ATAD2 controls chromatin-bound HIRA turnover

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Wang, Tao | Perazza, Daniel | Boussouar, Fayçal | Cattaneo, Matteo | Bougdour, Alexandre | Chuffart, Florent | Barral, Sophie | Vargas, Alexandra | Liakopoulou, Ariadni | Puthier, Denis | Bargier, Lisa | Morozumi, Yuichi | Jamshidikia, Mahya | Garcia-Saez, Isabel | Petosa, Carlo | Rousseaux, Sophie | Verdel, A | Khochbin, Saadi

Edité par CCSD ; Life Science Alliance LLC -

International audience. Taking advantage of the evolutionary conserved nature of ATAD2, we report here a series of parallel functional studies in human, mouse, and Schizosaccharomyces pombe to investigate ATAD2's conserved functions. In S. pombe, the deletion of ATAD2 ortholog, abo1, leads to a dramatic decrease in cell growth, with the appearance of suppressor clones recovering normal growth. The identification of the corresponding suppressor mutations revealed a strong genetic interaction between Abo1 and the histone chaperone HIRA. In human cancer cell lines and in mouse embryonic stem cells, we observed that the KO of ATAD2 leads to an accumulation of HIRA. A ChIP-seq mapping of nucleosome-bound HIRA and FACT in Atad2 KO mouse ES cells demonstrated that both chaperones are trapped on nucleosomes at the transcription start sites of active genes, resulting in the abnormal presence of a chaperone-bound nucleosome on the TSS-associated nucleosomefree regions. Overall, these data highlight an important layer of regulation of chromatin dynamics ensuring the turnover of histone-bound chaperones.

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