H4K16 acetylation marks active genes and enhancers of embryonic stem cells, but does not alter chromatin compaction

Taylor, Gillian C.A.; Eskeland, Ragnhild; Hekimoglu-Balkan, Betül; Pradeepa, Madapura M.; Bickmore, Wendy A.

doi:10.1101/gr.155028.113

Cited by 162 publications

(158 citation statements)

References 60 publications

(98 reference statements)

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“…3B). Genome-wide distribution of H3K36Me2 and H4K16Ac epigenetic marks has been previously reported (27)(28)(29). The NSD2 (Nuclear receptor SET Domain-containing family of histone lysine methyltransferase) target genes, for example TGFA, MET, and RRAS2, were found to have high H3K36Me2 occupancy (Fig.…”

Section: Zmynd8 Interacts With Modified Histone H31 and H4 Through Imentioning

confidence: 62%

“…We at first investigated the cause of selective enrichment of ZMYND8 at the gene body. H3K36Me2 and H4K16Ac have been shown to be significantly enriched at the gene body by ChIP-Seq studies in different cell lines (27)(28)(29). To understand whether the preferential recruitment of ZMYND8 to the gene body of the ATRA-inducible genes in SH-SY5Y cells is through its modified histone-binding ability, we analyzed the histone PTM on these genes (Fig.…”

Section: Zmynd8 Is Itself An Atra-responsive Gene and Regulatesmentioning

confidence: 99%

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Selective Recognition of H3.1K36 Dimethylation/H4K16 Acetylation Facilitates the Regulation of All-trans-retinoic Acid (ATRA)-responsive Genes by Putative Chromatin Reader ZMYND8

Adhikary

Sanyal

Basu

et al. 2016

Journal of Biological Chemistry

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ZMYND8 (zinc finger MYND (Myeloid, Nervy and DEAF-1)-type containing 8), a newly identified component of the transcriptional coregulator network, was found to interact with the Nucleosome Remodeling and Deacetylase (NuRD) complex. Previous reports have shown that ZMYND8 is instrumental in recruiting the NuRD complex to damaged chromatin for repressing transcription and promoting double strand break repair by homologous recombination. However, the mode of transcription regulation by ZMYND8 has remained elusive. Here, we report that through its specific key residues present in its conserved chromatin-binding modules, ZMYND8 interacts with the selective epigenetic marks H3.1K36Me2/H4K16Ac. Furthermore, ZMYND8 shows a clear preference for canonical histone H3.1 over variant H3.3. Interestingly, ZMYND8 was found to be recruited to several developmental genes, including the all-trans-retinoic acid (ATRA)-responsive ones, through its modified histone-binding ability. Being itself inducible by ATRA, this zinc finger transcription factor is involved in modulating other ATRA-inducible genes. We found that ZMYND8 interacts with transcription initiation-competent RNA polymerase II phosphorylated at Ser-5 in a DNA templatedependent manner and can alter the global gene transcription. Overall, our study identifies that ZMYND8 has CHD4-independent functions in regulating gene expression through its modified histone-binding ability.ZMYND8 (zinc finger MYND (Myeloid, Nervy and DEAF-1)-type containing 8) is a putative chromatin reader/effector harboring a PWWP domain, a bromodomain, and a PHD type zinc finger. It associates with the CHD4 protein of NuRD chromatin remodeling complex implicated in gene transcription, cell cycle progression, and genome integrity (1, 2). Reader proteins specifically recognize histone post-translational modifications (PTMs) 5 and translate such recognition(s) into meaningful biological outcomes by virtue of either their intrinsic activities or those of their interacting partners (3). These readers may interpret histone PTMs via "monovalent" or "multivalent" recognition (4). In monovalent recognition, a chromatin reader recognizes one histone PTM. In contrast, in multivalent recognition, readers recognize multiple histone modifications intra/inter-nucleosomally. An accessible surface is provided by these readers (such as a cavity or surface groove), which accommodates the modified histone residues, and determines the modification (e.g. acetylation versus methylation) or state specificity (such as mono-versus trimethylation of lysine) (3).ZMYND8 is a well known component of the transcription coregulator complex and is associated with several demethylase machinery components, including KDM5A, KDM5C, or LSD1 (5, 6). Through its ability to interact with Xenopus RCoR2, ZMYND8 plays a significant role in embryonic neural differentiation (7). Apart from this, ZMYND8 is also involved in T-cell lymphoma and breast and cervical cancer (8 -10). Another interesting feature is that ZMYND8 is significantly involved...

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Section: Zmynd8 Interacts With Modified Histone H31 and H4 Through Imentioning

confidence: 62%

Section: Zmynd8 Is Itself An Atra-responsive Gene and Regulatesmentioning

confidence: 99%

Selective Recognition of H3.1K36 Dimethylation/H4K16 Acetylation Facilitates the Regulation of All-trans-retinoic Acid (ATRA)-responsive Genes by Putative Chromatin Reader ZMYND8

Adhikary

Sanyal

Basu

et al. 2016

Journal of Biological Chemistry

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“…65 The mechanism regarding the differential expression pattern of H4K16ac-enriched genes in pollen is unclear. It is possible that, like in human HEK293 cells, 37 H4K16ac has distinct effects on transcription in pollen. In the future, it will be important to directly examine the roles of H4K16ac in regulating transcriptional activity in the different stages of the development.…”

Section: Discussionmentioning

confidence: 99%

“…1B), but is enriched at promoters and transcribed regions of active genes in human. 37,38,40 To explore the conservation of H4K16ac and H3K23ac distribution patterns in plants, we determined their genome-wide occupancy in rice by using ChIP-seq.…”

Section: Conserved and Unique Distribution Pattern Of H4k16ac And H3kmentioning

confidence: 99%

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High-resolution mapping of H4K16 and H3K23 acetylation reveals conserved and unique distribution patterns inArabidopsisand rice

et al. 2015

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Developmental Transcriptional Enhancers: A Subtle Interplay between Accessibility and Activity

Bozek

Gompel

2020

BioEssays

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Measurements of open chromatin in specific cell types are widely used to infer the spatiotemporal activity of transcriptional enhancers. How reliable are these predictions? In this review, it is argued that the relationship between the accessibility and activity of an enhancer is insufficiently described by simply considering open versus closed chromatin, or active versus inactive enhancers. Instead, recent studies focusing on the quantitative nature of accessibility signal reveal subtle differences between active enhancers and their different inactive counterparts: the closed silenced state and the accessible primed and repressed states. While the open structure as such is not a specific indicator of enhancer activity, active enhancers display a higher degree of accessibility than the primed and repressed states. Molecular mechanisms that may account for these quantitative differences are discussed. A model that relates molecular events at an enhancer to changes in its activity and accessibility in a developing tissue is also proposed.

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H4K16 acetylation marks active genes and enhancers of embryonic stem cells, but does not alter chromatin compaction

Cited by 162 publications

References 60 publications

Selective Recognition of H3.1K36 Dimethylation/H4K16 Acetylation Facilitates the Regulation of All-trans-retinoic Acid (ATRA)-responsive Genes by Putative Chromatin Reader ZMYND8

Selective Recognition of H3.1K36 Dimethylation/H4K16 Acetylation Facilitates the Regulation of All-trans-retinoic Acid (ATRA)-responsive Genes by Putative Chromatin Reader ZMYND8

High-resolution mapping of H4K16 and H3K23 acetylation reveals conserved and unique distribution patterns inArabidopsisand rice

Developmental Transcriptional Enhancers: A Subtle Interplay between Accessibility and Activity

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