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聚合酶I反式激活因子上游结合因子与核小体的结合会取代连接组蛋白H1。

Nucleosome binding by the polymerase I transactivator upstream binding factor displaces linker histone H1.

作者信息

Kermekchiev M, Workman J L, Pikaard C S

机构信息

Biology Department, Washington University, St. Louis, Missouri 63130, USA.

出版信息

Mol Cell Biol. 1997 Oct;17(10):5833-42. doi: 10.1128/MCB.17.10.5833.

DOI:10.1128/MCB.17.10.5833
PMID:9315641
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC232431/
Abstract

Upstream binding factor (UBF) is a vertebrate RNA polymerase I transcription factor that can bend and wrap DNA. To investigate UBF's likely role as an architectural protein of rRNA genes organized in chromatin, we tested UBF's ability to bind rRNA gene enhancers assembled into nucleosome cores (DNA plus core histones) and nucleosomes (DNA plus core histones plus histone H1). UBF bound with low affinity to nucleosome cores formed with enhancer DNA probes of 162 bp. However, on nucleosome cores which contained approximately 60 bp of additional linker DNA, UBF bound with high affinity similar to its binding to naked DNA, forming a ternary DNA-core histone-UBF complex. UBF could be stripped from ternary complexes with competitor DNA to liberate nucleosome cores, rather than free DNA, suggesting that UBF binding to nucleosome cores does not displace the core histones H2A, H2B, H3, and H4. DNase I, micrococcal nuclease, and exonuclease III footprinting suggests that UBF and histone H1 interact with DNA on both sides flanking the histone octamer. Footprinting shows that UBF outcompetes histone H1 for binding to a nucleosome core and will displace, if not dissociate, H1 from its binding site on a preassembled nucleosome. These data suggest that UBF may act to prevent or reverse the assembly of transcriptionally inactive chromatin structures catalyzed by linker histone binding.

摘要

上游结合因子(UBF)是一种脊椎动物RNA聚合酶I转录因子,能够使DNA弯曲和缠绕。为了研究UBF作为染色质中rRNA基因的结构蛋白可能发挥的作用,我们测试了UBF结合组装成核小体核心(DNA加核心组蛋白)和核小体(DNA加核心组蛋白加组蛋白H1)的rRNA基因增强子的能力。UBF与由162 bp增强子DNA探针形成的核小体核心的结合亲和力较低。然而,对于含有约60 bp额外连接DNA的核小体核心,UBF以类似于其与裸DNA结合的高亲和力结合,形成三元DNA-核心组蛋白-UBF复合物。UBF可以用竞争DNA从三元复合物中剥离,以释放核小体核心,而不是游离DNA,这表明UBF与核小体核心的结合不会取代核心组蛋白H2A、H2B、H3和H4。DNase I、微球菌核酸酶和外切核酸酶III足迹分析表明,UBF和组蛋白H1与组蛋白八聚体两侧的DNA相互作用。足迹分析表明,UBF在与核小体核心结合方面比组蛋白H1更具竞争力,并且如果不能使其解离,将从预组装核小体上的结合位点取代H1。这些数据表明,UBF可能起到预防或逆转由连接组蛋白结合催化的转录无活性染色质结构组装的作用。

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