| Literature DB >> 28406299 |
Philippe Panchaud1, Thierry Bruyère1, Anne-Catherine Blumstein1, Daniel Bur1, Alain Chambovey1, Eric A Ertel1, Markus Gude1, Christian Hubschwerlen1, Loïc Jacob1, Thierry Kimmerlin1, Thomas Pfeifer1, Lars Prade1, Peter Seiler1, Daniel Ritz1, Georg Rueedi1.
Abstract
Our strategy to combat resistant bacteria consisted of targeting the GyrB/ParE ATP-binding sites located on bacterial DNA gyrase and topoisomerase IV and not utilized by marketed antibiotics. Screening around the minimal ethyl urea binding motif led to the identification of isoquinoline ethyl urea 13 as a promising starting point for fragment evolution. The optimization was guided by structure-based design and focused on antibacterial activity in vitro and in vivo, culminating in the discovery of unprecedented substituents able to interact with conserved residues within the ATP-binding site. A detailed characterization of the lead compound highlighted the potential for treatment of the problematic fluoroquinolone-resistant MRSA, VRE, and S. pneumoniae, and the possibility to offer patients an intravenous-to-oral switch therapy was supported by the identification of a suitable prodrug concept. Eventually, hERG K-channel block was identified as the main limitation of this chemical series, and efforts toward its minimization are reported.Entities:
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Year: 2017 PMID: 28406299 DOI: 10.1021/acs.jmedchem.6b01834
Source DB: PubMed Journal: J Med Chem ISSN: 0022-2623 Impact factor: 7.446