Whole-genome sequencing for analysis of an outbreak of meticillin-resistant Staphylococcus aureus: a descriptive study

Harris, Simon R.; Cartwright, Edward; Török, M. Estée; Holden, Matthew T. G.; Brown, Nicholas M.; Ogilvy-Stuart, Amanda; Ellington, Matthew J.; Quail, Michael A.; Bentley, Stephen D.; Parkhill, Julian; Peacock, Sharon J.

doi:10.1016/s1473-3099(12)70268-2

Cited by 517 publications

(485 citation statements)

References 15 publications

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“…A popular method has been to construct phylogenies on the basis of SNPs (single-nucleotide differences among samples) that have been identified either by the mapping of short-read sequence data to a reference genome, or by aligning de novo-assembled sequences to a reference genome 37,40 . This approach has been used successfully to investigate the epidemiology and evolution of a number of single-clone pathogens or members of the same lineage [41][42][43][44][45][46][47][48][49][50][51][52] , but it is limited by its requirement for a reference sequence or whole-genome alignment 40 . The analysis of diverse or highly recombining organisms in this way will prove challenging because the number of total polymorphisms increases as the number of polymorphisms conforming to a clonal model of descent decreases (BOX 1).…”

Section: Post-wgs Cataloguing Of Diversitymentioning

confidence: 99%

“…This, in turn, depends on the particular question being addressed, as some questions require more discrimination among specimens than others. To use the clinical setting as an example: very high resolution is necessary for the detection of outbreaks and the investigation of within-patient variation 43 ; lower resolution is required to determine the membership of a particular clonal complex or lineage 61 ; and even lower resolution is sufficient for determining the species causing an infection 37,62,63 . The gene-bygene approach is inherently hierarchical and scalable, as fewer genes can be used for lowerresolution typing, whereas higher levels of resolution can be attained by increasing the number of genes included in the analysis.…”

Section: Post-wgs Cataloguing Of Diversitymentioning

confidence: 99%

“…Consequently, staphylococci have been subjected to many molecular epidemiology studies 80 , including WGS analyses [41][42][43][44][45][46]82 . Many areas of the biology and pathology of these organisms have been investigated, including their evolution (particularly the origins of MRSA) in hospitals and communities 83,84 , the spread of clones among animals and humans 85 , the dynamics of colonization and infection 86 , and outbreak detection and control 87 .…”

Section: Applying Gene-by-gene Analysismentioning

confidence: 99%

“…The detection and control of S. aureus outbreaks remains a high priority in health care systems [41][42][43] . The gene-by-gene approach described above can rapidly establish very highresolution relationships among isolates, as demonstrated by an analysis of isolate data from a study that described an MRSA outbreak in a special-care baby unit 43 .…”

Section: Applying Gene-by-gene Analysismentioning

confidence: 99%

“…Furthermore, an allele-based rMLST analysis of 669 S. aureus isolates identified 229 unique rSTs based on 51 rps loci (two para logous loci, rpsN and rpmG, were excluded for the purposes of this analysis) and resolved the isolates into lineages that corresponded to previously described clonal complexes 83,90 , also indicating genealogical relationships among the clonal complexes (FIG. 3b).The detection and control of S. aureus outbreaks remains a high priority in health care systems [41][42][43] . The gene-by-gene approach described above can rapidly establish very highresolution relationships among isolates, as demonstrated by an analysis of isolate data from a study that described an MRSA outbreak in a special-care baby unit 43 .…”

