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基于可扩展基因组编辑的方法绘制人类细胞中多蛋白复合物图谱。

A Scalable Genome-Editing-Based Approach for Mapping Multiprotein Complexes in Human Cells.

机构信息

Centre Hospitalier Universitaire de Québec Research Center and Faculty of Medicine, Laval University, Quebec City, QC G1V 4G2, Canada; St-Patrick Research Group in Basic Oncology and Laval University Cancer Research Center, Quebec City, QC G1R 3S3, Canada.

Centre Hospitalier Universitaire de Québec Research Center and Faculty of Medicine, Laval University, Quebec City, QC G1V 4G2, Canada.

出版信息

Cell Rep. 2015 Oct 20;13(3):621-633. doi: 10.1016/j.celrep.2015.09.009. Epub 2015 Oct 8.

Abstract

Conventional affinity purification followed by mass spectrometry (AP-MS) analysis is a broadly applicable method used to decipher molecular interaction networks and infer protein function. However, it is sensitive to perturbations induced by ectopically overexpressed target proteins and does not reflect multilevel physiological regulation in response to diverse stimuli. Here, we developed an interface between genome editing and proteomics to isolate native protein complexes produced from their natural genomic contexts. We used CRISPR/Cas9 and TAL effector nucleases (TALENs) to tag endogenous genes and purified several DNA repair and chromatin-modifying holoenzymes to near homogeneity. We uncovered subunits and interactions among well-characterized complexes and report the isolation of MCM8/9, highlighting the efficiency and robustness of the approach. These methods improve and simplify both small- and large-scale explorations of protein interactions as well as the study of biochemical activities and structure-function relationships.

摘要

常规的亲和纯化结合质谱(AP-MS)分析是一种广泛应用的方法,用于破译分子相互作用网络并推断蛋白质功能。然而,它对外源过表达的靶蛋白引起的扰动很敏感,并且不能反映对各种刺激的多层次生理调节。在这里,我们开发了基因组编辑和蛋白质组学之间的接口,以从其自然基因组环境中分离天然蛋白质复合物。我们使用 CRISPR/Cas9 和 TAL 效应物核酸酶(TALEN)标记内源性基因,并将几种 DNA 修复和染色质修饰全酶纯化至近乎均一。我们揭示了几个已充分研究的复合物中的亚基和相互作用,并报告了 MCM8/9 的分离,突出了该方法的效率和稳健性。这些方法改进并简化了蛋白质相互作用的小规模和大规模探索,以及生化活性和结构-功能关系的研究。

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