Among the underlying mechanisms of bacterial carbapenem resistance, carbapenemases are of significant public health concern. Carbapenemases are frequently encoded on mobile genetic elements (eg, plasmids) that often contain additional resistance determinants, can be transferred between bacterial taxa, 1 and are associated with rapid increases in carbapenem resistance. Reference Kizny Gordon, Mathers and Cheong2–Reference Walters, Witwer and Lee4 In the United States, nearly 35% of carbapenem-resistant Enterobacterales (CRE) harbor a carbapenemase, with Klebsiella pneumoniae carbapenemase (KPC) most commonly identified. 5 Carbapenemases are less commonly the mechanism of carbapenem resistance in Pseudomonas aeruginosa; ∼2% of carbapenem-resistant Pseudomonas aeruginosa (CRPA) harbor a carbapenemase, most frequently the Verona-integron-encoded metallo-β-lactamase (VIM). Reference Walters, Witwer and Lee4,6,Reference Woodworth, Walters and Weiner7 Carbapenemase-producing organisms (CPOs) can cause outbreaks in healthcare facilities resulting in infections with limited treatment options. Reference Kizny Gordon, Mathers and Cheong2,8,Reference Reyes, Komarow and Chen9
Patients most susceptible to acquiring CPOs have complex medical needs. Reference Dumyati, Stone, Nace, Crnich and Jump10,Reference Munoz-Price11 Most patients with CPOs are asymptomatically colonized, presenting challenges for identification and initiation of transmission-based precautions. Reference Woodworth, Walters and Weiner7 CPO transmission may occur via transient hand carriage by healthcare personnel or via contaminated shared medical equipment. Additionally, a growing body of literature describes CPO transmission from healthcare facility wastewater plumbing to patients. Reference Mathers, Vegesana and German Mesner3,Reference Castanheira, Bell, Turnidge, Mathai and Jones12,Reference Rankin, Caicedo, Dotson, Gable and Chu13
On July 5, 2017, the Florida Department of Health (FDOH) was notified of 2 carbapenemase-producing organisms, VIM-producing Pseudomonas aeruginosa and KPC-producing Klebsiella pneumoniae, in specimens from a patient of long-term acute-care hospital-A (LTACH A) on admission to a local acute-care hospital. In response, the FDOH conducted an onsite infection control assessment at LTACH A that identified significant gaps in hand hygiene and transmission-based precautions adherence, raising concern for transmission. In July 2017, a facility-wide point-prevalence survey (PPS) of 36 patients identified 4 patients with KPC-producing CRE and 3 patients with VIM-producing CRPA. Here, we describe epidemiologic and laboratory investigations to control transmission.
Methods
Setting
LTACH A is a freestanding facility with a 6-bed intensive care unit (ICU) and a progressive care unit that expanded from 40 to 50 private rooms in January 2018.
Case definitions and case finding
We defined a case as the detection of bla VIM or bla KPC in a clinical isolate or screening specimen from a patient admitted to LTACH A for ≥1 night between July 13, 2017, and December 18, 2018. An incident case was the first identification of bla VIM or bla KPC; case patients could have 2 incident cases (1 bla VIM and 1 bla KPC). Incident cases were considered to have been acquired in LTACH A if they were identified from a patient without a history of colonization or infection with that carbapenemase and with ≥1 negative screening result at least 1 week before incident specimen collection. Cases considered present on admission had specimens collected within 3 days of admission to LTACH A.
In July 2017, we requested the commercial laboratory of LTACH A to submit carbapenem-resistant organisms identified in clinical specimens to the FDOH Bureau of Public Health Laboratory (BPHL) for carbapenem resistance mechanism testing. In August 2017, we initiated admission and discharge screening and biweekly facility-wide point-prevalence surveys (PPSs) to detect carbapenemase genes. Human subjects advisors in Florida reviewed the investigation activities and determined that they constituted public health response. This research was exempt from human subjects review by the Centers for Disease Control and Prevention (CDC) and was conducted consistent with applicable federal law and CDC policy [45 C.F.R. part 46.102(I)(2)].
