Molecular and functional analysis of pTAV320, a repABC-type replicon of the Paracoccus versutus composite plasmid pTAV1

Bartosik, Dariusz; Baj, Jadwiga; Włodarczyk, Michał

doi:10.1099/00221287-144-11-3149

Cited by 59 publications

(63 citation statements)

References 28 publications

(37 reference statements)

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“…The E. coli-specific mobilizable vector pABW1 (Bartosik et al, 1997) was digested with PstI and ligated with the 2?9 kb entrapment cartridge from pGBG1 (Schneider et al, 2000). The resulting plasmid (pMMB1) was digested with XbaI and KpnI and ligated with a 5?6 kb linear form of the repABC-containing mini-replicon pTAV320 (Bartosik et al, 1998), recovered from shuttle plasmid pABW22A (Table 1). The resulting positive selection vector was designated pMMB2 (Fig.…”

Section: Methodsmentioning

confidence: 99%

“…1; see Methods for details). This plasmid was a fusion of: (i) an E. coli-specific vector, pABW1 (Bartosik et al, 1997); (ii) mini-replicon pTAV320, carrying a repABC-type replicon originating from low-copy-number plasmid pTAV1 (107 kb) of Paracoccus versutus UW1 (Bartosik et al, 1998); and (iii) a cI-tetA selective cartridge (Schneider et al, 2000).…”

Section: Identification Of Tnppa1mentioning

confidence: 99%

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Identification of a transposable genomic island of Paracoccus pantotrophus DSM 11072 by its transposition to a novel entrapment vector pMMB2

et al. 2006

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A novel shuttle entrapment vector, pMMB2, was used to identify a large transposable element, TnPpa1 (44?3 kb), of Paracoccus pantotrophus DSM 11072. TnPpa1 has a composite structure with divergently oriented copies of a cryptic transposon, Tn3434 (Tn3 family), located at both termini. The core region of the element contains a large set of putative genes, whose products show similarity to enzymes involved in central intermediary metabolism (e.g. tricarboxylic acid cycle or 2-methylcitrate cycle), transporters, transcriptional regulators and conserved proteins of unknown function. A 4?2 kb DNA segment of TnPpa1 is homologous to a region of chromosome cII of Rhodobacter sphaeroides 2.4.1, which exemplifies the mosaic structure of this element. TnPpa1 is bordered by 5 bp long directly repeated sequences and is located within a mega-sized replicon, pWKS5, in the DSM 11072 genome. Spontaneous inversion of the core region of TnPpa1 was detected in the host genome. Analysis of the distribution of TnPpa1 in three other strains of P. pantotrophus revealed that this element was present exclusively within DSM 11072, which suggests its relatively recent acquisition by lateral transfer. The identification of TnPpa1 (which may be considered a transposable genomic island) provides evidence for the transposition and lateral transfer of large DNA segments of chromosomal origin (carrying various housekeeping genes), which may have a great impact on the evolution of bacterial genomes.

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Section: Methodsmentioning

confidence: 99%

Section: Identification Of Tnppa1mentioning

confidence: 99%

Identification of a transposable genomic island of Paracoccus pantotrophus DSM 11072 by its transposition to a novel entrapment vector pMMB2

et al. 2006

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“…Two different-sized replicons were obtained: (i) pMSA5 -containing a 3.5-kb EcoRI restriction fragment of pSinA, and (ii) pMSA10 -containing a 4.5-kb BamHI restriction fragment of pSinA. Sequencing showed that pMSA10 carries: (i) a single replication initiation protein gene (repC) (ORF3) without other components of the typical repABC operon (Bartosik et al, 1998), (ii) a gene potentially involved in recombinational resolution of plasmid multimers (mrs; ORF4) and (iii) two additional genes: phd (ORF5) and pemK (ORF6), which probably create a putative hybrid phd-pemK addiction system. Despite the absence of the repAB genes, pMSA10 was still able to replicate in various representatives of Alphaproteobacteria, including: A. tumefaciens LBA288, Brevundimonas sp.…”

