4.7 Article

Antimicrobial Activity of the Manganese Photoactivated Carbon Monoxide-Releasing Molecule [Mn(CO)3(tpa-κ3N)]+ Against a Pathogenic Escherichia coli that Causes Urinary Infections

Journal

ANTIOXIDANTS & REDOX SIGNALING
Volume 24, Issue 14, Pages 765-780

Publisher

MARY ANN LIEBERT, INC
DOI: 10.1089/ars.2015.6484

Keywords

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Funding

  1. Leverhulme trust [RPG-20130041]
  2. BBSRC [BB/H016805/1]
  3. EPSRC
  4. Biotechnology and Biological Sciences Research Council [BB/H016805/1, BB/M022579/1] Funding Source: researchfish
  5. Engineering and Physical Sciences Research Council [1615044, EP/J004081/2] Funding Source: researchfish
  6. BBSRC [BB/H016805/1, BB/M022579/1] Funding Source: UKRI
  7. EPSRC [EP/J004081/2] Funding Source: UKRI

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Aims: We set out to investigate the antibacterial activity of a new Mn-based photoactivated carbon monoxide-releasing molecule (PhotoCORM, [Mn(CO)(3)(tpa-kappa N-3)](+)) against an antibiotic-resistant uropathogenic strain (EC958) of Escherichia coli. Results: Activated PhotoCORM inhibits growth and decreases viability of E. coli EC958, but non-illuminated carbon monoxide-releasing molecule (CORM) is without effect. NADH-supported respiration rates are significantly decreased by activated PhotoCORM, mimicking the effect of dissolved CO gas. CO from the PhotoCORM binds to intracellular targets, namely respiratory oxidases in strain EC958 and a bacterial globin heterologously expressed in strain K-12. However, unlike previously characterized CORMs, the PhotoCORM is not significantly accumulated in cells, as deduced from the cellular manganese content. Activated PhotoCORM reacts avidly with hydrogen peroxide producing hydroxyl radicals; the observed peroxide-enhanced toxicity of the PhotoCORM is ameliorated by thiourea. The PhotoCORM also potentiates the effect of the antibiotic, doxycycline. Innovation: The present work investigates for the first time the antimicrobial activity of a light-activated PhotoCORM against an antibiotic-resistant pathogen. A comprehensive study of the effects of the PhotoCORM and its derivative molecules upon illumination is performed and mechanisms of toxicity of the activated PhotoCORM are investigated. Conclusion: The PhotoCORM allows a site-specific and time-controlled release of CO in bacterial cultures and has the potential to provide much needed information on the generality of CORM activities in biology. Understanding the mechanism(s) of activated PhotoCORM toxicity will be key in exploring the potential of this and similar compounds as antimicrobial agents, perhaps in combinatorial therapies with other agents.

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