Please use this identifier to cite or link to this item: http://hdl.handle.net/10397/109703
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dc.contributorDepartment of Applied Biology and Chemical Technology-
dc.creatorWan, Y-
dc.creatorChan, EWC-
dc.creatorChen, S-
dc.date.accessioned2024-11-08T06:11:25Z-
dc.date.available2024-11-08T06:11:25Z-
dc.identifier.urihttp://hdl.handle.net/10397/109703-
dc.language.isoenen_US
dc.publisherAmerican Society for Microbiologyen_US
dc.rightsCopyright © 2023 Wan et al. This is an open-access article distributed under the terms of the Creative Commons Attribution 4.0 International license (https://creativecommons.org/licenses/by/4.0/).en_US
dc.rightsThe following publication Wan Y, Wai Chi Chan E, Chen S. 2023. Maintenance and generation of proton motive force are both essential for expression of phenotypic antibiotic tolerance in bacteria. Microbiol Spectr 11:e00832-23 is available at https://doi.org/10.1128/spectrum.00832-23.en_US
dc.subjectActive responseen_US
dc.subjectAntibiotic toleranceen_US
dc.subjectProton motive forceen_US
dc.titleMaintenance and generation of proton motive force are both essential for expression of phenotypic antibiotic tolerance in bacteriaen_US
dc.typeJournal/Magazine Articleen_US
dc.identifier.spagee00832-23-
dc.identifier.volume11-
dc.identifier.issue5-
dc.identifier.doi10.1128/spectrum.00832-23-
dcterms.abstractBacterial antibiotic tolerance, a phenomenon first observed in 1944, is known to be responsible for both onset and exacerbation of recurrent and chronic bacterial infections. The development of antibiotic tolerance was previously thought to be due to a switch to physiological dormancy when bacteria encounter adverse growth conditions. Our recent laboratory findings, however, showed that a set of genes related to the maintenance of proton motive force (PMF) are up-regulated under starvation, indicating that the tolerant sub-population, which are commonly known as persisters, can actively maintain their tolerance phenotypes. In this study, we investigated the relative functional roles of proteins involved in the maintenance and active generation of PMF in mediating tolerance formation in bacteria and found that the PspA and RcsB proteins play a key role in PMF maintenance in persisters, as deletion of genes encoding these two proteins resulted in significantly lower tolerance levels. Consistently, expression of the OsmC and Bdm proteins, which is under regulation by RcsB, is required to maintain PMF and the antibiotic tolerance phenotypes. On the other hand, the NuoL, Ndh, AppC, CyoB, and NuoF proteins, which are electron transport chain (ETC) components, were also found to be actively expressed in persisters in order to generate PMF to support functioning of various tolerance mechanisms such as efflux activities. Our data show that active generation of PMF is even more important than the PMF maintenance functions of PspA and RcsB in the expression of antibiotic tolerance phenotypes in persisters. Assessment of double- and triple-gene knockout strains, in which the PMF maintenance genes and those encoding ETC components were simultaneously deleted, confirms that these two groups of genes are both required for the expression of antibiotic tolerance phenotypes and that a lack of these functions would result in complete PMF dissipation and accumulation of antibiotics in the intracellular compartment of persisters and eventually cell death. Products of these genes are, therefore, ideal targets for future development of anti-tolerance agents.-
dcterms.accessRightsopen accessen_US
dcterms.bibliographicCitationMicrobiology spectrum, Oct. 2023, v. 11, no. 5, e00832-23-
dcterms.isPartOfMicrobiology spectrum-
dcterms.issued2023-10-
dc.identifier.scopus2-s2.0-85175843425-
dc.identifier.pmid37623371-
dc.identifier.eissn2165-0497-
dc.description.validate202411 bcch-
dc.description.oaVersion of Recorden_US
dc.identifier.FolderNumberOA_Scopus/WOSen_US
dc.description.fundingSourceOthersen_US
dc.description.fundingTextShenzhen Key Project of Basic Research; Chengdu Science and Technology Bureau; City University of Hong Kong Chengdu Research Instituteen_US
dc.description.pubStatusPublisheden_US
dc.description.oaCategoryCCen_US
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