Suppression of Staphylococcus aureus biofilm formation and virulence by a benzimidazole derivative, UM-C162

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作者
Cin Kong
Chin-Fei Chee
Katharina Richter
Nicky Thomas
Noorsaadah Abd. Rahman
Sheila Nathan
机构
[1] School of Biosciences and Biotechnology,Department of Chemistry
[2] Faculty of Science and Technology,Department of Biomedical Sciences
[3] Universiti Kebangsaan Malaysia,undefined
[4] Nanotechnology & Catalysis Research Centre,undefined
[5] University of Malaya,undefined
[6] Department of Surgery,undefined
[7] Basil Hetzel Institute for Translational Health Research,undefined
[8] The University of Adelaide,undefined
[9] Adelaide Biofilm Test Facility,undefined
[10] Sansom Institute for Health Research,undefined
[11] University of South Australia,undefined
[12] School of Pharmacy and Medical Sciences,undefined
[13] University of South Australia,undefined
[14] Faculty of Science,undefined
[15] University of Malaya,undefined
[16] Faculty of Science,undefined
[17] University of Nottingham Malaysia Campus,undefined
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摘要
Staphylococcus aureus is a major cause of nosocomial infections and secretes a diverse spectrum of virulence determinants as well as forms biofilm. The emergence of antibiotic-resistant S. aureus highlights the need for alternative forms of therapeutics other than conventional antibiotics. One route to meet this need is screening small molecule derivatives for potential anti-infective activity. Using a previously optimized C. elegans – S. aureus small molecule screen, we identified a benzimidazole derivative, UM-C162, which rescued nematodes from a S. aureus infection. UM-C162 prevented the formation of biofilm in a dose-dependent manner without interfering with bacterial viability. To examine the effect of UM-C162 on the expression of S. aureus virulence genes, a genome-wide transcriptome analysis was performed on UM-C162-treated pathogen. Our data indicated that the genes associated with biofilm formation, particularly those involved in bacterial attachment, were suppressed in UM-C162-treated bacteria. Additionally, a set of genes encoding vital S. aureus virulence factors were also down-regulated in the presence of UM-C162. Further biochemical analysis validated that UM-C162-mediated disruption of S. aureus hemolysins, proteases and clumping factors production. Collectively, our findings propose that UM-C162 is a promising compound that can be further developed as an anti-virulence agent to control S. aureus infections.
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