2016
DOI: 10.1128/aac.02117-16
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Sorting Out Antibiotics' Mechanisms of Action: a Double Fluorescent Protein Reporter for High-Throughput Screening of Ribosome and DNA Biosynthesis Inhibitors

Abstract: e In order to accelerate drug discovery, a simple, reliable, and cost-effective system for high-throughput identification of a potential antibiotic mechanism of action is required. To facilitate such screening of new antibiotics, we created a double-reporter system for not only antimicrobial activity detection but also simultaneous sorting of potential antimicrobials into those that cause ribosome stalling and those that induce the SOS response due to DNA damage. In this reporter system, the red fluorescent pr… Show more

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Cited by 90 publications
(83 citation statements)
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“…To accelerate the discovery of antibiotics and to early identify the potential antibacterial mechanism of 83 selected strains, a double fluorescent protein reporter system (pDualrep2) [48] was implemented. The E. coil cell transformed by the plasmid pDualrep2 is a sensor for translation inhibitors, which can be monitored by induction of Katushka2S expression, and DNA damaging agents, monitored by induction of RFP expression.…”
Section: Discussionmentioning
confidence: 99%
“…To accelerate the discovery of antibiotics and to early identify the potential antibacterial mechanism of 83 selected strains, a double fluorescent protein reporter system (pDualrep2) [48] was implemented. The E. coil cell transformed by the plasmid pDualrep2 is a sensor for translation inhibitors, which can be monitored by induction of Katushka2S expression, and DNA damaging agents, monitored by induction of RFP expression.…”
Section: Discussionmentioning
confidence: 99%
“…To determine the mode of action of phazolicin we tested its activity in vivo using an E. colibased double-reporter system that allows one to identify antibiotics inducing ribosome stalling or inhibiting DNA replication 19 is an inhibitor of translation (Figure 2A, left panel). In this assay, we observed a difference in the size of PHZ-induced inhibition zones between the E. coli strain with the deleted tolC gene and the wild-type strain (Figure 2A, right panel).…”
Section: Phz Inhibits Bacterial Protein Translation Both In Vivo and mentioning
confidence: 99%
“…BW25113ΔtolC-pDualrep2 was used as previously described 19 . Briefly, 2 µL of solutions of tested compounds were applied onto the agar plate that already contained a lawn of the reporter strain.…”
Section: Testing Of Phz Activity In Vivomentioning
confidence: 99%
“…This promoter is regulated by LexA transcriptional repressor, which is inactivated upon induction of the DNA damage SOS response [19]. The cells transformed by the resulting plasmid pDualrep2 [15] became a sensor for translation inhibitors which might be monitored by induction of Katushka2S expression and DNA damaging agents, such as topoisomerase II inhibitors, monitored by induction of RFP expression. These proteins possess readily distinguishable spectral properties that allow their separate detection via fluorescence scanner.…”
mentioning
confidence: 99%
“…On the right is the situation when LexA is inactivated when DNA is damaged. In this case RFP is upregulated lincomycin, clindamycin, nalidixic acid, levofloxacin, ciprofloxacin, tobramycin, neomycin, etoposide, furagin, microcin B17, spectinomycin, etamycin A, hygromycin B, griseoviridin, tylosin, amicoumacin A, fusidic acid, puromycin, and gentamicin were tested against the created reporter strain [15]. It appeared that induction of RFP reporter is caused by all known topoisomerase inhibitors and in addition DNA precursor biosynthesis inhibitors.…”
mentioning
confidence: 99%