A simple method for generating high-resolution maps of genome-wide protein binding

被引:76
|
作者
Skene, Peter J. [1 ]
Henikoff, Steven [1 ,2 ]
机构
[1] Fred Hutchinson Canc Res Ctr, Seattle, WA 98104 USA
[2] Fred Hutchinson Canc Res Ctr, Howard Hughes Med Inst, Seattle, WA 98104 USA
来源
ELIFE | 2015年 / 4卷
关键词
RNA-POLYMERASE; SUPER-ENHANCERS; NUCLEOSOMES;
D O I
10.7554/eLife.09225
中图分类号
Q [生物科学];
学科分类号
07 ; 0710 ; 09 ;
摘要
Chromatin immunoprecipitation (ChIP) and its derivatives are the main techniques used to determine transcription factor binding sites. However, conventional ChIP with sequencing (ChIP-seq) has problems with poor resolution, and newer techniques require significant experimental alterations and complex bioinformatics. Previously, we have used a new crosslinking ChIP-seq protocol (X-ChIP-seq) to perform high-resolution mapping of RNA Polymerase II (Skene et al., 2014). Here, we build upon this work and compare X-ChIP-seq to existing methodologies. By using micrococcal nuclease, which has both endo-and exo-nuclease activity, to fragment the chromatin and thereby generate precise protein-DNA footprints, high-resolution X-ChIP-seq achieves single base-pair resolution of transcription factor binding. A significant advantage of this protocol is the minimal alteration to the conventional ChIP-seq workflow and simple bioinformatic processing.
引用
收藏
页数:9
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