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Structure-function analysis of Hmo1 unveils an ancestral organization of HMG-Box factors involved in ribosomal DNA transcription from yeast to human

机译:Hmo1的结构功能分析揭示了HMG-Box因子的祖先组织参与了从酵母到人类的核糖体DNA转录

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摘要

Ribosome biogenesis is a major metabolic effort for growing cells. In Saccharomyces cerevisiae, Hmo1, an abundant high-mobility group box protein (HMGB) binds to the coding region of the RNA polymerase I transcribed ribosomal RNAs genes and the promoters of ∼70% of ribosomal protein genes. In this study, we have demonstrated the functional conservation of eukaryotic HMGB proteins involved in ribosomal DNA (rDNA) transcription. We have shown that when expressed in budding yeast, human UBF1 and a newly identified Sp-Hmo1 (Schizosaccharomyces pombe) localize to the nucleolus and suppress growth defect of the RNA polymerase I mutant rpa49-Δ. Owing to the multiple functions of both proteins, Hmo1 and UBF1 are not fully interchangeable. By deletion and domains swapping in Hmo1, we identified essential domains that stimulate rDNA transcription but are not fully required for stimulation of ribosomal protein genes expression. Hmo1 is organized in four functional domains: a dimerization module, a canonical HMGB motif followed by a conserved domain and a C-terminal nucleolar localization signal. We propose that Hmo1 has acquired species-specific functions and shares with UBF1 and Sp-Hmo1 an ancestral function to stimulate rDNA transcription.
机译:核糖体的生物发生是细胞生长的主要代谢途径。在酿酒酵母中,Hmo1是一种丰富的高迁移率族框蛋白(HMGB),它与转录了核糖体RNA基因的RNA聚合酶I和大约70%核糖体蛋白基因的启动子结合。在这项研究中,我们证明了参与核糖体DNA(rDNA)转录的真核HMGB蛋白的功能保守性。我们已经表明,当在发芽酵母中表达时,人UBF1和新近鉴定出的Sp-Hmo1(粟酒裂殖酵母)位于核仁中,并抑制RNA聚合酶I突变体rpa49-Δ的生长缺陷。由于两种蛋白质的多功能,Hmo1和UBF1不能完全互换。通过删除和Hmo1中的域交换,我们确定了刺激rDNA转录的必需域,但并不是完全需要刺激核糖体蛋白基因表达的域。 Hmo1被组织在四个功能域中:二聚化模块,规范的HMGB基序,其后是保守域和C端核仁定位信号。我们建议Hmo1已获得物种特定的功能,并与UBF1和Sp-Hmo1共享祖先功能,以刺激rDNA转录。

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