Section: Plasmid Psina Is Responsible For Arsenite Oxidationmentioning

confidence: 99%

Structural and functional genomics of plasmid pSinA of Sinorhizobium sp. M14 encoding genes for the arsenite oxidation and arsenic resistance

Drewniak

Dziewit

Ciezkowska

et al. 2013

Journal of Biotechnology

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Plasmid pSinA of Sinorhizobium sp. M14 (Alphaproteobacteria) is the first described, natural, self-transferable plasmid harboring a complete set of genes for oxidation of arsenite. Removal of this plasmid from cells of the host strain caused the loss of resistance to arsenic and heavy metals (Cd, Co, Zn and Hg) and abolished the ability to grow on minimal salt medium supplemented with sodium arsenite as the sole energy source. Plasmid pSinA was introduced into other representatives of Alphaproteobacteria which resulted in acquisition of new abilities concerning arsenic resistance and oxidation, as well as heavy metals resistance. Microcosm experiments revealed that plasmid pSinA can also be transferred via conjugation into other indigenous bacteria from microbial community of As-contaminated soils, including representatives of Alpha-and Gammaproteobacteria. Analysis of "natural" transconjugants showed that pSinA is functional (expresses arsenite oxidase) and is stably maintained in their cells after approximately 60 generations of growth under nonselective conditions. This work clearly demonstrates that pSinA is a self-transferable, broad-host-range plasmid, which plays an important role in horizontal transfer of arsenic metabolism genes.

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“…The size of particular RepA proteins and their N-terminal DNA binding domain suggest that the segregation systems of most rhizobial repABC replicons are Type Ia and thus are members of the MinD/ParA superfamily [14,23]. RepA and RepB proteins in conjunction with parS, a centromere-like sequence, provide the plasmid segregation machinery, which is required for efficient maintenance of the lowcopy DNA replicons in a dividing population of rhizobial cells [18,20,24]. The third protein-encoding gene of the operon, repC, is essential for plasmid replication ( Figure 1).…”

Section: Rhizobial Plasmid Maintenance Systemsmentioning

confidence: 99%

“…The third protein-encoding gene of the operon, repC, is essential for plasmid replication ( Figure 1). RepC, an initiator protein, functions by binding to the origin of replication oriV located within its own coding sequence, close to or inside of a large A+T region [18,24,25]. The repC gene is the minimal region sufficient for replication when inserted into a non-replicating (e.g.…”

Section: Rhizobial Plasmid Maintenance Systemsmentioning

confidence: 99%

Rhizobial plasmids — replication, structure and biological role

Mazur

Koper

2012

Open Life Sciences

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AbstractSoil bacteria, collectively named rhizobia, can establish mutualistic relationships with legume plants. Rhizobia often have multipartite genome architecture with a chromosome and several extrachromosomal replicons making these bacteria a perfect candidate for plasmid biology studies. Rhizobial plasmids are maintained in the cells using a tightly controlled and uniquely organized replication system. Completion of several rhizobial genome-sequencing projects has changed the view that their genomes are simply composed of the chromosome and cryptic plasmids. The genetic content of plasmids and the presence of some important (or even essential) genes contribute to the capability of environmental adaptation and competitiveness with other bacteria. On the other hand, their mosaic structure results in the plasticity of the genome and demonstrates a complex evolutionary history of plasmids. In this review, a genomic perspective was employed for discussion of several aspects regarding rhizobial plasmids comprising structure, replication, genetic content, and biological role. A special emphasis was placed on current post-genomic knowledge concerning plasmids, which has enriched the view of the entire bacterial genome organization by the discovery of plasmids with a potential chromosome-like role.

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Molecular and functional analysis of pTAV320, a repABC-type replicon of the Paracoccus versutus composite plasmid pTAV1

Cited by 59 publications

References 28 publications

Identification of a transposable genomic island of Paracoccus pantotrophus DSM 11072 by its transposition to a novel entrapment vector pMMB2

Identification of a transposable genomic island of Paracoccus pantotrophus DSM 11072 by its transposition to a novel entrapment vector pMMB2

Structural and functional genomics of plasmid pSinA of Sinorhizobium sp. M14 encoding genes for the arsenite oxidation and arsenic resistance

Rhizobial plasmids — replication, structure and biological role

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