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Behaviors of nucleosomes with mutant histone H4s in euchromatic domains of living human cells.

Authors :
Semeigazin, Adilgazy
Iida, Shiori
Minami, Katsuhiko
Tamura, Sachiko
Ide, Satoru
Higashi, Koichi
Toyoda, Atsushi
Kurokawa, Ken
Maeshima, Kazuhiro
Source :
Histochemistry & Cell Biology. Jul2024, Vol. 162 Issue 1/2, p23-40. 18p.
Publication Year :
2024

Abstract

Since Robert Feulgen first stained DNA in the cell, visualizing genome chromatin has been a central issue in cell biology to uncover how chromatin is organized and behaves in the cell. To approach this issue, we have developed single-molecule imaging of nucleosomes, a basic unit of chromatin, to unveil local nucleosome behavior in living cells. In this study, we investigated behaviors of nucleosomes with various histone H4 mutants in living HeLa cells to address the role of H4 tail acetylation, including H4K16Ac and others, which are generally associated with more transcriptionally active chromatin regions. We ectopically expressed wild-type (wt) or mutated H4s (H4K16 point; H4K5,8,12,16 quadruple; and H4 tail deletion) fused with HaloTag in HeLa cells. Cells that expressed wtH4-Halo, H4K16-Halo mutants, and multiple H4-Halo mutants had euchromatin-concentrated distribution. Consistently, the genomic regions of the wtH4-Halo nucleosomes corresponded to Hi-C contact domains (or topologically associating domains, TADs) with active chromatin marks (A-compartment). Utilizing single-nucleosome imaging, we found that none of the H4 deacetylation or acetylation mimicked H4 mutants altered the overall local nucleosome motion. This finding suggests that H4 mutant nucleosomes embedded in the condensed euchromatic domains with excess endogenous H4 nucleosomes cannot cause an observable change in the local motion. Interestingly, H4 with four lysine-to-arginine mutations displayed a substantial freely diffusing fraction in the nucleoplasm, whereas H4 with a truncated N-terminal tail was incorporated in heterochromatic regions as well as euchromatin. Our study indicates the power of single-nucleosome imaging to understand individual histone/nucleosome behavior reflecting chromatin environments in living cells. [ABSTRACT FROM AUTHOR]

Details

Language :
English
ISSN :
09486143
Volume :
162
Issue :
1/2
Database :
Academic Search Index
Journal :
Histochemistry & Cell Biology
Publication Type :
Academic Journal
Accession number :
178293279
Full Text :
https://doi.org/10.1007/s00418-024-02293-x