Case investigation
We completed medical record reviews for incident cases using a standard abstraction form to collect patient demographics, past medical history, underlying medical conditions, discharge status, presence of indwelling device(s), and antibiotic administration at the time of or in the 14 days before incident specimen collection. We calculated slopes of newly acquired cases and CPO prevalence by fitting a linear regression line in 2-week intervals (based on PPSs) over the outbreak duration using R Studio version 1.2.1335 software (R Foundation for Statistical Computing, Vienna, Austria).
Cohort study
We conducted a retrospective cohort study to assess risk factors associated with bla VIM and/or bla KPC acquisition during the initial months of the outbreak. All patients admitted to LTACH A from July 5 to December 7, 2017, with ≥2 colonization screenings performed were included. Information regarding maintenance of medical devices, hemodialysis procedures, enteral feedings, respiratory therapy, speech, occupational, and physical therapy as well as peripherally inserted central catheter (PICC) insertion and line maintenance were obtained from procedure log books. Medical records were not abstracted for noncases; thus, we were unable to select comorbid conditions as a confounder in our regression models. Mortality data were collected through Florida’s electronic death registry. 14 Univariable analysis was conducted using the Welch unequal variance t test for continuous variables and the Pearson χ Reference Kizny Gordon, Mathers and Cheong2 test for categorical variables. Confounders were identified using prior knowledge. A multivariable logistic regression adjusting for age, sex, length of stay, and ICU admission was conducted to estimate the relative risks (RRs) and 95% confidence intervals (CIs) for acquisition of bla VIM and bla KPC during hospitalization at LTACH A. Statistical tests based on a 2-tailed probability and significance level of α = 5% were conducted using Stata IC version 16.0 software (Statacorp LLC, College Station, TX).
Infection control observations and interventions
Scheduled and unannounced infection control assessments with observations of practice were conducted using the CDC Infection Control Assessment and Response (ICAR) Tool for Acute Care Hospitals (www.cdc.gov/hai/prevent/infection-control-assessment-tools.html). We audited adherence to the World Health Organization Five Moments for Hand Hygiene 15 and recorded hand hygiene (HH) and personal protective equipment (PPE) observations via the iScrub Lite mobile phone application (version 1.5.3, 2018, SwipeSense, Chicago, IL). We also observed environmental cleaning, respiratory care, antibiotic compounding, and device reprocessing.
Laboratory investigation
Carbapenem-resistant Enterobacterales and P. aeruginosa from clinical cultures were forwarded to the CDC and the BPHL for carbapenem resistance mechanism testing. Colonization screenings were conducted by testing rectal swabs for carbapenemase genes using the Cepheid Xpert CarbaR (Cepheid, Sunnyvale, CA). Reference Carba-R16 when carbapenemase genes were detected, a swab was cultured to recover carbapenem-resistant organisms (Supplementary File 1 online).
Environmental sampling
Environmental samples were collected from sink drains, splash zone surfaces, and mobile equipment (Supplementary Table 1 online). Environmental samples underwent broth enrichment and plating onto selective media agar to screen for suspect isolates.
Characteristics of Case Patients with Carbapenemase-Producing Organisms, by Carbapenemase Gene Detected at Long-Term Acute-Care Hospital-A, Florida, July 2017–December 2018 a
Note. VIM, Verona-integron-encoded metallo-β-lactamase; KPC, Klebsiella pneumoniae carbapenemase; LOS, length of stay; ICU, intensive care unit; BiPAP/CPAP, bilevel/continuous positive airway pressure; PICC, peripherally inserted central catheter. P values were calculated using the Pearson χ2 test for categorical variables and the Welch unequal variance t test for continuous variables.
a Excludes 8 case patients who had CPO identified from admission screening.
