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提高 DNA 复制叉相关蛋白的检测水平。

Improved detection of DNA replication fork-associated proteins.

机构信息

Department of Cancer Biology and the Abramson Family Cancer Research Institute, Perelman School of Medicine, University of Pennsylvania, Philadelphia, PA, USA.

Department of Biochemistry, Molecular Biology and Biophysics, University of Minnesota, Minneapolis, MN, USA.

出版信息

Cell Rep. 2024 May 28;43(5):114178. doi: 10.1016/j.celrep.2024.114178. Epub 2024 May 2.

Abstract

Innovative methods to retrieve proteins associated with actively replicating DNA have provided a glimpse into the molecular dynamics of replication fork stalling. We report that a combination of density-based replisome enrichment by isolating proteins on nascent DNA (iPOND2) and label-free quantitative mass spectrometry (iPOND2-DRIPPER) substantially increases both replication factor yields and the dynamic range of protein quantification. Replication protein abundance in retrieved nascent DNA is elevated up to 300-fold over post-replicative controls, and recruitment of replication stress factors upon fork stalling is observed at similar levels. The increased sensitivity of iPOND2-DRIPPER permits direct measurement of ubiquitination events without intervening retrieval of diglycine tryptic fragments of ubiquitin. Using this approach, we find that stalled replisomes stimulate the recruitment of a diverse cohort of DNA repair factors, including those associated with poly-K63-ubiquitination. Finally, we uncover the temporally controlled association of stalled replisomes with nuclear pore complex components and nuclear cytoskeleton networks.

摘要

创新的方法来检索与活跃复制 DNA 相关的蛋白质,使我们能够一窥复制叉停滞的分子动力学。我们报告说,通过在新生 DNA 上分离蛋白质进行基于密度的复制体富集(iPOND2)和无标记定量质谱(iPOND2-DRIPPER)的组合,大大增加了复制因子的产量和蛋白质定量的动态范围。与复制后对照相比,回收的新生 DNA 中复制蛋白的丰度提高了高达 300 倍,并且在叉停滞时观察到复制压力因子的募集水平相似。iPOND2-DRIPPER 的灵敏度提高,使得可以直接测量泛素化事件,而无需对泛素的二甘氨酸肽段进行干预检索。使用这种方法,我们发现停滞的复制体刺激了各种 DNA 修复因子的募集,包括与多 K63-泛素化相关的因子。最后,我们揭示了停滞的复制体与核孔复合体成分和核细胞骨架网络的时间控制关联。

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