Genome-wide analysis of salicylate and dibenzofuran metabolism in Sphingomonas wittichii RW1
dc.contributor.author
Coronado, Edith
dc.contributor.author
Roggo, Clémence
dc.contributor.author
Johnson, David R.
dc.contributor.author
van der Meer, Jan Roelof
dc.date.accessioned
2018-11-05T15:12:11Z
dc.date.available
2017-06-10T12:03:32Z
dc.date.available
2018-11-05T15:12:11Z
dc.date.issued
2012-08
dc.identifier.issn
1664-302X
dc.identifier.other
10.3389/fmicb.2012.00300
en_US
dc.identifier.uri
http://hdl.handle.net/20.500.11850/60323
dc.identifier.doi
10.3929/ethz-b-000060323
dc.description.abstract
Sphingomonas wittichii RW1 is a bacterium isolated for its ability to degrade the xenobiotic compounds dibenzodioxin and dibenzofuran (DBF). A number of genes involved in DBF degradation have been previously characterized, such as the dxn cluster, dbfB, and the electron transfer components fdx1, fdx3, and redA2. Here we use a combination of whole genome transcriptome analysis and transposon library screening to characterize RW1 catabolic and other genes implicated in the reaction to or degradation of DBF. To detect differentially expressed genes upon exposure to DBF, we applied three different growth exposure experiments, using either short DBF exposures to actively growing cells or growing them with DBF as sole carbon and energy source. Genome-wide gene expression was examined using a custom-made microarray. In addition, proportional abundance determination of transposon insertions in RW1 libraries grown on salicylate or DBF by ultra-high throughput sequencing was used to infer genes whose interruption caused a fitness loss for growth on DBF. Expression patterns showed that batch and chemostat growth conditions, and short or long exposure of cells to DBF produced very different responses. Numerous other uncharacterized catabolic gene clusters putatively involved in aromatic compound metabolism increased expression in response to DBF. In addition, only very few transposon insertions completely abolished growth on DBF. Some of those (e.g., in dxnA1) were expected, whereas others (in a gene cluster for phenylacetate degradation) were not. Both transcriptomic data and transposon screening suggest operation of multiple redundant and parallel aromatic pathways, depending on DBF exposure. In addition, increased expression of other non-catabolic genes suggests that during initial exposure, S. wittichii RW1 perceives DBF as a stressor, whereas after longer exposure, the compound is recognized as a carbon source and metabolized using several pathways in parallel.
en_US
dc.format
application/pdf
en_US
dc.language.iso
en
en_US
dc.publisher
Frontiers Research Foundation
en_US
dc.rights.uri
http://creativecommons.org/licenses/by/3.0/
dc.subject
Polycyclic aromatic hydrocarbons
en_US
dc.subject
Bioremediation
en_US
dc.subject
Transposon screening
en_US
dc.subject
Microarray analysis
en_US
dc.title
Genome-wide analysis of salicylate and dibenzofuran metabolism in Sphingomonas wittichii RW1
en_US
dc.type
Journal Article
dc.rights.license
Creative Commons Attribution 3.0 Unported
ethz.journal.title
Frontiers in Microbiology
ethz.journal.volume
3
en_US
ethz.journal.abbreviated
Front Microbiol
ethz.pages.start
300
en_US
ethz.size
13 p.
en_US
ethz.version.deposit
publishedVersion
en_US
ethz.publication.place
Lausanne
en_US
ethz.publication.status
published
en_US
ethz.leitzahl
ETH Zürich::00002 - ETH Zürich::00012 - Lehre und Forschung::00007 - Departemente::02350 - Dep. Umweltsystemwissenschaften / Dep. of Environmental Systems Science::02721 - Inst. f. Biogeochemie u. Schadstoffdyn. / Inst. Biogeochem. and Pollutant Dynamics::03743 - Ackermann, Martin / Ackermann, Martin
en_US
ethz.leitzahl.certified
ETH Zürich::00002 - ETH Zürich::00012 - Lehre und Forschung::00007 - Departemente::02350 - Dep. Umweltsystemwissenschaften / Dep. of Environmental Systems Science::02721 - Inst. f. Biogeochemie u. Schadstoffdyn. / Inst. Biogeochem. and Pollutant Dynamics::03743 - Ackermann, Martin / Ackermann, Martin
ethz.date.deposited
2017-06-10T12:03:52Z
ethz.source
ECIT
ethz.identifier.importid
imp593650206ba2e25317
ethz.ecitpid
pub:96382
ethz.eth
yes
en_US
ethz.availability
Open access
en_US
ethz.rosetta.installDate
2017-07-14T23:20:25Z
ethz.rosetta.lastUpdated
2022-03-28T21:35:11Z
ethz.rosetta.versionExported
true
ethz.COinS
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