A λ Cro-Like Repressor Is Essential for the Induction of Conjugative Transfer of SXT/R391 Elements in Response to DNA Damage

Poulin-Laprade, Dominic; Burrus, Vincent

doi:10.1128/jb.00638-15

Cited by 22 publications

(27 citation statements)

References 79 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…1, blue arrows; Table 1). It also contained a regulatory region (eex, setCD, croS and setR), which can be activated upon DNA damage (Beaber et al, 2002;Garriss et al, 2013;Poulin-Laprade & Burrus, 2015) and a recombination system (bet/exo) responsible for generating hybrid forms . Moreover, sequence analysis of the entry exclusion gene, eex, confirmed that ICESh95 belongs to ICE exclusion group S (99 % nucleotide identity to eexS from ICE SXT MO10 ) (Marrero & Waldor, 2007).…”

Section: Genome Analysis Of the Clinical Strain Shewanella Sp Sh95mentioning

confidence: 99%

Genome analysis of a clinical isolate of Shewanella sp. uncovered an active hybrid integrative and conjugative element carrying an integron platform inserted in a novel genomic locus

et al. 2016

View full text Add to dashboard Cite

Shewanella spp. are currently considered to be emerging pathogens that can code for a bla OXA carbapenemase in their chromosome. Complete genome analysis of the clinical isolate Shewanella sp. Sh95 revealed that this strain is a novel species, which shares a lineage with marine isolates. Characterization of its resistome showed that it codes for genes drfA15, qacH and bla OXA-48. We propose that Shewanella sp. Sh95 acts as reservoir of bla . Moreover, analysis of mobilome showed that it contains a novel integrative and conjugative element (ICE), named ICESh95. Comparative analysis between the close relatives ICESpuPO1 from Shewanella sp. W3-18-1 and ICE SXT MO10 from Vibrio cholerae showed that ICESh95 encompassed two new regions, a type III restriction modification system and a multidrug resistance integron. The integron platform contained a novel arrangement formed by gene cassettes drfA15 and qacH, and a class C-attC group II intron. Furthermore, insertion of ICESh95 occurred at a unique target site, which correlated with the presence of a different xis/ int module. Mobility of ICESh95 was assessed and demonstrated its ability to self-transfer with high efficiency to different species of bacteria. Our results show that ICESh95 is a selftransmissible, mobile element, which can contribute to the dissemination of antimicrobial resistance; this is clearly a threat when natural bacteria from water ecosystems, such as Shewanella, act as vectors in its propagation.

show abstract

Section: Genome Analysis Of the Clinical Strain Shewanella Sp Sh95mentioning

confidence: 99%

Genome analysis of a clinical isolate of Shewanella sp. uncovered an active hybrid integrative and conjugative element carrying an integron platform inserted in a novel genomic locus

et al. 2016

View full text Add to dashboard Cite

show abstract

“…Moreover, G+C content was 44.8, 47.2, and 46.9% for ICE Mfu Ind1a, ICE Mfu Ind1b, and ICE Mpr Chn1, respectively. Most of the core genes of SXT/R391 ICEs (Beaber et al, 2002; Wozniak et al, 2009; Spagnoletti et al, 2014; Carraro et al, 2015; Poulin-Laprade and Burrus, 2015; Poulin-Laprade et al, 2015) were found to be preserved and were arranged in the same syntenic order in the three elements (Figure 1A, Supplementary Table 1) and showed 60–99% sequence identity at the level of amino acid to the corresponding proteins encoded by SXT/R391 ICEs (Supplementary Table 2). …”

Section: Resultsmentioning

confidence: 99%

“…All the SXT/R391 ICEs are chromosomal MGEs sharing a conserved integrase that mediates site-specific integration into the 5′ end of prfC or t-RNA-ser in the absence of a prfC site (Hochhut and Waldor, 1999; Hochhut et al, 2001; Burrus and Waldor, 2003; Burrus et al, 2006; Taviani et al, 2012; Carraro and Burrus, 2014; Luo et al, 2016). Members of this ICE family contain 52 conserved core genes, many of which are involved in integration/excision, conjugative transfer and regulation of the ICEs (Beaber et al, 2002; Burrus et al, 2006; Wozniak et al, 2009; Bi et al, 2012; Spagnoletti et al, 2014; Carraro et al, 2015; Poulin-Laprade and Burrus, 2015; Poulin-Laprade et al, 2015). In addition, five hotspots (HS1—5) and five variable (VRI—V) regions have also been identified (Lei et al, 2016), which contain variable genes conferring element-specific properties and providing beneficial phenotypes to their hosts (Osorio et al, 2008; Wozniak et al, 2009; Rodríguez-Blanco et al, 2012; Balado et al, 2013; Poulin-Laprade et al, 2015).…”

Section: Introductionmentioning

confidence: 99%

Characterization of Three Novel SXT/R391 Integrating Conjugative Elements ICEMfuInd1a and ICEMfuInd1b, and ICEMprChn1 Identified in the Genomes of Marinomonas fungiae JCM 18476T and Marinomonas profundimaris Strain D104

Badhai

Das

2016

Front. Microbiol.

