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白细胞介素-2基因的染色质重塑:近端与远端增强子区域的不同改变。

Chromatin remodeling of the interleukin-2 gene: distinct alterations in the proximal versus distal enhancer regions.

作者信息

Ward S B, Hernandez-Hoyos G, Chen F, Waterman M, Reeves R, Rothenberg E V

机构信息

Division of Biology MC156-29, California Institute of Technology, Pasadena, CA 91125, USA.

出版信息

Nucleic Acids Res. 1998 Jun 15;26(12):2923-34. doi: 10.1093/nar/26.12.2923.

DOI:10.1093/nar/26.12.2923
PMID:9611237
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC147656/
Abstract

Known transcription factor-DNA interactions in the minimal enhancer of the murine interleukin-2 gene (IL-2) do not easily explain the T cell specificity of IL-2 regulation. To seek additional determinants of cell type specificity, in vivo methodologies were employed to examine chromatin structure 5' and 3' of the 300 bp IL-2 proximal promoter/enhancer region. Restriction enzyme accessibility revealed that until stimulation the IL-2 proximal promoter/enhancer exists in a closed conformation in resting T and non-T cells alike. Within this promoter region, DMS and DNase I genomic footprinting also showed no tissue-specific differences prior to stimulation. However, DNase I footprinting of the distal -600 to -300 bp region revealed multiple tissue-specific and stimulation-independent DNase I hypersensitive sites. Gel shift assays detected T cell-specific complexes binding within this region, which include TCF/LEF or HMG family and probable Oct family components. Upon stimulation, new DNase I hypersensitive sites appeared in both the proximal and distal enhancer regions, implying that there may be a functional interaction between these two domains. These studies indicate that a region outside the established IL-2 minimal enhancer may serve as a stable nucleation site for tissue-specific factors and as a potential initiation site for activation-dependent chromatin remodeling.

摘要

已知小鼠白细胞介素-2基因(IL-2)最小增强子中的转录因子与DNA的相互作用并不能轻易解释IL-2调控的T细胞特异性。为了寻找细胞类型特异性的其他决定因素,采用体内方法来检测300 bp IL-2近端启动子/增强子区域5'和3'端的染色质结构。限制性内切酶可及性分析表明,在刺激之前,IL-2近端启动子/增强子在静息T细胞和非T细胞中均以封闭构象存在。在该启动子区域内,二甲基亚砜(DMS)和DNase I基因组足迹分析也显示在刺激之前没有组织特异性差异。然而,对-600至-300 bp远端区域的DNase I足迹分析揭示了多个组织特异性且与刺激无关的DNase I超敏位点。凝胶迁移试验检测到该区域内结合的T细胞特异性复合物,其中包括TCF/LEF或HMG家族以及可能的Oct家族成分。刺激后,近端和远端增强子区域均出现新的DNase I超敏位点,这意味着这两个结构域之间可能存在功能相互作用。这些研究表明,已确定的IL-2最小增强子之外的区域可能作为组织特异性因子的稳定成核位点,并作为激活依赖性染色质重塑的潜在起始位点。

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GABP factors bind to a distal interleukin 2 (IL-2) enhancer and contribute to c-Raf-mediated increase in IL-2 induction.GA结合蛋白因子与远端白细胞介素2(IL-2)增强子结合,并有助于c-Raf介导的IL-2诱导增加。
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