Rationally designed<i>mariner</i>vectors to allow functional genomic analysis of<i>Actinobacillus pleuropneumoniae</i>and other bacteria by transposon-directed insertion-site sequencing (TraDIS)

Jt, Bossé; Y, Li; Lg, Leanse; Zhou, Lei; Rr, Chaudhuri; Se, Peters; Wang, J; Maglennon, Gareth; Holden, Matthew T. G.; Dj, Maskell; Tucker, Alexander W.; Wren, BW; An, Rycroft; Pr, Langford

doi:10.1101/433086

Cited by 2 publications

(2 citation statements)

References 50 publications

(67 reference statements)

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“…To further remove any residual plasmid from the sequencing library, I-SceI recognition sites were incorporated into pMTL-CW20, which provided a mechanism for removal of plasmid reads at the sequencing library stage. After adapter ligation, an I-SceI restriction is used to cleave the site between the adapter and the library primer binding site on the transposon, making those fragments originating from plasmid DNA unsuitable templates for the subsequent PCR amplification step, as described in a similar strategy ( 27 ). Since there is no I-SceI recognition site in the C. autoethanogenum genome, transposon insertion sites in the genome will be identified as usual.…”

Section: Resultsmentioning

confidence: 99%

Required Gene Set for Autotrophic Growth of Clostridium autoethanogenum

Woods

Humphreys

Tomi-Andrino

et al. 2022

Appl Environ Microbiol

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Section: Resultsmentioning

confidence: 99%

Required Gene Set for Autotrophic Growth of Clostridium autoethanogenum

Woods

Humphreys

Tomi-Andrino

et al. 2022

Appl Environ Microbiol

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“…To further remove any residual plasmid from the sequencing library I-SceI recognition sites were incorporated into pMTL-CW20 which provided a mechanism for removal of plasmid reads at the sequencing library stage. After adapter-ligation an I-SceI restriction is used to cleave the site between the adapter and the library primer binding site on the transposon, making those fragments originating from plasmid DNA unsuitable templates for the subsequent PCR amplification step as described in a similar strategy 26 . In the initial transposon library grown on rich medium, 0.2% of reads mapped to the transposon-delivery plasmid.…”

Section: Control Of Transposition a Fundamental Requirement Of An Effective Transposon-deliverymentioning

confidence: 99%

Application of transposon-insertion sequencing to determine gene essentiality in the acetogen Clostridium autoethanogenum

Woods

Tomi-Andrino

et al. 2021

Preprint

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The majority of the genes present in bacterial genomes remain poorly characterised with up to one third of those that are protein encoding having no definitive function. Transposon insertion sequencing represents a high-throughput technique that can help rectify this deficiency. The technology, however, can only be realistically applied to easily transformable species leaving those with low DNA-transfer rates out of reach. Here we have developed a number of approaches that overcome this barrier in the autotrophic species Clostridium autoethanogenum using a mariner-based transposon system. The inherent instability of such systems in the Escherichia coli conjugation donor due to transposition events was counteracted through the incorporation of a conditionally lethal codA marker on the plasmid backbone. Relatively low frequencies of transformation of the plasmid into C. autoethanogenum were circumvented through the use of a plasmid that is conditional for replication coupled with the routine implementation of an Illumina library preparation protocol that eliminates plasmid-based reads. A transposon library was then used to determine the essential genes needed for growth using carbon monoxide as a sole carbon and energy source.

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Rationally designedmarinervectors to allow functional genomic analysis ofActinobacillus pleuropneumoniaeand other bacteria by transposon-directed insertion-site sequencing (TraDIS)

Cited by 2 publications

References 50 publications

Required Gene Set for Autotrophic Growth of Clostridium autoethanogenum

Required Gene Set for Autotrophic Growth of Clostridium autoethanogenum

Application of transposon-insertion sequencing to determine gene essentiality in the acetogen Clostridium autoethanogenum

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