| Literature DB >> 27226597 |
Philipp Knyphausen1, Susanne de Boor1, Nora Kuhlmann1, Lukas Scislowski1, Antje Extra1, Linda Baldus1, Magdalena Schacherl2, Ulrich Baumann2, Ines Neundorf2, Michael Lammers3.
Abstract
Sirtuins are NAD(+)-dependent lysine deacylases, regulating a variety of cellular processes. The nuclear Sirt1, the cytosolic Sirt2, and the mitochondrial Sirt3 are robust deacetylases, whereas the other sirtuins have preferences for longer acyl chains. Most previous studies investigated sirtuin-catalyzed deacylation on peptide substrates only. We used the genetic code expansion concept to produce natively folded, site-specific, and lysine-acetylated Sirt1-3 substrate proteins, namely Ras-related nuclear, p53, PEPCK1, superoxide dismutase, cyclophilin D, and Hsp10, and analyzed the deacetylation reaction. Some acetylated proteins such as Ras-related nuclear, p53, and Hsp10 were robustly deacetylated by Sirt1-3. However, other reported sirtuin substrate proteins such as cyclophilin D, superoxide dismutase, and PEPCK1 were not deacetylated. Using a structural and functional approach, we describe the ability of Sirt1-3 to deacetylate two adjacent acetylated lysine residues. The dynamics of this process have implications for the lifetime of acetyl modifications on di-lysine acetylation sites and thus constitute a new mechanism for the regulation of proteins by acetylation. Our studies support that, besides the primary sequence context, the protein structure is a major determinant of sirtuin substrate specificity.Entities:
Keywords: GTPase; acetylation; p53; sirtuin; synthetic biology
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Year: 2016 PMID: 27226597 PMCID: PMC4938187 DOI: 10.1074/jbc.M116.726307
Source DB: PubMed Journal: J Biol Chem ISSN: 0021-9258 Impact factor: 5.157