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果蝇Myb和E2F2-RBF通过Myb-MuvB/dREAM复合物对基因表达进行表观遗传调控。

Epigenetic regulation of gene expression by Drosophila Myb and E2F2-RBF via the Myb-MuvB/dREAM complex.

作者信息

Wen Hong, Andrejka Laura, Ashton Jonathan, Karess Roger, Lipsick Joseph S

机构信息

Department of Pathology and Department of Genetics, Stanford University, Stanford, CA 94305, USA.

出版信息

Genes Dev. 2008 Mar 1;22(5):601-14. doi: 10.1101/gad.1626308.

Abstract

The Drosophila Myb oncoprotein, the E2F2 transcriptional repressor, and the RBF and Mip130/LIN-9 tumor suppressor proteins reside in a conserved Myb-MuvB (MMB)/dREAM complex. We now show that Myb is required in vivo for the expression of Polo kinase and components of the spindle assembly checkpoint (SAC). Surprisingly, the highly conserved DNA-binding domain was not essential for assembly of Myb into MMB/dREAM, for transcriptional regulation in vivo, or for rescue of Myb-null mutants to adult viability. E2F2, RBF, and Mip130/LIN-9 acted in opposition to Myb by repressing the expression of Polo and SAC genes in vivo. Remarkably, the absence of both Myb and Mip130, or of both Myb and E2F2, caused variegated expression in which high or low levels of Polo were stably inherited through successive cell divisions in imaginal wing discs. Restoration of Myb resulted in a uniformly high level of Polo expression similar to that seen in wild-type tissue, whereas restoration of Mip130 or E2F2 extinguished Polo expression. Our results demonstrate epigenetic regulation of gene expression by Myb, Mip130/LIN-9, and E2F2-RBF in vivo, and also provide an explanation for the ability of Mip130-null mutants to rescue the lethality of Myb-null mutants in vivo.

摘要

果蝇Myb癌蛋白、E2F2转录抑制因子以及RBF和Mip130/LIN-9肿瘤抑制蛋白存在于保守的Myb-MuvB(MMB)/dREAM复合物中。我们现在表明,Myb在体内是Polo激酶和纺锤体组装检查点(SAC)组分表达所必需的。令人惊讶的是,高度保守的DNA结合结构域对于Myb组装到MMB/dREAM中、体内转录调控或拯救Myb基因缺失突变体至成年存活并非必需。E2F2、RBF和Mip130/LIN-9在体内通过抑制Polo和SAC基因的表达与Myb起相反作用。值得注意的是,Myb和Mip130两者缺失,或Myb和E2F2两者缺失,会导致斑驳表达,其中高水平或低水平的Polo在成虫翅盘中通过连续细胞分裂稳定遗传。Myb的恢复导致Polo表达水平均匀升高,类似于野生型组织中的情况,而Mip130或E2F2的恢复则消除了Polo表达。我们的结果证明了Myb、Mip130/LIN-9和E2F2-RBF在体内对基因表达的表观遗传调控,也为Mip130基因缺失突变体在体内拯救Myb基因缺失突变体致死性的能力提供了解释。

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