Plasmids Shaped the Recent Emergence of the Major Nosocomial Pathogen Enterococcus faecium

Willems

et al. 2020

Preprint

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Conditionally essential genes for survival during starvation inEnterococcus faeciumE745

Maat

Willems

et al. 2020

Preprint

“…Recombination events and estimation of sequence clusters using BratNextGen and hierBAPS were performed as previously described (21). PopPUNK (version 2.0.1) was run specifying the flag '--easy-run' with a minimum k-mer size of 13 (flag --min-k) and creating the files required to generate a microreact project (flag --microreact) (27).…”

Section: Population Structure Of Vrefm Isolatesmentioning

confidence: 99%

Mode and dynamics of vanA-type vancomycin-resistance dissemination in Dutch hospitals

Top

Corander

et al. 2020

Preprint

Background: Enterococcus faecium is a commensal of the gastrointestinal tract of animals and humans but also a causative agent of hospital-acquired infections. Resistance against glycopeptides and especially to vancomycin, a first-line antibiotic to treat infections with multidrug-resistant Gram-positive pathogens, has motivated the inclusion of E. faecium in the WHO global priority list. Vancomycin resistance can be conferred by the vanA gene cluster on the transposon Tn1546, which is frequently present in plasmids. The vanA gene cluster can be disseminated clonally but also horizontally either by plasmid dissemination or Tn1546 transposition between different genomic locations. Here, we reconstructed all nested genetic elements (clone, plasmid,transposon) to study how the dissemination of vanA-type vancomycin-resistance occurred in Dutch hospitals (2012-2015). Methods: We performed a retrospective study of the genomic epidemiology of 309 vancomycin-resistant E. faecium (VRE) isolates across 32 Dutch hospitals (2012-2015). Genomic information regarding clonality and Tn1546 characterisation was extracted using hierBAPS sequence clusters (SC) and TETyper, respectively. Plasmids were predicted using gplas in combination with a network approach based on shared k-mer content. This allowed determining all nested genomic elements (clone, plasmid and transposon) involved in the dissemination of the vanA gene cluster. Next, we conducted an "all vs. all" pairwise comparison between isolates sharing a potential epidemiological link to elucidate whether clonal, plasmid or Tn1546 spread accounted for the dissemination of vanA resistance. Results: The 309 VRE isolates belonged to 18 different SCs of which SC13 (n = 102, 33%), SC17 (n = 52,16.8%) and SC18 (n = 42, 13.6%) were predominant. We identified seven different plasmid types bearing the vanA gene cluster, four of which were highly similar (identity ~99%, coverage ~84%) to previously described complete plasmid sequences. We estimated that clonal dissemination contributed most (~45%) to the spread of vancomycin-resistance in Dutch hospitals, followed by Tn1546 mobilisation (~12%) and plasmid dissemination (~6%). Conclusions: The dissemination of the vanA gene cluster in Dutch hospitals between 2012 and 2015 was dominated by clonal spread. However, we also identified outbreak settings with high frequencies of Tn1546 transposition and/or plasmid dissemination in which the spread of resistance was mainly driven by horizontal gene transfer (HGT). This study demonstrates the feasibility of distinguishing between modes of dissemination with short-read data and provides one of the first quantitative assessments to estimate the relative contribution of nested genomic elements in the dissemination of vanA-type vancomycin-resistance cluster.

“…Previous whole genome sequencing (WGS) studies identified a split in the E. faecium population into two lineages, including a hospital-associated clade (clade A) and a communityrelated clade (clade B) (5,6). Later, clade A was subdivided into clade A1 representing the majority of hospital associated isolates and clade A2 for animal-related isolates (7), although two studies which included a larger collection of animal-related isolates suggested that these isolates clustered in polyphyletic groups and not in a distinct clade A (8,9). In a recent study also including 55 isolates from Latin America, phylogenomics suggests that the animal isolates represent multiple lineages that diverged prior to the emergence of the clinical subclades in clade A (10).…”

Section: Introductionmentioning

confidence: 99%

“…Recently, we determined the plasmid content (plasmidome) of 1,644 E. faecium isolates from different sources, countries and years using short-and long-read whole genome sequencing technologies in combination with machine-learning classifiers (9,11). This analysis revealed that the hospital-associated isolates carried a larger number of plasmid sequences compared to isolates from other sources and different configurations of plasmidome populations in the hospital environment.…”

Section: Introductionmentioning

confidence: 99%

Genomic rearrangements uncovered by genome-wide co-evolution analysis of a major nosocomial pathogenEnterococcus faecium

Top

Schürch

et al. 2020

Preprint

Enterococcus faecium is a gut commensal of the gastro-digestive tract, but also known as nosocomial pathogen among hospitalized patients. Population genetics based on whole-genome sequencing has revealed that E. faecium strains from hospitalized patients form a distinct clade, designated as clade A1 and that plasmids are major contributors to the emergence of nosocomial E. faecium. Here we further explored the adaptive evolution of E. faecium using a genome-wide co-evolution study (GWES) to identify co-evolving SNPs. We identified three genomic regions harboring large numbers of SNPs in tight linkage which are not proximal to each other based on the completely assembled chromosome of clade A1 reference hospital isolate AUS0004. Close examination of these regions revealed that they are located at the borders of four different types of large-scale genomic rearrangements, insertion sites of two different genomic islands and an IS30-like transposon. In non-clade A1 isolates, these regions are adjacent to each other and they lack the insertions of the genomic islands and IS30-like transposon. Additionally, among the clade A1 isolates there is one group of pet isolates lacking the genomic rearrangement and insertion of the genomic islands, suggesting a distinct evolutionary trajectory. In silico analysis of the biological functions of the genes encoded in three regions revealed a common link to a stress response. This suggests that these rearrangements may reflect adaptation to the stringent conditions in the hospital environment, such as antibiotics and detergents, to which bacteria are exposed. In conclusion, to our knowledge, this is the first study using GWES to identify genomic rearrangements, suggesting that there is considerable untapped potential to unravel hidden evolutionary signals from population genomic data.