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视网膜母细胞瘤缺失型成红细胞中E2f-2失调是细胞周期和成熟缺陷的基础。

Deregulated E2f-2 underlies cell cycle and maturation defects in retinoblastoma null erythroblasts.

作者信息

Dirlam Alexandra, Spike Benjamin T, Macleod Kay F

机构信息

Ben May Department for Cancer Research, Gordon Center for Integrative Sciences, The University of Chicago, 929 East 57th Street, Chicago, IL 60637, USA.

出版信息

Mol Cell Biol. 2007 Dec;27(24):8713-28. doi: 10.1128/MCB.01118-07. Epub 2007 Oct 8.

Abstract

By assessing the contribution of deregulated E2F activity to erythroid defects in Rb null mice, we have identified E2f-2 as being upregulated in end-stage red cells, where we show it is the major pRb-associated E2f and the predominant E2f detected at key target gene promoters. Consistent with its expression pattern, E2f-2 loss restored terminal erythroid maturation to Rb null red cells, including the ability to undergo enucleation. Deletion of E2f-2 also extended the life span of Rb null mice despite persistent defects in placental development, indicating that deregulated E2f-2 activity in differentiating erythroblasts contributes to the premature lethality of Rb null mice. We show that the aberrant entry of Rb null erythroblasts into S phase at times in differentiation when wild-type erythroblasts are exiting the cell cycle is inhibited by E2f-2 deletion. E2f-2 loss induced cell cycle arrest in both wild-type and Rb null erythroblasts and was associated with increased DNA double-strand breaks. These results implicate deregulated E2f-2 in the cell cycle defects observed in Rb null erythroblasts and reveal a novel role for E2f-2 during terminal red blood cell differentiation. The identification of a tissue-restricted role for E2f-2 in erythropoiesis highlights the nonredundant nature of E2f transcription factor activities in cell growth and differentiation.

摘要

通过评估E2F活性失调对Rb基因敲除小鼠红细胞缺陷的影响,我们发现E2f-2在终末阶段红细胞中上调,我们的研究表明它是与磷酸化Rb(pRb)相关的主要E2f,也是在关键靶基因启动子处检测到的主要E2f。与其表达模式一致,E2f-2缺失使Rb基因敲除的红细胞恢复了终末红细胞成熟,包括去核能力。E2f-2的缺失也延长了Rb基因敲除小鼠的寿命,尽管胎盘发育存在持续缺陷,这表明分化中的成红细胞中E2f-2活性失调导致了Rb基因敲除小鼠的过早死亡。我们发现,E2f-2缺失可抑制Rb基因敲除的成红细胞在野生型成红细胞退出细胞周期的分化阶段异常进入S期。E2f-2缺失在野生型和成红细胞中均诱导细胞周期停滞,并与DNA双链断裂增加有关。这些结果表明,E2f-2活性失调与Rb基因敲除的成红细胞中观察到的细胞周期缺陷有关,并揭示了E2f-2在终末红细胞分化过程中的新作用。E2f-2在红细胞生成中组织限制性作用的确定突出了E2f转录因子活性在细胞生长和分化中的非冗余性质。

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