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Actin R256 Mono-methylation Is a Conserved Post-translational Modification Involved in Transcription.

Cell reports (2020-10-01)
Ashok Kumar, Yuan Zhong, Amelie Albrecht, Pau Biak Sang, Adrian Maples, Zhenan Liu, Vinesh Vinayachandran, Rohit Reja, Chia-Fang Lee, Ashutosh Kumar, Jiyuan Chen, Jing Xiao, Bongsoo Park, Jianjun Shen, Bin Liu, Maria D Person, Kathleen M Trybus, Kam Y J Zhang, B Franklin Pugh, Kristine E Kamm, Dianna M Milewicz, Xuetong Shen, Prabodh Kapoor
RESUMEN

Nuclear actin has been elusive due to the lack of knowledge about molecular mechanisms. From actin-containing chromatin remodeling complexes, we discovered an arginine mono-methylation mark on an evolutionarily conserved R256 residue of actin (R256me1). Actin R256 mutations in yeast affect nuclear functions and cause diseases in human. Interestingly, we show that an antibody specific for actin R256me1 preferentially stains nuclear actin over cytoplasmic actin in yeast, mouse, and human cells. We also show that actin R256me1 is regulated by protein arginine methyl transferase-5 (PRMT5) in HEK293 cells. A genome-wide survey of actin R256me1 mark provides a landscape for nuclear actin correlated with transcription. Further, gene expression and protein interaction studies uncover extensive correlations between actin R256me1 and active transcription. The discovery of actin R256me1 mark suggests a fundamental mechanism to distinguish nuclear actin from cytoplasmic actin through post-translational modification (PTM) and potentially implicates an actin PTM mark in transcription and human diseases.

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ANTI-FLAG® M2 monoclonal 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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S-(5′-Adenosyl)-L-homocysteine, crystalline
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Anticuerpo anti-actina, clon C4, ascites fluid, clone C4, Chemicon®
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PRMT5/MEP50 Active human, recombinant, expressed in baculovirus infected insect cells, ≥70% (SDS-PAGE)