b Units unless otherwise specified.
c For patients with both bla VIM and bla KPC, 5 of 6 had both carbapenemase genes identified on the same date (n=3) or within 7 days (n=2); date-specific analyses were performed using the date of specimen collection for the first incident case.
d One of the 46 KPC cases was identified as KPC-CRPA, the remainder were KPC-CRE.
e Pairwise comparison between bla KPC and bla VIM was <.05.
f Clinical specimen sources include sputum (n=2), urine (n=4), and wounds (n=2).
g Unable to conclusively assign time-point of CPO acquisition of no admission screening established before our first PPS and for those case-patients identified before when admission screening was implemented.
h Pairwise comparison between bla VIM vs. bla VIM and bla KPC was <.05.
i Pairwise comparison between bla KPC vs. bla VIM and bla KPC was <.05.
j n=48.
k No Charlson comorbidity index includes patients who may have had other comorbid conditions but did not have conditions included in the Charlson comorbitiy index.
l n=58.
m n=43.
n n=45.
o n=8.
p n=5.
q n=32.
r n=44.
s n=31.
Molecular characterization
Pulsed-field gel electrophoresis (PFGE) was performed on clinical and environmental isolates. A subset of isolates was selected for short-read whole-genome sequencing (WGS) based on epidemiological findings and representativeness of isolates in distinct PFGE clusters. The isolates that underwent short-read WGS also underwent long-read WGS to better resolve plasmid structures (Supplementary File 2 online).
Results
Outbreak overview
From July 13, 2017, to December 18, 2018, 76 incident cases were identified from 69 case patients: 11 had bla VIM, 51 had bla KPC, and 7 had bla VIM and bla KPC. All bla VIM were identified in P. aeruginosa, and bla KPC was identified in 19 Klebsiella pneumoniae, 7 Citrobacter freundii, 5 Enterobacter cloacae complex, 1 Klebsiella oxytoca, 1 Serratia marcescens, 1 Providencia rettgeri, 1 Providencia stuartii, and 1 Citrobacter farmeri. Also, 5 patients had multiple organisms harboring bla KPC, and an organism was not recovered from 18 screening tests in which bla KPC was identified.
In total, 8 case patients (2 bla VIM, 5 bla KPC, 1 bla KPC and bla VIM) were identified from admission screens; 53 case patients (7 bla VIM, 42 bla KPC, 4 bla KPC and bla VIM) were identified from PPS or discharge screens; and 8 case patients (2 bla VIM, 4 bla KPC, 2 bla KPC and bla VIM) were identified from clinical cultures.
Incident cases and prevalence
From July 2017 to December 2018, a gradual decrease in incidence of bla VIM (slope, −0.079 every 2 weeks; P = .004) and bla KPC (slope, −0.135 every 2 weeks; P = .003) was observed (Fig. 1). Declines were sharpest during the first 6 months (July 2017–January 2018: bla VIM slope, −0.220 every 2 weeks, P = .021 and bla KPC slope, −0.353 every 2 weeks; P = .018). The investigation closed on December 18, 2018, after no newly acquired cases were identified in LTACH A for 2 consecutive months.
Prevalence and new acquisitions of carbapenemase-producing organisms detected through colonization screening at long-term acute-care hospital A, Florida, July 2017–December 2018. Prevalence (ie, colonization pressure) is the total number of cases currently hospitalized/census. Newly acquired indicates the percentage of patients with incident bla VIM and bla KPC among all screened patients. Note. VIM-CRPA, Verona-integron-encoded metallo-beta-lactamase–producing carbapenem-resistant Pseudomonas aeruginosa; KPC-CRE, Klebsiella pneumoniae carbapenemase–producing carbapenem-resistant Enterobacteriaceae.
