Darya Chetverina, Nadezhda E Vorobyeva, Marina Yu Mazina, Lika V Fab, Dmitry Lomaev, Alexandra Golovnina, Vladic Mogila, Pavel Georgiev, Rustam H Ziganshin, Maksim Erokhin
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At the same time, it was demonstrated that the PRE DNA-binding proteins are not exclusively localized to PREs but can bind other DNA regulatory elements, including enhancers, promoters, and boundaries. To gain an insight into the PRE DNA-binding protein regulatory network, here, using ChIP-seq and immuno-affinity purification coupled to the high-throughput mass spectrometry, we searched for differences in abundance of the Combgap, Zeste, Psq, and Adf1 PRE DNA-binding proteins. While there were no conspicuous differences in co-localization of these proteins with other functional transcription factors, we show that Combgap and Zeste are more tightly associated with the Polycomb repressive complex 1 (PRC1), while Psq interacts strongly with the TrxG proteins, including the BAP SWI/SNF complex. The Adf1 interactome contained Mediator subunits as the top interactors. In addition, Combgap efficiently interacted with AGO2, NELF, and TFIID. Combgap, Psq, and Adf1 have architectural proteins in their networks. We further investigated the existence of direct interactions between different PRE DNA-binding proteins and demonstrated that Combgap-Adf1, Psq-Dsp1, and Pho-Spps can interact in the yeast two-hybrid assay. 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引用次数: 0
摘要
多聚核糖体蛋白(PcG)和三轴蛋白(TrxG)分别是控制多细胞生物基因沉默和活跃状态的关键表观遗传调控因子。在果蝇中,PcG/TrxG 蛋白通过与称为多聚酶反应元件(PRE)的特定 DNA 序列结合而被招募到染色质中。虽然 PcG/TrxG 蛋白招募的确切机制尚不清楚,但有人认为其重要作用属于序列特异性 DNA 结合因子。同时,研究表明,PRE DNA 结合蛋白并不只定位在 PREs 上,还能结合其他 DNA 调控元件,包括增强子、启动子和边界。为了深入了解 PRE DNA 结合蛋白的调控网络,我们利用 ChIP-seq 和免疫亲和纯化技术,结合高通量质谱分析,寻找 Combgap、Zeste、Psq 和 Adf1 PRE DNA 结合蛋白丰度的差异。虽然这些蛋白与其他功能转录因子的共定位没有明显差异,但我们发现 Combgap 和 Zeste 与多聚核抑制复合体 1(PRC1)的联系更为紧密,而 Psq 与 TrxG 蛋白(包括 BAP SWI/SNF 复合体)的相互作用很强。Adf1 相互作用组中的首要相互作用者是 Mediator 亚基。此外,Combgap 还与 AGO2、NELF 和 TFIID 进行了有效的相互作用。Combgap、Psq和Adf1的网络中都有结构蛋白。我们进一步研究了不同 PRE DNA 结合蛋白之间是否存在直接的相互作用,并在酵母双杂交实验中证明 Combgap-Adf1、Psq-Dsp1 和 Pho-Spps 可以相互作用。总之,我们的数据表明,Combgap、Psq、Zeste 和 Adf1 与涉及不同调控活动的蛋白复合物有关,并表明它们在转录调控中可能发挥多功能作用。
Comparative interactome analysis of the PRE DNA-binding factors: purification of the Combgap-, Zeste-, Psq-, and Adf1-associated proteins.
The Polycomb group (PcG) and Trithorax group (TrxG) proteins are key epigenetic regulators controlling the silenced and active states of genes in multicellular organisms, respectively. In Drosophila, PcG/TrxG proteins are recruited to the chromatin via binding to specific DNA sequences termed polycomb response elements (PREs). While precise mechanisms of the PcG/TrxG protein recruitment remain unknown, the important role is suggested to belong to sequence-specific DNA-binding factors. At the same time, it was demonstrated that the PRE DNA-binding proteins are not exclusively localized to PREs but can bind other DNA regulatory elements, including enhancers, promoters, and boundaries. To gain an insight into the PRE DNA-binding protein regulatory network, here, using ChIP-seq and immuno-affinity purification coupled to the high-throughput mass spectrometry, we searched for differences in abundance of the Combgap, Zeste, Psq, and Adf1 PRE DNA-binding proteins. While there were no conspicuous differences in co-localization of these proteins with other functional transcription factors, we show that Combgap and Zeste are more tightly associated with the Polycomb repressive complex 1 (PRC1), while Psq interacts strongly with the TrxG proteins, including the BAP SWI/SNF complex. The Adf1 interactome contained Mediator subunits as the top interactors. In addition, Combgap efficiently interacted with AGO2, NELF, and TFIID. Combgap, Psq, and Adf1 have architectural proteins in their networks. We further investigated the existence of direct interactions between different PRE DNA-binding proteins and demonstrated that Combgap-Adf1, Psq-Dsp1, and Pho-Spps can interact in the yeast two-hybrid assay. Overall, our data suggest that Combgap, Psq, Zeste, and Adf1 are associated with the protein complexes implicated in different regulatory activities and indicate their potential multifunctional role in the regulation of transcription.
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