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E2f3a和E2f3b对E2f3总活性的贡献有重叠但又不同。

E2f3a and E2f3b make overlapping but different contributions to total E2f3 activity.

作者信息

Danielian P S, Friesenhahn L B, Faust A M, West J C, Caron A M, Bronson R T, Lees J A

机构信息

David H. Koch Institute for Integrative Cancer Research, Massachusetts Institute of Technology, Cambridge, MA 02139, USA.

出版信息

Oncogene. 2008 Nov 20;27(51):6561-70. doi: 10.1038/onc.2008.253. Epub 2008 Jul 28.

Abstract

The E2f transcription factors are key downstream targets of the retinoblastoma protein tumor suppressor that control cell proliferation. E2F3 has garnered particular attention because it is amplified in various human tumors. E2f3 mutant mice typically die around birth and E2f3-deficient cells have a proliferation defect that correlates with impaired E2f target gene activation and also induction of p19(Arf) and p53. The E2f3 locus encodes two isoforms, E2f3a and E2f3b, which differ in their N-termini. However, it is unclear how E2f3a versus E2f3b contributes to E2f3's requirement in either proliferation or development. To address this, we use E2f3a- and E2f3b-specific knockouts. We show that inactivation of E2f3a results in a low penetrance proliferation defect in vitro whereas loss of E2f3b has no effect. This proliferation defect appears insufficient to disrupt normal development as E2f3a and E2f3b mutant mice are both fully viable and have no detectable defects. However, when combined with E2f1 mutation, inactivation of E2f3a, but not E2f3b, causes significant proliferation defects in vitro, neonatal lethality and also a striking cartilage defect. Thus, we conclude that E2f3a and E2f3b have largely overlapping functions in vivo and that E2f3a can fully substitute for E2f1 and E2f3 in most murine tissues.

摘要

E2f转录因子是视网膜母细胞瘤蛋白肿瘤抑制因子的关键下游靶点,可控制细胞增殖。E2F3因其在多种人类肿瘤中发生扩增而备受关注。E2f3突变小鼠通常在出生前后死亡,E2f3缺陷细胞具有增殖缺陷,这与E2f靶基因激活受损以及p19(Arf)和p53的诱导有关。E2f3基因座编码两种异构体,E2f3a和E2f3b,它们的N端不同。然而,尚不清楚E2f3a与E2f3b在增殖或发育过程中对E2f3的需求有何贡献。为了解决这个问题,我们使用了E2f3a和E2f3b特异性敲除。我们发现,E2f3a的失活在体外导致低 penetrance 增殖缺陷,而E2f3b的缺失则没有影响。这种增殖缺陷似乎不足以破坏正常发育,因为E2f3a和E2f3b突变小鼠都完全存活且没有可检测到的缺陷。然而,当与E2f1突变结合时,E2f3a的失活而非E2f3b的失活在体外导致显著的增殖缺陷、新生儿致死率以及明显的软骨缺陷。因此,我们得出结论,E2f3a和E2f3b在体内具有很大程度的重叠功能,并且E2f3a在大多数小鼠组织中可以完全替代E2f1和E2f3。

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