Clinical characteristics and risk factors of case patients not identified on admission to LTACH A
Patient characteristics and risk factors for the 61 case patients (88%) who did not have a CPO identified on admission are described in Table 1. The median age was 66 years (IQR, 56–73 years). Demographic risk factors were similar among patients with bla VIM, bla KPC, and both bla VIM and bla KPC. Case patients with both bla VIM and bla KPC had higher median Charlson scores and were more likely to have diabetes than those with bla VIM alone (median score, 6 vs 3; P = .033; diabetes, 100% vs 33%, respectively; P ≤ .05) or bla KPC alone (median score, 6 vs 3; P = .048; diabetes, 100% vs 67%, respectively; P ≤ .05).
Cohort study
From July 5 to December 7, 2017, 146 patients were hospitalized at LTACH A, of whom 98 (67%) met our cohort study inclusion criteria. Among the 98 patients in the cohort, the 22 patients with CPO acquired at LTACH A had similar demographics to the 76 who did not acquire a CPO. Healthcare risk factors differed in that a greater proportion of case patients had PICC lines (68% vs 40%; P = .017) and ≥3 indwelling devices (77% vs 41%; P = .003) (Table 2).
Demographic and Clinical Characteristics of Patients with and without Hospital-Acquired Carbapenemase-Producing Organisms (CPOs) During Initial Months of an Outbreak, Long-Term Acute-Care Hospital A (LTACH A), Florida, July 13–December 7, 2017
Note. VIM, Verona-integron-encoded metallo-β-lactamase; KPC, Klebsiella pneumoniae carbapenemase; LOS, length of stay; ICU, intensive care unit; BiPAP/CPAP, bilevel/continuous positive airway pressure; PICC, peripherally inserted central catheter. P values were calculated using the Pearson χ Reference Kizny Gordon, Mathers and Cheong2 test for categorical variables and the Welch unequal variance t test for continuous variables.
a Units unless otherwise specified.
b 4 patients had both VIM and KPC detected; referent group for VIM is no VIM detection; referent group for KPC is no KPC detection.
c Device cutoff was determined a priori.
Patients with a feeding tube or ≥3 indwelling medical devices had an increased risk of acquiring bla KPC (aRR, 1.18; 95% CI, 1.01–1.39; aRR, 1.21 95% CI, 1.02–1.43, respectively) and bla VIM (aRR, 1.07; 95% CI, 1.02–1.14; aRR, 1.14; 95% CI, 1.03–1.26) relative to patients without a feeding tube or with <3 indwelling medical devices (Table 3). The risk of acquiring bla VIM increased with the presence of a tracheostomy and decreased with receipt of bilevel positive airway pressure (BiPAP) or continuous positive airway pressure (CPAP).
Association of Medical Exposures and Acquisition of Carbapenemase-Producing Organisms During Initial Months of an Outbreak, by Carbapenemase Gene Detected, Long-Term Acute-Care Hospital A (LTACHA), Florida, July 13–December 7, 2017
Note. VIM, Verona-integron-encoded metallo-β-lactamase; KPC, Klebsiella pneumoniae carbapenemase; LOS, length of stay; ICU, intensive care unit; BiPAP/CPAP, bilevel/continuous positive airway pressure; PICC, peripherally inserted central catheter. P values were based on a 2-tailed probability and a significance level set at α < .05.
a All models were adjusted for age, sex, length of stay, and intensive care unit stay.
b Device cutoff was determined a priori; the referent group for medical exposures was the absence of the device and the referent group for ≥3 devices was 0–2 devices. Device history was collected through procedure logs provided by LTACH-A on a monthly basis.
Infection control assessments and interventions
Beginning in July, we conducted 5 announced and 8 unannounced infection control assessments. At the initial assessment, we observed appropriate hand hygiene (HH) in 61% of opportunities and glove and gown use in 61% and 67% of opportunities, respectively. Access to alcohol-based hand rub (ABHR) and personal protective equipment (PPE) was limited. Recommended interventions included increasing HH and PPE audits and access to ABHR and PPE, placing case patients in cohorts by CPO status to different wings with dedicated patient-care staff, and scheduling case-patient specialized care appointments (eg, hemodialysis and physical therapy) and daily room cleaning after patients without known CPOs. However, CPO acquisitions remained high through October 2017 (Fig. 2 and Supplementary File 3 online).
