| Literature DB >> 33488970 |
Marina Bukhtiyarova1, Erica M Cook1, Paula J Hancock1, Alan W Hruza2, Anthony W Shaw1, Gregory C Adam1, Richard J O Barnard1, Philip M McKenna1, M Katharine Holloway1, Ian M Bell1, Steve Carroll1, Ivan Cornella-Taracido3, Christopher D Cox1, Peter S Kutchukian1, David A Powell1, Corey Strickland2, B Wesley Trotter3, Matthew Tudor1, Scott Wolkenberg1, Jing Li1, David M Tellers1.
Abstract
By employing a phenotypic screen, a set of compounds, exemplified by 1, were identified which potentiate the ability of histone deacetylase inhibitor vorinostat to reverse HIV latency. Proteome enrichment followed by quantitative mass spectrometric analysis employing a modified analogue of 1 as affinity bait identified farnesyl transferase (FTase) as the primary interacting protein in cell lysates. This ligand-FTase binding interaction was confirmed via X-ray crystallography and temperature dependent fluorescence studies, despite 1 lacking structural and binding similarity to known FTase inhibitors. Although multiple lines of evidence established the binding interaction, these ligands exhibited minimal inhibitory activity in a cell-free biochemical FTase inhibition assay. Subsequent modification of the biochemical assay by increasing anion concentration demonstrated FTase inhibitory activity in this novel class. We propose 1 binds together with the anion in the active site to inhibit farnesyl transferase. Implications for phenotypic screening deconvolution and HIV reactivation are discussed.Entities:
Year: 2020 PMID: 33488970 PMCID: PMC7812668 DOI: 10.1021/acsmedchemlett.0c00551
Source DB: PubMed Journal: ACS Med Chem Lett ISSN: 1948-5875 Impact factor: 4.345