Journal ArticleDOI
Engineering multiple genomic deletions in Gram-negative bacteria: analysis of the multi-resistant antibiotic profile of Pseudomonas putida KT2440.
TLDR
The directed edition of the P. putida chromosome shown here not only enhances the amenability of this bacterium to deep genomic engineering, but also validates the corresponding approach for similar handlings of a large variety of Gram-negative microorganisms.Abstract:
Summary
The genome of the soil bacterium Pseudomonas putida strain KT2440 has been erased of various determinants of resistance to antibiotics encoded in its extant chromosome To this end, we employed a coherent genetic platform that allowed the precise deletion of multiple genomic segments in a large variety of Gram-negative bacteria including (but not limited to) P putida The method is based on the obligatory recombination between free-ended homologous DNA sequences that are released as linear fragments generated upon the cleavage of the chromosome with unique I-SceI sites, added to the segment of interest by the vector system Despite the potential for a SOS response brought about by the appearance of double stranded DNA breaks during the process, fluctuation experiments revealed that the procedure did not increase mutation rates – perhaps due to the protection exerted by I-SceI bound to the otherwise naked DNA termini With this tool in hand we made sequential deletions of genes mexC, mexE, ttgA and ampC in the genome of the target bacterium, orthologues of which are known to determine various degrees of antibiotic resistance in diverse microorganisms Inspection of the corresponding phenotypes demonstrated that the efflux pump encoded by ttgA sufficed to endow P putida with a high-level of tolerance to β-lactams, chloramphenicol and quinolones, but had little effect on, eg aminoglycosides Analysis of the mutants revealed also a considerable diversity in the manifestation of the resistance phenotype within the population and suggested a degree of synergism between different pumps The directed edition of the P putida chromosome shown here not only enhances the amenability of this bacterium to deep genomic engineering, but also validates the corresponding approach for similar handlings of a large variety of Gram-negative microorganismsread more
Citations
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Journal ArticleDOI
Mechanistic Modeling of Genetic Circuits for ArsR Arsenic Regulation.
Yves Berset,Yves Berset,Davide Merulla,Aurélie Joublin,Vassily Hatzimanikatis,Jan Roelof van der Meer +5 more
TL;DR: A comprehensive mechanistic model was empirically tested and validated in E. coli carrying different circuit configurations and predicted a particular useful circuit variant having steeper response at low arsenite concentrations, which was experimentally confirmed and may be useful as arsenic bioreporter in the field.
Journal ArticleDOI
Engineering adipic acid metabolism in Pseudomonas putida.
Yannic S. Ackermann,Wing-Jin Li,Leonie Op de Hipt,Paul-Joachim Niehoff,William Casey,Tino Polen,Sebastian Köbbing,Hendrik Ballerstedt,Benedikt Wynands,Kevin E. O’Connor,Lars M. Blank,Nick Wierckx +11 more
TL;DR: In this article, a reverse-engineered strain of Pseudomonas putida KT2440 was found to grow on adipate with a rate of 0.35 ± 0.01 h−1, reaching a final biomass yield of 0 27 − 0.27 − 1.00 gCDW gadipate−1.
Journal ArticleDOI
Fis overexpression enhances Pseudomonas putida biofilm formation by regulating the ratio of LapA and LapF
TL;DR: The results suggest that the profusion of LapA in the Fis-overexpressed cells causes enhanced biofilm formation in mature stages of P. putidaBiofilm formation.
Journal ArticleDOI
Ongoing evolution of Pseudomonas aeruginosa PAO1 sublines complicates studies of DNA damage repair and tolerance.
TL;DR: The accumulating mutations and discordant phenotypes of the PAO1 derivatives challenge the reproducibility and comparability of the results obtained with different PAO 1 sublines and also limit the usage of the MPAO1 transposon library in DNA damage tolerance and mutagenesis studies.
Journal ArticleDOI
Characterization of aromatic acid/proton symporters in Pseudomonas putida KT2440 toward efficient microbial conversion of lignin-related aromatics.
Ayumu Wada,Erica T. Prates,Ryo Hirano,Allison Z. Werner,Naofumi Kamimura,Daniel Jacobson,Gregg T. Beckham,Eiji Masai +7 more
TL;DR: In this article, the authors focused on five genes encoding aromatic acid/H+ symporter family transporters categorized into major facilitator superfamily that uses the proton motive force.
References
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