Site-specific regulation of histone H1 phosphorylation in pluripotent cell differentiation

Abstract: BackgroundStructural variation among histone H1 variants confers distinct modes of chromatin binding that are important for differential regulation of chromatin condensation, gene expression and other processes. Changes in the expression and genomic distributions of H1 variants during cell differentiation appear to contribute to phenotypic differences between cell types, but few details are known about the roles of individual H1 variants and the significance of their disparate capacities for phosphorylation. I… Show more

“…These data are consistent with a previous report by our lab, in which pS187-H1.4 was identified as a bonafide substrate for the kinase activity of CDK9 [9], and further verifies the pS187-H1.4 signal. Table 2.…”

“…In a more recent study, we showed that the global levels of H1 phosphorylation at H1.5-Ser18 (pS18-H1.5), H1.2/H1.5-Ser173 (pS173-H1.2/5) and pS187-H1.4 are subject to differential regulation and that CDK9 phosphorylated pS187-H1. 4 was associated with maintenance of pluripotency [9]. This provided the first evidence that pS187-H1.4 is may be important for transcriptional activation.…”

“…H1.4 undergoes various post-translational modifications (PTMs), such as K26 methylation [41] which allows binding of HP1 and subsequent heterochromatin function, and Gcn5-mediated H1.4K34Ac [42], which works to activate transcription by facilitating the binding of chromatin remodelers and recruitment of transcription factors. Furthermore, ChIP and qRT-PCR studies from our laboratory in Hela, NT2 and mESC cells have implicated pS187-H1.4 in transcriptional activation, showing enrichment of this modified variant at promoters of active genes [8,9].…”

“…We previously generated a collection of unique, highly specific antisera using synthetic phosphopeptides and recombinant proteins and demonstrated their ability to recognize phosphorylation at single sites [8,9]. These sites are either exclusive to an individual human H1 variant or are shared between only two variants.…”

“…Chromatin immunoprecipitation was performed using protocols described before [9] with minor adjustments. Briefly, cells were cross-linked using final concentration 1% methanol-free paraformaldehyde (Thermo Fisher Scientific) for 8 minutes quenched by 125mM final concentration glycine for 10 minutes.…”

Site-specific phosphorylation of histone H1.4 is associated with transcription activation

“…These data are consistent with a previous report by our lab, in which pS187-H1.4 was identified as a bonafide substrate for the kinase activity of CDK9 [9], and further verifies the pS187-H1.4 signal. Table 2.…”

“…In a more recent study, we showed that the global levels of H1 phosphorylation at H1.5-Ser18 (pS18-H1.5), H1.2/H1.5-Ser173 (pS173-H1.2/5) and pS187-H1.4 are subject to differential regulation and that CDK9 phosphorylated pS187-H1. 4 was associated with maintenance of pluripotency [9]. This provided the first evidence that pS187-H1.4 is may be important for transcriptional activation.…”

“…H1.4 undergoes various post-translational modifications (PTMs), such as K26 methylation [41] which allows binding of HP1 and subsequent heterochromatin function, and Gcn5-mediated H1.4K34Ac [42], which works to activate transcription by facilitating the binding of chromatin remodelers and recruitment of transcription factors. Furthermore, ChIP and qRT-PCR studies from our laboratory in Hela, NT2 and mESC cells have implicated pS187-H1.4 in transcriptional activation, showing enrichment of this modified variant at promoters of active genes [8,9].…”

“…We previously generated a collection of unique, highly specific antisera using synthetic phosphopeptides and recombinant proteins and demonstrated their ability to recognize phosphorylation at single sites [8,9]. These sites are either exclusive to an individual human H1 variant or are shared between only two variants.…”

“…Chromatin immunoprecipitation was performed using protocols described before [9] with minor adjustments. Briefly, cells were cross-linked using final concentration 1% methanol-free paraformaldehyde (Thermo Fisher Scientific) for 8 minutes quenched by 125mM final concentration glycine for 10 minutes.…”

Site-specific phosphorylation of histone H1.4 is associated with transcription activation

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