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MLST revisited: the gene-by-gene approach to bacterial genomics

et al. 2013

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Multilocus sequence typing (MLST) was proposed in 1998 as a portable sequence-based method for identifying clonal relationships among bacteria. Today, in the whole-genome era of microbiology, the need for systematic, standardized descriptions of bacterial genotypic variation remains a priority. Here, to meet this need, we draw on the successes of MLST and 16S rRNA gene sequencing to propose a hierarchical gene-by-gene approach that reflects functional and evolutionary relationships and catalogues bacteria 'from domain to strain'. Our gene-based typing approach using online platforms such as the Bacterial Isolate Genome Sequence Database (BIGSdb) allows the scalable organization and analysis of whole-genome sequence data.Advances in nucleotide-sequencing technology have provided unparalleled access to the enormous genetic diversity that has accumulated in the bacterial domain during 3.5-4 billion years of evolution 1 . Numerous sets of whole-genome sequencing (WGS) data for bacterial isolates (BOX 1) are available 2 , and metagenomic studies using these technologies continue to reveal further, seemingly boundless, diversity in bacterial communities 3 . Faced with this plethora of information, microbiologists must develop structured means of describing this diversity and of linking phenotype and genotype, thereby facilitating an improved understanding of the microbiological world. Given that we have precise information on the function of only a very small proportion of bacterial genes, and no knowledge at all about most, this is a formidable, if extremely exciting, challenge.Here, we focus primarily on pathogenic bacteria, although the concepts discussed are applicable more widely to all bacteria and archaea. Bacterial pathogens played a crucial part in the development of experimental microbiology and remain the most intensively studied prokaryotes more than 100 years later 4 . Pathogens have emerged across the diversity of the bacterial -but, interestingly, not the archaeal -domain on many occasions and are both polyphyletic and highly diverse. Thus, although pathogens represent only a tiny subset of the bacterial world, the challenges faced by the clinical microbiology laboratory are representative of those faced by microbiology as a whole.Taxonomic and functional analyses are based on the observations that diversity among bacteria is not continuous and that distinct, stable types with particular properties exist 5 . These founding principles of microbiology 6 have been upheld by much subsequent research, but the study of such clusters remains largely descriptive, and the evolutionary mechanisms that led to cluster emergence and persistence remain incompletely understood 7,8 . Structuring is also evident within bacterial genomes, as diversity is unevenly distributed among genes Pre-WGS cataloguing of diversityA major advance in defining bacterial diversity was the proposal, by the late Carl Woese and colleagues, of a universal and 'natural' -that is, genealogical -classification system based on small-su...

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Section: Post-wgs Cataloguing Of Diversitymentioning

confidence: 99%

Section: Post-wgs Cataloguing Of Diversitymentioning

confidence: 99%

Section: Applying Gene-by-gene Analysismentioning

confidence: 99%

Section: Applying Gene-by-gene Analysismentioning

confidence: 99%

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MLST revisited: the gene-by-gene approach to bacterial genomics

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Rapid Bacterial Whole-Genome Sequencing to Enhance Diagnostic and Public Health Microbiology

Ellington²,

et al. 2013

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IMPORTANCE The latest generation of benchtop DNA sequencing platforms can provide an accurate whole-genome sequence (WGS) for a broad range of bacteria in less than a day. These could be used to more effectively contain the spread of multidrug-resistant pathogens. OBJECTIVE To compare WGS with standard clinical microbiology practice for the investigation of nosocomial outbreaks caused by multidrug-resistant bacteria, the identification of genetic determinants of antimicrobial resistance, and typing of other clinically important pathogens. DESIGN, SETTING, AND PARTICIPANTS A laboratory-based study of hospital inpatients with a range of bacterial infections at Cambridge University Hospitals NHS Foundation Trust, a secondary and tertiary referral center in England, comparing WGS with standard diagnostic microbiology using stored bacterial isolates and clinical information. MAIN OUTCOMES AND MEASURES Specimens were taken and processed as part of routine clinical care, and cultured isolates stored and referred for additional reference laboratory testing as necessary. Isolates underwent DNA extraction and library preparation prior to sequencing on the Illumina MiSeq platform. Bioinformatic analyses were performed by persons blinded to the clinical, epidemiologic, and antimicrobial susceptibility data. RESULTS We investigated 2 putative nosocomial outbreaks, one caused by vancomycin-resistant Enterococcus faecium and the other by carbapenem-resistant Enterobacter cloacae; WGS accurately discriminated between outbreak and nonoutbreak isolates and was superior to conventional typing methods. We compared WGS with standard methods for the identification of the mechanism of carbapenem resistance in a range of gram-negative bacteria (Acinetobacter baumannii, E cloacae, Escherichia coli, and Klebsiella pneumoniae). This demonstrated concordance between phenotypic and genotypic results, and the ability to determine whether resistance was attributable to the presence of carbapenemases or other resistance mechanisms. Whole-genome sequencing was used to recapitulate reference laboratory typing of clinical isolates of Neisseria meningitidis and to provide extended phylogenetic analyses of these. CONCLUSIONS AND RELEVANCE The speed, accuracy, and depth of information provided by WGS platforms to confirm or refute outbreaks in hospitals and the community, and to accurately define transmission of multidrug-resistant and other organisms, represents an important advance.