View full text Add to dashboard Cite

The genus Marinomonas comprises Gram negative bacteria which are widespread in the marine environment and there is no report on the genomic analysis of SXT/R391 ICEs derived from this group of bacteria. This study describes the genomic features of three new SXT/R391 integrating conjugating elements (ICEs) identified in the genome of Marinomonas fungiae JCM 18476T (ICEMfuInd1a and ICEMfuInd1b) and in Marinomonas profundimaris strain D104 (ICEMprChn1). Structural organizations of the three ICEs were similar to the typical SXT/R391 family of ICEs and showed high degree of conservation in the core genes. Sequence analysis revealed ICEMfuInd1b and ICEMprChn1 were inserted into the genome at 5′-end of an typical host prfC gene, while ICEMfuInd1a was inserted at 5′-end of an atypical hipA-like gene. Despite their coexistence, the ICEMfuInd1a and ICEMfuInd1b were not present in a tandem fashion in the genome of M. fungiae. Phylogenetic analyses revealed the three ICEs either evolved independently or high degrees of recombination events had masked their evolution from a common SXT ancestor. Further, we found that the typical entry exclusion mechanism mediated by the TraG/EeX protein pair was likely defective in preventing the conjugative transfer of a second copy of the same S (SXT) group ICE into the M. fungiae genome due to mutations. Our analysis showed the presence of 16, 25, and 27 variable genes in the hotspots of ICEMfuInd1a, ICEMfuInd1b, and ICEMprChn1, respectively, many of which were not reported earlier for SXT/R391 ICEs. Sequence analysis predicted these hotspot regions were shaped by acquisition of genes through homologous recombination between the SXT and R391 related ICEs or mobile genetic elements present in disparate marine bacteria. Multidrug resistance genes which are hallmark feature of SXT/R391 ICEs were not present in either of the two ICEs from M. fungiae but were present within a transposon cassette in the HS-1 of the ICEMprChn1 from M. profundimaris. Finally, our data provided information on the genetic diversity and predicted functions encoded by variable genes present in the hotspot regions of these new ICEs.

show abstract

“…That switch entails essentially a balance of the counteracting transcription factors CI, CII and Cro [46,47]. Interestingly, other ICEs of the SXT/R391 family carry this typical double negative feedback loop architecture, which may therefore control their (bistable) activation [20,22,32].…”

Section: Discussionmentioning

confidence: 99%

“…In terms of its genetic makeup, ICE clc is very distinct from the well-known SXT/R391 family of ICEs and from ICE St1 /ICE St3 of Streptococcus thermophilus [11,20,21]. These carry analogous genetic regulatory circuitry to the lambda prophage, which is characterized by a typical double-negative feedback control [20–22]. Transcriptomic studies indicated that about half of the ICE clc coding capacity (~50 kb) is higher expressed in stationary phase cultures grown on 3-chlorobenzoate (3-CBA), and organized in at least half a dozen transcriptional units [23].…”

Section: Introductionmentioning

confidence: 99%

A four-step regulatory cascade controls bistable transfer competence development of the integrative and conjugative element ICEclcinPseudomonas

Carraro

Richard

Sulser

et al. 2019

Preprint

View full text Add to dashboard Cite

Genetic bistability controls different phenotypic programs in defined subpopulations of genetically identical bacteria. Conjugative transfer of the integrative and conjugative element ICEclc in Pseudomonas requires development of a transfer competence state in stationary phase, but this state arises only in 3-5% of individual cells. The mechanisms controlling and underlying the bistable switch between non-active and transfer competence cells have long remained enigmatic. Using a variety of genetic tools combined with stochastic modeling, we characterize here the factors and overall network architecture controlling bistable ICEclc activation of transfer competence. Two new key regulators (BisR and BisDC) were uncovered, that link the hierarchical cascade of ICEclc transfer competence activation to in total four regulatory nodes. The final activator complex named BisDC drives a positive feedback on its own transcription, and directly controls the “late” ICE promoters for excision and transfer. Stochastic mathematical modeling conceptually explained the arisal and maintenance of bistability by the feedback loop, and demonstrated its importance to guarantee consistent prolonged downstream output in activated cells. A minimized gene set allowing controllable bistable output in a Pseudomonas putida in absence of the ICEclc largely confirmed model predictions. Phylogenetic analyses further showed that the two new ICEclc regulatory factors are widespread among putative ICEs found in Gamma- and Beta- proteobacteria, highlighting the conceptual importance of our findings for the behaviour of this wide family of conjugative elements.Author summaryIntegrative and conjugative elements (ICEs) are mobile genetic elements present in virtually every bacterial species, which can confer adaptive functions to their host, such as antibiotic resistance or xenometabolic pathways. Integrated ICEs maintain by replication along with the genome of their bacterial host, but in order to transfer, the ICE excises and conjugates into a new recipient cell. Single-cell studies on a unique but widely representative ICE model from Pseudomonas (ICEclc) showed that transfer only occurs from a small dedicated subpopulation of cells that arises during stationary phase conditions. This bistable subpopulation differentiation is highly significant for ICE behaviour and fitness, but how it is regulated has remained largely unknown. The present work unveiled the architecture of the ICEclc transfer competence regulation, and showed its widespread occurrence among ICEs of the same family. Stochastic mathematical modeling explained how bistability is generated and maintained, prolonging the capacity of stationary phase cells to complete all stages of ICE activation.

show abstract

A λ Cro-Like Repressor Is Essential for the Induction of Conjugative Transfer of SXT/R391 Elements in Response to DNA Damage

Cited by 22 publications

References 79 publications

Genome analysis of a clinical isolate of Shewanella sp. uncovered an active hybrid integrative and conjugative element carrying an integron platform inserted in a novel genomic locus

Genome analysis of a clinical isolate of Shewanella sp. uncovered an active hybrid integrative and conjugative element carrying an integron platform inserted in a novel genomic locus

Characterization of Three Novel SXT/R391 Integrating Conjugative Elements ICEMfuInd1a and ICEMfuInd1b, and ICEMprChn1 Identified in the Genomes of Marinomonas fungiae JCM 18476T and Marinomonas profundimaris Strain D104

A four-step regulatory cascade controls bistable transfer competence development of the integrative and conjugative element ICEclcinPseudomonas

Contact Info

Product

Resources

About