Reduction of ZFX levels decreases histone H4 acetylation and increases Pol2 pausing at target promoters

Author:

Hsu Emily1,Hutchison Katherine1,Liu Yao1,Nicolet Charles M1,Schreiner Shannon1ORCID,Zemke Nathan R2,Farnham Peggy J1ORCID

Affiliation:

1. Department of Biochemistry and Molecular Medicine and the Norris Comprehensive Cancer Center, Keck School of Medicine, University of Southern California , Los Angeles , CA 90089 , USA

2. Department of Cellular and Molecular Medicine, UCSD School of Medicine , La Jolla , CA 92093 , USA

Abstract

Abstract The ZFX transcriptional activator binds to CpG island promoters, with a major peak at ∼200–250 bp downstream from transcription start sites. Because ZFX binds within the transcribed region, we investigated whether it regulates transcriptional elongation. We used GRO-seq to show that loss or reduction of ZFX increased Pol2 pausing at ZFX-regulated promoters. To further investigate the mechanisms by which ZFX regulates transcription, we determined regions of the protein needed for transactivation and for recruitment to the chromatin. Interestingly, although ZFX has 13 grouped zinc fingers, deletion of the first 11 fingers produces a protein that can still bind to chromatin and activate transcription. We next used TurboID-MS to detect ZFX-interacting proteins, identifying ZNF593, as well as proteins that interact with the N-terminal transactivation domain (which included histone modifying proteins), and proteins that interact with ZFX when it is bound to the chromatin (which included TAFs and other histone modifying proteins). Our studies support a model in which ZFX enhances elongation at target promoters by recruiting H4 acetylation complexes and reducing pausing.

Funder

National Institutes of Health

Margaret Kersten Ponty Endowed Postdoctoral Fellowship Award in Oncology Research at the Norris Comprehensive Cancer Center

Publisher

Oxford University Press (OUP)

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