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Contamination of Hospital Plumbing

Snitkin

2019

JAMA Netw Open

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In recent years there have been an increasing number of reports of contamination of hospital plumbing with multidrug-resistant gram-negative organisms, with speculation that this contamination poses a significant risk to patients. 1 Hopman and colleagues 2 add to this body of literature with the report of a patient with a carbapenemase-producing Pseudomonas aeruginosa (CP-PA) infection that was shown to be genetically related to a strain of P aeruginosa from the shower in the patient's room. The patient was a man in his early 60s who had undergone a left-sided pneumonectomy and adjuvant radiotherapy. Subsequent to the procedure, this patient developed a wound infection with a Verona integron-mediated metallo-β-lactamase (VIM)-carrying strain of P aeruginosa. A series of surveillance cultures with negative results for P aeruginosa prior to the patient's infection indicated that his infection was acquired in the hospital. Surveillance culturing of all other patients on the same unit as the case patient failed to uncover any additional patients with positive results for P aeruginosa who might have been the source of his infection. The lack of colonized patients ultimately motivated environmental surveillance to identify potential reservoirs of P aeruginosa in the hospital. Environmental screening revealed CP-PA contamination in the shower drain in the case patient's room, as well as in showers and sinks in adjacent rooms that were connected to a common sewage collection point. The application of whole-genome sequencing (WGS) to patient and environmental isolates supported a single introduction into the hospital seeding both the patient's infection and the contamination of the plumbing. To evaluate the plausibility of airborne transmission from the contaminated shower drain to the patient, the authors evaluated air samples for CP-PA after running the shower for 10 minutes and 15 minutes after the shower had been turned off and found 1 positive result out of several dozen cultures. The hospital ultimately implemented enhanced disinfection of drains, which appeared to eliminate CP-PA from the plumbing. However, on returning to standard disinfection protocols, CP-PA regrowth was observed, which is consistent with findings from other studies that have reported challenges in achieving sustained decontamination of plumbing. 3 A major strength of this work was its use of WGS to demonstrate that environmental contamination across the ward was likely mediated by introduction of P aeruginosa into a single drain. This result highlights how contamination of sink and shower drains can propagate to proximate rooms via plumbing, and illuminates an epidemiologic signature that may be associated with plumbing-mediated outbreaks. However, this study also highlights the challenges in ascertaining the risk that contaminated plumbing poses to patients. In particular, even with a convincing link between the patient and environment provided by WGS, the directionality of the transmission is not evident from the data and analyses provided. A...

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Whole-genome sequencing for analysis of an outbreak of meticillin-resistant Staphylococcus aureus: a descriptive study

Cited by 517 publications

References 15 publications

MLST revisited: the gene-by-gene approach to bacterial genomics

MLST revisited: the gene-by-gene approach to bacterial genomics

Rapid Bacterial Whole-Genome Sequencing to Enhance Diagnostic and Public Health Microbiology

Contamination of Hospital Plumbing

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