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Differential regulation of the histone chaperone HIRA during muscle cell differentiation by a phosphorylation switch.

Experimental & molecular medicine (2016-08-16)
Jae-Hyun Yang, Tae-Yang Song, Chanhee Jo, Jinyoung Park, Han-Young Lee, Ilang Song, Suji Hong, Kwan Young Jung, Jaehoon Kim, Jeung-Whan Han, Hong-Duk Youn, Eun-Jung Cho
RÉSUMÉ

Replication-independent incorporation of variant histone H3.3 has a profound impact on chromatin function and numerous cellular processes, including the differentiation of muscle cells. The histone chaperone HIRA and H3.3 have essential roles in MyoD regulation during myoblast differentiation. However, the precise mechanism that determines the onset of H3.3 deposition in response to differentiation signals is unclear. Here we show that HIRA is phosphorylated by Akt kinase, an important signaling modulator in muscle cells. By generating a phosphospecific antibody, we found that a significant amount of HIRA was phosphorylated in myoblasts. The phosphorylation level of HIRA and the occupancy of phosphorylated protein on muscle genes gradually decreased during cellular differentiation. Remarkably, the forced expression of the phosphomimic form of HIRA resulted in reduced H3.3 deposition and suppressed the activation of muscle genes in myotubes. Our data show that HIRA phosphorylation limits the expression of myogenic genes, while the dephosphorylation of HIRA is required for proficient H3.3 deposition and gene activation, demonstrating that the phosphorylation switch is exploited to modulate HIRA/H3.3-mediated muscle gene regulation during myogenesis.

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Anticorps monoclonal ANTI-FLAG® M2 antibody produced in mouse, clone M2, purified immunoglobulin (Purified IgG1 subclass), buffered aqueous solution (10 mM sodium phosphate, 150 mM NaCl, pH 7.4, containing 0.02% sodium azide)
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Anticorps anti-histone H3.3, from rabbit, purified by affinity chromatography
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Anti-Histone H4 Antibody, Upstate®, from rabbit