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hal.structure.identifierUSC-EA3671 Mycoplasmal and Chlamydial Infections in Humans
dc.contributor.authorRIDEAU, Fabien
hal.structure.identifierUSC-EA3671 Mycoplasmal and Chlamydial Infections in Humans
dc.contributor.authorLE ROY, Chloé
hal.structure.identifierUSC-EA3671 Mycoplasmal and Chlamydial Infections in Humans
dc.contributor.authorDESCAMPS, Elodie
hal.structure.identifierUSC-EA3671 Mycoplasmal and Chlamydial Infections in Humans
dc.contributor.authorRENAUDIN, Hélène
hal.structure.identifierBiologie du fruit et pathologie [BFP]
dc.contributor.authorLARTIGUE-PRAT, Carole
hal.structure.identifierUSC-EA3671 Mycoplasmal and Chlamydial Infections in Humans
hal.structure.identifierInstitut National de la Recherche Agronomique [INRA]
dc.contributor.authorBEBEAR, Cécile
dc.date.issued2017
dc.identifier.issn2161-5063
dc.description.abstractEnMycoplasma hominis is a minimal human pathogen that is responsible for genital and neonatal infections. Despite many attempts, there is no efficient genetic tool to manipulate this bacterium, limiting most investigations of its pathogenicity and its uncommon energy metabolism that relies on arginine. The recent cloning and subsequent engineering of other mycoplasma genomes in yeast opens new possibilities for studies of the genomes of genetically intractable organisms. Here, we report the successful one-step cloning of the M. hominis PG21 genome in yeast using the transformation-associated recombination (TAR) cloning method. At low passages, the M. hominis genome cloned into yeast displayed a conserved size. However, after ~60 generations in selective media, this stability was affected, and large degradation events were detected, raising questions regarding the stability of large heterologous DNA molecules cloned in yeast and the need to minimize host propagation. Taking these results into account, we selected early passage yeast clones and successfully modified the M. hominis PG21 genome using the CRISPR/Cas9 editing tool, available in Saccharomyces cerevisiae. Complete M. hominis PG21 genomes lacking the adhesion-related vaa gene were efficiently obtained.
dc.language.isoen
dc.publisherAmerican Chemical Society
dc.rights.urihttp://creativecommons.org/licenses/by-sa/
dc.subjectbactérie pathogène
dc.subjectmollicute
dc.subjectsanté humaine
dc.subject.enhuman health
dc.subject.enpathogenic bacteria
dc.subject.entransformation-associated recombination (TAR) cloning
dc.subject.enMycoplasma hominis
dc.subject.enCRISPR/Cas9
dc.subject.engenome stability
dc.subject.enVaa
dc.subject.enyeast centromeric plasmid
dc.title.enCloning, stability and modification of Mycoplasma hominis genome in yeast.
dc.typeArticle de revue
dc.identifier.doi10.1021/acssynbio.6b00379
dc.subject.halSciences du Vivant [q-bio]/Médecine humaine et pathologie
bordeaux.journalACS Synthetic Biology
bordeaux.page891-901
bordeaux.volume6
bordeaux.issue5
bordeaux.peerReviewedoui
hal.identifierhal-01605841
hal.version1
hal.popularnon
hal.audienceNon spécifiée
hal.origin.linkhttps://hal.archives-ouvertes.fr//hal-01605841v1
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