An Oct4-Centered Protein Interaction Network in Embryonic Stem Cells

被引:452
作者
van den Berg, Debbie L. C. [1 ]
Snoek, Tim [1 ]
Mullin, Nick P. [3 ]
Yates, Adam [3 ]
Bezstarosti, Karel [2 ]
Demmers, Jeroen [2 ]
Chambers, Ian [3 ]
Poot, Raymond A. [1 ]
机构
[1] Erasmus MC, Dept Cell Biol, NL-3015 GE Rotterdam, Netherlands
[2] Erasmus MC, Prote Ctr, NL-3015 GE Rotterdam, Netherlands
[3] Univ Edinburgh, Sch Biol Sci, Inst Stem Cell Res, MRC Ctr Regenerat Med, Edinburgh EH9 3JQ, Midlothian, Scotland
基金
英国医学研究理事会; 英国惠康基金;
关键词
REGULATES SELF-RENEWAL; TRANSCRIPTIONAL REGULATION; RECEPTOR-BETA; PLURIPOTENCY; OCT4; NANOG; COMPLEX; MOUSE; SOX2; COACTIVATOR;
D O I
10.1016/j.stem.2010.02.014
中图分类号
Q813 [细胞工程];
学科分类号
摘要
Transcription factors, such as Oct4, are critical for establishing and maintaining pluripotent cell identity. Whereas the genomic locations of several pluripotency transcription factors have been reported, the spectrum of their interaction partners is underexplored. Here, we use an improved affinity protocol to purify Oct4-interacting proteins from mouse embryonic stem cells (ESCs). Subsequent purification of Oct4 partners Sall4, Tcfcp2l1, Dax1, and Esrrb resulted in an Oct4 interactome of 166 proteins, including transcription factors and chromatin-modifying complexes with documented roles in self-renewal, but also many factors not previously associated with the ESC network. We find that Esrrb associated with the basal transcription machinery and also detect interactions between transcription factors and components of the TGF-beta, Notch, and Wnt signaling pathways. Acute depletion of Oct4 reduced binding of Tcfcp2l1, Dax1, and Esrrb to several target genes. In conclusion, our purification protocol allowed us to bring greater definition to the circuitry controlling pluripotent cell identity.
引用
收藏
页码:369 / 381
页数:13
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