| Literature DB >> 31204287 |
Michael Maurer1, Daniela Linder1, Kamila B Franke1, Jasmin Jäger1, Gabrielle Taylor2, Felix Gloge3, Sebastian Gremer1, Laura Le Breton4, Matthias P Mayer4, Eilika Weber-Ban2, Marta Carroni5, Bernd Bukau1, Axel Mogk6.
Abstract
ATP-driven bacterial AAA+ proteases have been recognized as drug targets. They possess an AAA+ protein (e.g., ClpC), which threads substrate proteins into an associated peptidase (e.g., ClpP). ATPase activity and substrate selection of AAA+ proteins are regulated by adapter proteins that bind to regulatory domains, such as the N-terminal domain (NTD). The antibacterial peptide Cyclomarin A (CymA) kills Mycobacterium tuberculosis cells by binding to the NTD of ClpC. How CymA affects ClpC function is unknown. Here, we reveal the mechanism of CymA-induced toxicity. We engineered a CymA-sensitized ClpC chimera and show that CymA activates ATPase and proteolytic activities. CymA mimics adapter binding and enables autonomous protein degradation by ClpC/ClpP with relaxed substrate selectivity. We reconstitute CymA toxicity in E. coli cells expressing engineered ClpC and ClpP, demonstrating that gain of uncontrolled proteolytic activity causes cell death. This validates drug-induced overriding of AAA+ protease activity control as effective antibacterial strategy.Entities:
Keywords: AAA+ protein; ClpP; Hsp100; antibiotic; protease; protein degradation
Year: 2019 PMID: 31204287 DOI: 10.1016/j.chembiol.2019.05.008
Source DB: PubMed Journal: Cell Chem Biol ISSN: 2451-9448 Impact factor: 8.116