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Identification of E2F target genes that are rate limiting for dE2F1-dependent cell proliferation

机译:鉴定对dE2F1依赖性细胞增殖具有速率限制的E2F靶基因

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Background: Microarray studies have shown that the E2F transcription factor influences the expression of many genes but it is unclear how many of these targets are important for E2F-mediated control of cell proliferation. Results: We assembled a collection of mutant alleles of 44 dE2F1-dependent genes and tested whether these could modify visible phenotypes caused by the tissue-specific depletion of dE2F1. More than half of the mutant alleles dominantly enhanced de2f1-dsRNA phenotypes suggesting that the in vivo functions of dE2F1 can be limited by the reduction in the level of expression of many different targets. Unexpectedly, several mutant alleles suppressed de2f1-dsRNA phenotypes. One of the strongest of these suppressors was Orc5. Depletion of ORC5 increased proliferation in cells with reduced dE2F1 and specifically elevated the expression of dE2F1-regulated genes. Importantly, these effects were independent of dE2F1 protein levels, suggesting that reducing the level of ORC5 did not interfere with the general targeting of dE2F1. Conclusions: We propose that the interaction between ORC5 and dE2F1 may reflect a feedback mechanism between replication initiation proteins and dE2F1 that ensures that proliferating cells maintain a robust level of replication proteins for the next cell cycle.
机译:背景:微阵列研究表明E2F转录因子影响许多基因的表达,但尚不清楚这些靶中有多少对E2F介导的细胞增殖控制很重要。结果:我们收集了44个dE2F1依赖性基因的突变等位基因,并测试了这些基因是否可以修饰由dE2F1的组织特异性消耗引起的可见表型。一半以上的突变等位基因显着增强了de2f1-dsRNA表型,这表明dE2F1的体内功能可能受到许多不同靶标表达水平降低的限制。出乎意料的是,几个突变体等位基因抑制了de2f1-dsRNA表型。这些抑制器中最强大的一种是Orc5。减少ORC5会增加dE2F1减少的细胞的增殖,并特别提高dE2F1调控基因的表达。重要的是,这些作用与dE2F1蛋白水平无关,这表明降低ORC5的水平不会干扰dE2F1的总体靶向。结论:我们认为ORC5与dE2F1之间的相互作用可能反映了复制起始蛋白与dE2F1之间的反馈机制,该机制可确保增殖细胞在下一细胞周期中维持强大的复制蛋白水平。

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