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Automated in situ chromatin profiling efficiently resolves cell types and gene regulatory programs.

Epigenetics & chromatin (2018-12-24)
Derek H Janssens, Steven J Wu, Jay F Sarthy, Michael P Meers, Carrie H Myers, James M Olson, Kami Ahmad, Steven Henikoff
RÉSUMÉ

Our understanding of eukaryotic gene regulation is limited by the complexity of protein-DNA interactions that comprise the chromatin landscape and by inefficient methods for characterizing these interactions. We recently introduced CUT&RUN, an antibody-targeted nuclease cleavage method that profiles DNA-binding proteins, histones and chromatin-modifying proteins in situ with exceptional sensitivity and resolution. Here, we describe an automated CUT&RUN platform and apply it to characterize the chromatin landscapes of human cells. We find that automated CUT&RUN profiles of histone modifications crisply demarcate active and repressed chromatin regions, and we develop a continuous metric to identify cell-type-specific promoter and enhancer activities. We test the ability of automated CUT&RUN to profile frozen tumor samples and find that our method readily distinguishes two pediatric glioma xenografts by their subtype-specific gene expression programs. The easy, cost-effective workflow makes automated CUT&RUN an attractive tool for high-throughput characterization of cell types and patient samples.

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Sigma-Aldrich
Anticorps anti-CTCF, serum, Upstate®
Sigma-Aldrich
Anti-dimethyl-Histone H3 (Lys4) Antibody, Upstate®, from rabbit
Sigma-Aldrich
Anticorps anti-acétyl-histone H3 (Lys27), clone RM172, clone RM172, from rabbit