| Literature DB >> 32447347 |
Cong Lin1, Hongxin Li1, Jiwei Liu2, Qianying Hu1, Shuai Zhang2, Na Zhang2, Lingxia Liu1, Yingjie Dai1, Donghui Cao3, Xiaoxue Li1, Baiqu Huang2, Jun Lu4, Yu Zhang5.
Abstract
Senescence is accompanied with histones level alteration; however, the roles and the mechanisms of histone reduction in cellular senescence are largely unknown. Protein arginine methyltransferase 1 (PRMT1) is the major enzyme that generates monomethyl and asymmetrical dimethyl arginine. Here we showed that abrogation of PRMT1-mediated senescence was accompanied with decreasing histone H4 level. Consistently, under multiple classic senescence models, H4 decreasing was also been found prior to the other 3 core histones. Noticeably, asymmetric demethylation of histone H4 at arginine 3 (H4R3me2as), catalyzed by PRMT1, was decreased prior to histone H4. In addition, we showed that the PRMT1-mediated H4R3me2as maintained H4 stability. Reduction of H4R3me2as level increased the interaction between proteasome activator PA200 and histone H4, which catalyzes the poly-ubiquitin-independent degradation of H4. Moreover, H4 degradation promoted nucleosome decomposition, resulting in increased senescence-associated genes transcription. Significantly, H4 was restored by 3 well-informed anti-aging drugs (metformin, rapamycin, and resveratrol) much earlier than other senescence markers detected under H2O2-induced senescence. Thus, we uncovered a novel function of H4R3me2as in modulation of cellular senescence via regulating H4 stability. This finding also points to the value of histone H4 as a senescence indicator and a potential anti-aging drug screening marker.Entities:
Year: 2020 PMID: 32447347 PMCID: PMC7429905 DOI: 10.1038/s41418-020-0562-8
Source DB: PubMed Journal: Cell Death Differ ISSN: 1350-9047 Impact factor: 15.828