Imperial Cancer Research Fund, London, UK.

出版信息

EMBO J. 1989 Apr;8(4):1129-38. doi: 10.1002/j.1460-2075.1989.tb03483.x.

Abstract

The human beta-interferon promoter contains at least two positive acting domains (PRD I and PRD II). PRD I has been previously shown to stimulate basal transcription and to respond to induction by double-stranded RNA (dsRNA). Here we show that PRD II functions independently as a constitutive element that also responds to induction. A cellular factor that specifically binds to PRD II has been identified, and the levels of this factor increase markedly in extracts from cells treated with dsRNA. The inducible factor has a binding specificity that is indistinguishable from the transcription factor NF-kappa B. As has been shown for NF-kappa B, the PRD II-specific factor can be activated in uninduced extracts by treatment with detergent, suggesting that the inactive state is due to association with an inhibitory factor. Induction by dsRNA therefore provides a novel means for the post-translational activation of NF-kappa B. Potential binding sites for NF-kappa B are present in the 5' flanking regions of a number of genes involved in the immune response, several of which are inducible by dsRNA. These findings demonstrate a role for NF-kappa B in the physiological activation of genes in non-lymphoid cells.

摘要

人β-干扰素启动子包含至少两个正向作用结构域(PRD I和PRD II)。先前已表明PRD I可刺激基础转录并对双链RNA(dsRNA)诱导作出反应。在此我们表明PRD II作为一个组成元件独立发挥作用,并且也对诱导作出反应。已鉴定出一种特异性结合PRD II的细胞因子,在用dsRNA处理的细胞提取物中该因子的水平显著增加。这种诱导性因子具有与转录因子NF-κB难以区分的结合特异性。正如对NF-κB所显示的那样,PRD II特异性因子可通过用去污剂处理在未诱导的提取物中被激活,这表明无活性状态是由于与一种抑制性因子结合所致。因此,dsRNA诱导为NF-κB的翻译后激活提供了一种新途径。在许多参与免疫反应的基因的5'侧翼区域存在NF-κB的潜在结合位点,其中一些基因可被dsRNA诱导。这些发现证明了NF-κB在非淋巴细胞中基因的生理激活中的作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3297/400924/d24def1375ca/emboj00128-0135-a.jpg

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