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转录因子xUBF对非洲爪蟾核糖体核心启动子的识别涉及多个HMG盒结构域,并导致xUBF结构域间相互作用。

Recognition of the Xenopus ribosomal core promoter by the transcription factor xUBF involves multiple HMG box domains and leads to an xUBF interdomain interaction.

作者信息

Leblanc B, Read C, Moss T

机构信息

Centre de Recherche en Cancérologie, Université Laval, Hôtel-Dieu de Québec, Canada.

出版信息

EMBO J. 1993 Feb;12(2):513-25. doi: 10.1002/j.1460-2075.1993.tb05683.x.

Abstract

The interaction of the ribosomal transcription factor xUBF with the RNA polymerase I core promoter of Xenopus laevis has been studied both at the DNA and protein levels. It is shown that a single xUBF-DNA complex forms over the 40S initiation site (+1) and involves at least the DNA sequences between -20 and +60 bp. DNA sequences upstream of +10 and downstream of +18 are each sufficient to direct complex formation independently. HMG box 1 of xUBF independently recognizes the sequences -20 to -1 and +1 to +22 and the addition of the N-terminal dimerization domain to HMG box 1 stabilizes its interaction with these sequences approximately 10-fold. HMG boxes 2/3 interact with the DNA downstream of +22 and can independently position xUBF across the initiation site. The C-terminal segment of xUBF, HMG boxes 4, 5 or the acidic domain, directly or indirectly interact with HMG box 1, making the core promoter sequences between -11 and -15 hypersensitive to DNase. This interaction also requires the DNA sequences between +17 and +32, i.e. the HMG box 2/3 binding site. The data suggest extensive folding of the core promoter within the xUBF complex.

摘要

已在DNA和蛋白质水平上研究了非洲爪蟾核糖体转录因子xUBF与非洲爪蟾RNA聚合酶I核心启动子的相互作用。结果表明,在40S起始位点(+1)上形成了单一的xUBF-DNA复合物,且至少涉及-20至+60 bp之间的DNA序列。+10上游和+18下游的DNA序列各自足以独立指导复合物的形成。xUBF的HMG框1独立识别-20至-1和+1至+22的序列,并且将N端二聚化结构域添加到HMG框1可使其与这些序列的相互作用稳定约10倍。HMG框2/3与+22下游的DNA相互作用,并可独立地将xUBF定位在起始位点上。xUBF的C端片段、HMG框4、5或酸性结构域直接或间接与HMG框1相互作用,使-11至-15之间的核心启动子序列对DNase高度敏感。这种相互作用还需要+17至+32之间的DNA序列,即HMG框2/3结合位点。数据表明核心启动子在xUBF复合物中发生了广泛折叠。

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