The esBAF and ISWI nucleosome remodeling complexes influence occupancy of overlapping dinucleosomes and fragile nucleosomes in murine embryonic stem cells

David C Klein; Kris Troy; Sarah A Tripplehorn; Sarah J Hainer

doi:10.1186/s12864-023-09287-4

The esBAF and ISWI nucleosome remodeling complexes influence occupancy of overlapping dinucleosomes and fragile nucleosomes in murine embryonic stem cells

BMC Genomics. 2023 Apr 13;24(1):201. doi: 10.1186/s12864-023-09287-4.

Authors

David C Klein¹, Kris Troy^{1

2}, Sarah A Tripplehorn¹, Sarah J Hainer³

Affiliations

¹ Department of Biological Sciences, University of Pittsburgh, Pittsburgh, PA, 15213, USA.
² Department of Quantitative and Systems Biology, University of California, 95343, Merced, Merced, CA, USA.
³ Department of Biological Sciences, University of Pittsburgh, Pittsburgh, PA, 15213, USA. sarah.hainer@pitt.edu.

Abstract

Background: Nucleosome remodeling factors regulate the occupancy and positioning of nucleosomes genome-wide through ATP-driven DNA translocation. While many nucleosomes are consistently well-positioned, some nucleosomes and alternative nucleosome structures are more sensitive to nuclease digestion or are transitory. Fragile nucleosomes are nucleosome structures that are sensitive to nuclease digestion and may be composed of either six or eight histone proteins, making these either hexasomes or octasomes. Overlapping dinucleosomes are composed of two merged nucleosomes, lacking one H2A:H2B dimer, creating a 14-mer wrapped by ~ 250 bp of DNA. In vitro studies of nucleosome remodeling suggest that the collision of adjacent nucleosomes by sliding stimulates formation of overlapping dinucleosomes.

Results: To better understand how nucleosome remodeling factors regulate alternative nucleosome structures, we depleted murine embryonic stem cells of the transcripts encoding remodeler ATPases BRG1 or SNF2H, then performed MNase-seq. We used high- and low-MNase digestion to assess the effects of nucleosome remodeling factors on nuclease-sensitive or "fragile" nucleosome occupancy. In parallel we gel-extracted MNase-digested fragments to enrich for overlapping dinucleosomes. We recapitulate prior identification of fragile nucleosomes and overlapping dinucleosomes near transcription start sites, and identify enrichment of these features around gene-distal DNaseI hypersensitive sites, CTCF binding sites, and pluripotency factor binding sites. We find that BRG1 stimulates occupancy of fragile nucleosomes but restricts occupancy of overlapping dinucleosomes.

Conclusions: Overlapping dinucleosomes and fragile nucleosomes are prevalent within the ES cell genome, occurring at hotspots of gene regulation beyond their characterized existence at promoters. Although neither structure is fully dependent on either nucleosome remodeling factor, both fragile nucleosomes and overlapping dinucleosomes are affected by knockdown of BRG1, suggesting a role for the complex in creating or removing these structures.

Keywords: Chromatin; Fragile nucleosomes; Nucleosomes; Overlapping dinucleosomes; Remodeling; Stem cells; Subnucleosomes.

MeSH terms

Animals
Binding Sites
DNA-Binding Proteins* / genetics
Embryonic Stem Cells / metabolism
Histones / metabolism
Mice
Nucleosomes* / genetics

Substances

Nucleosomes
DNA-Binding Proteins
Histones

Abstract

MeSH terms

Substances

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