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X-ray Structure of a NF-κB p50/RelB/DNA Complex Reveals Assembly of Multiple Dimers on Tandem κB Sites

机译:NF-κBp50 / RelB / DNA复合体的X射线结构揭示了串联κB位点上多个二聚体的组装。

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摘要

We describe here the X-ray crystal structure of NF-κB p50/RelB heterodimer bound to a κB DNA. Although the global modes of subunit association and κB DNA recognition are similar to other NF-κB/DNA complexes, this complex reveals distinctive features not observed for non-RelB complexes. For example, Lys274 of RelB is removed from the protein–DNA interface whereas the corresponding residues in all other subunits make base-specific contacts. This mode of binding suggests that RelB may allow the recognition of more diverse κB sequences. Complementary surfaces on RelB and p50, as revealed by the crystal contacts, are highly suggestive of assembly of multiple p50/RelB heterodimers on tandem κB sites in solution. Consistent with this model our in vitro binding experiments reveal optimal assembly of two wild-type p50/RelB heterodimers on tandem HIV κB DNA with 2 bp spacing but not by a mutant heterodimer where one of the RelB packing surface is altered. We suggest that multiple NF-κB dimers assemble at diverse κB promoters through direct interactions utilizing unique protein–protein interaction surfaces.
机译:我们在这里描述与κBDNA结合的NF-κBp50 / RelB异二聚体的X射线晶体结构。尽管亚基缔合和κBDNA识别的整体模式与其他NF-κB/ DNA复合体相似,但该复合体显示出非RelB复合体未观察到的独特特征。例如,RelB的Lys274从蛋白质-DNA界面中去除,而所有其他亚基中的相应残基形成碱基特异性接触。这种结合方式表明,RelB可能允许识别更多种κB序列。如晶体接触所揭示的,RelB和p50上的互补表面高度暗示了溶液中串联κB位点上的多个p50 / RelB异二聚体的组装。与该模型一致,我们的体外结合实验揭示了两个野生型p50 / RelB异二聚体在2 bp间隔的串联HIVκBDNA上的最佳组装,但没有被RelB堆积表面之一改变的突变异二聚体组成。我们建议通过利用独特的蛋白质-蛋白质相互作用表面的直接相互作用,多个NF-κB二聚体在不同的κB启动子处聚集。

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