Epidemic curve and timing of infection control interventions to control new acquisitions of carbapenemase-producing organisms detected at long-term acute-care hospital (LTACH) A, Florida, July 2017–December 2018. “±” denotes action taken by LTACH A, but not recommended by public health officials. “KPC, admitted” represents patients identified with KPC at the time of admission. “VIM, admitted” represents patients identified with VIM at the time of admission. The incident specimen is the specimen that yielded the patient’s first identified organism and mechanism combination. Note. CDC, Centers for Disease Control and Prevention, Division of Healthcare Quality and Promotion; FDOH, Florida Department of Health; IC, infection control; PPS, point-prevalence screenings.
A follow-up assessment in November 2017 identified continued gaps in adherence to HH and contact precautions and multiple practices with potential to transmit CPOs from wastewater plumbing to patients, including storing medical supplies such as syringes used to flush enteral feeding tubes in the sink splash zone or above the swivette toilet, discarding nutritive materials in the hand washing sink, cleaning from the sink basin to the countertop, and compounding oral vancomycin in close proximity to a hand washing sink.
The FDOH provided HH and PPE training with return demonstration to ∼225 LTACH healthcare personnel; overall adherence at the next assessment was 90% for HH and 92% for both glove and gown use and was sustained in all 5 subsequent assessments over a 10-month period. Over several months, LTACH A implemented recommendations to mitigate spread from plumbing by assessing for patient care items in sink splash zones during daily infection control rounds. LTACH A also discontinued use of sinks for liquid waste disposal, adding reminder signage near sinks, and offsetting faucets from the drain (Fig. 2). Although not a public health recommendation, LTACH A treated drains with bleach for 4 months beginning in May 2018; this practice coincided with decreased attention to other interventions intended to reduce transmission from sink drains and correlated with a resurgence of bla KPC cases.
Environmental investigation
In November 2017 and January 2018, 91 environmental samples were collected from high-touch surfaces, medical equipment, sink drains in patient rooms, the pharmacy, medicine preparation rooms, and patient toilets. In total, 5 different Enterobacterales harboring bla KPC and 2 Pseudomonas spp harboring bla VIM were recovered from high-touch surfaces, sinks, and wastewater plumbing (Table 4).
Carbapenemase-Producing Organisms Detected from Environmental Samples Collected at Long-Term Acute-Care Hospital-A, Florida, November 2017 and January 2018 a
Note. ICU, intensive care unit.
a All environmental samples collected from long-term acute care hospital-A are provided in Supplementary Table 1 (online). In total, 91 environmental samples were collected. Whole-genome sequencing was not performed.
Molecular characterization of clinical and environmental isolates
A PFGE dendrogram annotated with metadata including the sequence type (ST) and carbapenemase alleles for the subset of representative isolates that underwent WGS are shown in Figure 3. Among 21 KPC-producing CRE that underwent WGS, 4 KPC alleles were identified: 7 bla KPC-2, 12 bla KPC-3, 1 bla KPC-4, and 1 bla KPC-8. Also, bla KPC-2 and bla KPC-3 were identified in different Enterobacterales and in both clinical and environmental isolates. Furthermore, 6 isolates with bla KPC-2 including 5 K. pneumoniae ST14 corresponding to the largest PFGE cluster identified, and 1 Providencia stuartii, harbored the gene on an IncC plasmid. Also, 12 isolates with bla KPC-3 represented 4 species: 5 E. cloacae complex, 4 C. freundii, 2 S. marcescens, and 1 K. pneumoniae. Among the 11 with long-read sequence data available, bla KPC-3 was identified on a Col (pHAD28) plasmid in 1 K. pneumoniae ST17 and on an IncFII plasmid in 4 C. freundii, 3 E. cloacae complex, and 1 S. marcescens, and on the chromosome in 2 E. cloacae (Fig. 3A).
