| Literature DB >> 26700437 |
Yukihiro Itoh1, Keisuke Aihara2, Paolo Mellini1, Toshifumi Tojo1, Yosuke Ota1, Hiroki Tsumoto3, Viswas Raja Solomon4, Peng Zhan1, Miki Suzuki1, Daisuke Ogasawara1, Akira Shigenaga2, Tsubasa Inokuma2, Hidehiko Nakagawa4, Naoki Miyata4, Tamio Mizukami5, Akira Otaka2, Takayoshi Suzuki1,6.
Abstract
Inhibition of lysine-specific demethylase 1 (LSD1), a flavin-dependent histone demethylase, has recently emerged as a new strategy for treating cancer and other diseases. LSD1 interacts physically with SNAIL1, a member of the SNAIL/SCRATCH family of transcription factors. This study describes the discovery of SNAIL1 peptide-based inactivators of LSD1. We designed and prepared SNAIL1 peptides bearing a propargyl amine, hydrazine, or phenylcyclopropane moiety. Among them, peptide 3, bearing hydrazine, displayed the most potent LSD1-inhibitory activity in enzyme assays. Kinetic study and mass spectrometric analysis indicated that peptide 3 is a mechanism-based LSD1 inhibitor. Furthermore, peptides 37 and 38, which consist of cell-membrane-permeable oligoarginine conjugated with peptide 3, induced a dose-dependent increase of dimethylated Lys4 of histone H3 in HeLa cells, suggesting that they are likely to exhibit LSD1-inhibitory activity intracellularly. In addition, peptide 37 decreased the viability of HeLa cells. We believe this new approach for targeting LSD1 provides a basis for development of potent selective inhibitors and biological probes for LSD1.Entities:
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Year: 2016 PMID: 26700437 DOI: 10.1021/acs.jmedchem.5b01323
Source DB: PubMed Journal: J Med Chem ISSN: 0022-2623 Impact factor: 7.446