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A CRISPR-based approach for proteomic analysis of a single genomic locus

机译:基于CRISPR的方法对单个基因组位点进行蛋白质组学分析

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摘要

Any given chromosomal activity (e.g., transcription) is governed predominantly by the local epiproteome. However, defining local epiproteomes has been limited by a lack of effective technologies to isolate discrete sections of chromatin and to identify with precision specific proteins and histone posttranslational modifications (PTMs). We report the use of the Cas9 and guide RNA (gRNA) components of the CRISPR system for gRNA-directed purification of a discrete section of chromatin. Quantitative mass spectrometry provides for unambiguous identification of proteins and histone PTMs specifically associated with the enriched chromatin. This CRISPR-based Chromatin Affinity Purification with Mass Spectrometry (CRISPR-ChAP-MS) approach revealed changes in the local epiproteome of a promoter during activation of transcription. CRISPR-ChAP-MS thus has broad applications for discovering molecular components and dynamic regulation of any in vivo activity at a given chromosomal location.
机译:任何给定的染色体活性(例如转录)主要由局部表观蛋白质组控制。然而,由于缺乏有效的技术来分离染色质的离散部分并精确鉴定特定的蛋白质和组蛋白翻译后修饰(PTM),限制了局部表观蛋白质组学的发展。我们报告了Cas9的使用和CRISPR系统的指导RNA(gRNA)组件用于染色质离散部分的gRNA指导纯化。定量质谱法可明确鉴定与富集染色质相关的蛋白质和组蛋白PTM。这种基于CRISPR的质谱染色质亲和纯化(CRISPR-ChAP-MS)方法揭示了转录激活过程中启动子的局部表观蛋白质组的变化。因此,CRISPR-ChAP-MS在发现分子成分和动态调节给定染色体位置上的任何体内活性方面具有广泛的应用。

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