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独特的 Oct4 界面对于重编程为多能性至关重要。

A unique Oct4 interface is crucial for reprogramming to pluripotency.

机构信息

Department for Cell and Developmental Biology, Max Planck Institute for Molecular Biomedicine, Röntgenstrasse 20, Münster D-48149, Germany.

出版信息

Nat Cell Biol. 2013 Mar;15(3):295-301. doi: 10.1038/ncb2680. Epub 2013 Feb 3.

Abstract

Terminally differentiated cells can be reprogrammed to pluripotency by the forced expression of Oct4, Sox2, Klf4 and c-Myc. However, it remains unknown how this leads to the multitude of epigenetic changes observed during the reprogramming process. Interestingly, Oct4 is the only factor that cannot be replaced by other members of the same family to induce pluripotency. To understand the unique role of Oct4 in reprogramming, we determined the structure of its POU domain bound to DNA. We show that the linker between the two DNA-binding domains is structured as an α-helix and exposed to the protein's surface, in contrast to the unstructured linker of Oct1. Point mutations in this α-helix alter or abolish the reprogramming activity of Oct4, but do not affect its other fundamental properties. On the basis of mass spectrometry studies of the interactome of wild-type and mutant Oct4, we propose that the linker functions as a protein-protein interaction interface and plays a crucial role during reprogramming by recruiting key epigenetic players to Oct4 target genes. Thus, we provide molecular insights to explain how Oct4 contributes to the reprogramming process.

摘要

终末分化细胞可通过强制表达 Oct4、Sox2、Klf4 和 c-Myc 重编程为多能性。然而,目前尚不清楚这如何导致在重编程过程中观察到的众多表观遗传变化。有趣的是,Oct4 是唯一不能被同一家族的其他成员取代以诱导多能性的因子。为了了解 Oct4 在重编程中的独特作用,我们确定了其与 DNA 结合的 POU 结构域的结构。我们表明,两个 DNA 结合结构域之间的连接子被构造成一个α-螺旋,并暴露在蛋白质表面,与 Oct1 的无规卷曲连接子相反。该α-螺旋中的点突变会改变或消除 Oct4 的重编程活性,但不会影响其其他基本特性。基于对野生型和突变型 Oct4 相互作用组的质谱研究,我们提出该连接子作为一个蛋白质-蛋白质相互作用界面,通过招募关键的表观遗传因子到 Oct4 靶基因,在重编程过程中发挥关键作用。因此,我们提供了分子见解,以解释 Oct4 如何有助于重编程过程。

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