RUNX1 在缺乏同源 DNA 结合基团的情况下调节启动子活性

IF 3 3区 生物学 Q3 BIOCHEMISTRY & MOLECULAR BIOLOGY Journal of cellular biochemistry Pub Date : 2024-04-15 DOI:10.1002/jcb.30570
Alex M. Woodworth, Kristine Hardy, Phillippa C. Taberlay, Joanne L. Dickinson, Adele F. Holloway
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引用次数: 0

摘要

Runt 相关转录因子 1(RUNX1)在正常造血细胞的发育和功能中发挥着重要作用,其功能在白血病中经常受到破坏。RUNX1 被广泛认为是一种序列特异性 DNA 结合因子,能识别其靶基因启动子和增强子区域中的 5′-TG(T/C)GGT-3′。此外,RUNX1 融合蛋白(如由 t(8;21)易位形成的 RUNX1-ETO)仍能识别并结合该序列,从而对真正的 RUNX1 靶点产生非典型基因调控效应。然而,我们对公开的 RUNX1 染色质免疫沉淀测序(ChIP-Seq)数据进行的分析提供了挑战这一教条的证据,揭示了 RUNX1 招募和功能的这种图案特异性模型是不完整的。我们的分析表明,大多数 RUNX1 基因组定位发生在启动子之外,20% 的 RUNX1 结合位点缺乏共识 RUNX 基序,与远端位点相比,在启动子区域缺乏同源结合位点的情况下结合更为常见。报告实验证明,RUNX1 与 RUNX1-ETO 不同,可以在没有识别 DNA 结合基团的情况下驱动启动子的活性。当 RUNX1-ETO 被招募到含有序列特异性基调的启动子上时,它会抑制启动子的活性;有趣的是,它能与没有 RUNX1 识别位点的启动子结合,但不会抑制启动子的活性。这些数据表明,RUNX1 对靶基因的调控是通过多种机制进行的,这取决于基因组位置、调控元件类型和招募方式。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

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RUNX1 regulates promoter activity in the absence of cognate DNA binding motifs

Runt-related transcription factor 1 (RUNX1) plays an important role in normal haematopoietic cell development and function, and its function is frequently disrupted in leukaemia. RUNX1 is widely recognised as a sequence-specific DNA binding factor that recognises the motif 5′-TG(T/C)GGT-3′ in promoter and enhancer regions of its target genes. Moreover, RUNX1 fusion proteins, such as RUNX1-ETO formed by the t(8;21) translocation, retain the ability to recognise and bind to this sequence to elicit atypical gene regulatory effects on bona fide RUNX1 targets. However, our analysis of publicly available RUNX1 chromatin immunoprecipitation sequencing (ChIP-Seq) data has provided evidence challenging this dogma, revealing that this motif-specific model of RUNX1 recruitment and function is incomplete. Our analyses revealed that the majority of RUNX1 genomic localisation occurs outside of promoters, that 20% of RUNX1 binding sites lack consensus RUNX motifs, and that binding in the absence of a cognate binding site is more common in promoter regions compared to distal sites. Reporter assays demonstrate that RUNX1 can drive promoter activity in the absence of a recognised DNA binding motif, in contrast to RUNX1-ETO. RUNX1-ETO supresses activity when it is recruited to promoters containing a sequence specific motif, while interestingly, it binds but does not repress promoters devoid of a RUNX1 recognition site. These data suggest that RUNX1 regulation of target genes occurs through multiple mechanisms depending on genomic location, the type of regulatory element and mode of recruitment.

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来源期刊
Journal of cellular biochemistry
Journal of cellular biochemistry 生物-生化与分子生物学
CiteScore
9.90
自引率
0.00%
发文量
164
审稿时长
1 months
期刊介绍: The Journal of Cellular Biochemistry publishes descriptions of original research in which complex cellular, pathogenic, clinical, or animal model systems are studied by biochemical, molecular, genetic, epigenetic or quantitative ultrastructural approaches. Submission of papers reporting genomic, proteomic, bioinformatics and systems biology approaches to identify and characterize parameters of biological control in a cellular context are encouraged. The areas covered include, but are not restricted to, conditions, agents, regulatory networks, or differentiation states that influence structure, cell cycle & growth control, structure-function relationships.
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