Open AccessSuppression of Enhancer Overactivation by a RACK7-Histone Demethylase Complex
Author(s) -
Hongjie Shen,
Wenqi Xu,
Rui Guo,
Bowen Rong,
Lei Gu,
Zhentian Wang,
Chenxi He,
Lijuan Zheng,
Xin Hu,
Zhen Hu,
Zhi-Ming Shao,
Pengyuan Yang,
Feizhen Wu,
Yujiang Geno Shi,
Yang Shi,
Fei Lan
Publication year - 2016
Publication title -
cell
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 26.304
H-Index - 776
eISSN - 1097-4172
pISSN - 0092-8674
DOI - 10.1016/j.cell.2016.02.064
Subject(s) - h3k4me3 , enhancer , demethylase , biology , histone , enhancer rnas , chromatin , genetics , regulation of gene expression , transcription factor , microbiology and biotechnology , computational biology , gene expression , gene , promoter
Regulation of enhancer activity is important for controlling gene expression programs. Here, we report that a biochemical complex containing a potential chromatin reader, RACK7, and the histone lysine 4 tri-methyl (H3K4me3)-specific demethylase KDM5C occupies many active enhancers, including almost all super-enhancers. Loss of RACK7 or KDM5C results in overactivation of enhancers, characterized by the deposition of H3K4me3 and H3K27Ac, together with increased transcription of eRNAs and nearby genes. Furthermore, loss of RACK7 or KDM5C leads to de-repression of S100A oncogenes and various cancer-related phenotypes. Our findings reveal a RACK7/KDM5C-regulated, dynamic interchange between histone H3K4me1 and H3K4me3 at active enhancers, representing an additional layer of regulation of enhancer activity. We propose that RACK7/KDM5C functions as an enhancer "brake" to ensure appropriate enhancer activity, which, when compromised, could contribute to tumorigenesis.
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