Pulsed-field gel electrophoresis and whole-genome sequencing results for clinical and environmental isolates with (A) VIM-CRPA and (B) KPC-CRE detected at long-term acute-care hospital (LTACH) A, Florida, July 2017–December 2018.
No single dominant PFGE cluster was observed for VIM-CRPA (Fig. 3B). Among 6 VIM Pseudomonas isolates from 3 patients and 3 environmental sources that underwent WGS, 2 alleles were identified: 4 bla VIM-2 and 3 bla VIM-61 and were indentified in both clinical and environmental isolates. bla VIM-61 is a novel allele closely related to bla VIM-7 and was identified in a patient’s P. aeruginosa ST298 isolate that was part of a PFGE cluster and in 2 environmental isolates.
Discussion
Our public health response to the identification of a patient colonized with VIM-CRPA and KPC-CRE revealed large, concurrent CPO outbreaks in an LTACH. Epidemiologic and laboratory evidence suggest that the observed diversity in organisms and mechanisms is explained by ongoing CPO importation and carbapenemase gene transfer across different species and strains. Several factors contributed to transmission. We controlled the outbreak by improving core infection control practices, intervening on spread from sink drains, and initiating admission, PPS, and discharge screening.
LTACHs in the United States play a vital role in managing critically ill patients requiring long hospitalizations. LTACHs can serve as amplifiers of multidrug-resistant organism (MDRO) transmission due to the combination of (1) the complex patient population they serve, (2) challenges with implementing infection control practices aimed at preventing transmission, Reference Gould, Rothenberg and Steinberg17,Reference Toth, Khader and Slayton18 and (3) patient sharing with other healthcare facilities. In LTACH A, unrecognized importation of CPOs, combined with inadequate training and support for core infection control practices, likely contributed to spread of CPOs among patients and to the healthcare environment, creating reservoirs of resistant bacteria. Improved infection control practices andcoupled with enhanced detection of CPOs upon admission helped prevent later introductions from wider dissemination. Although the admission prevalence was relatively low (2%), LTACH A is regionally influential through patient sharing networks Reference Rankin and Matthews19 and has continued admission screening in partnership with public health due to the perceived value of proactively identifying patients with CPOs. Outbreaks at LTACHs, as well as intensive interventions to prevent MDRO transmission in this setting, may have meaningful impacts on increasing or decreasing, respectively, regional MDRO spread. Reference Hayden, Lin and Lolans20–Reference Ben-David, Masarwa and Fallach24 Thus, these sustained efforts at LTACH-A may provide considerable benefits to the broader region.
Most case patient isolates with bla KPC-2 belonged to large PFGE clusters of K. pneumoniae that were identified early in the investigation (September 2017–January 2018), when adherence to core infection control practices was poor. Isolates harboring bla KPC-3 corresponded to the 2 largest PFGE clusters of E. cloacae and 3 other Enterobacterales and were identified for the duration of the outbreak. Although the diversity of PFGE patterns and periodic identification of case patients on admission could have led to the conclusion that KPC cases were due to multiple introductions followed by small clusters of transmission, added resolution from WGS suggests horizontal transfer of plasmids among species may have contributed to some of the observed diversity. As short- and long-read WGS become increasingly available, their integration into public health responses may improve identification of plasmid outbreaks.
CPO outbreaks attributed to hospital wastewater plumbing have been increasingly reported, with sink drains being the most recognized reservoir. Reference Knoester, de Boer and Maarleveld25–Reference Vergara-López, Domínguez, Conejo, Pascual and Rodríguez-Baño28 Wastewater plumbing is readily contaminated with CPOs during patient care; the biofilm omnipresent in plumbing structures provides a fertile environment for plasmid exchange. Reference Kizny Gordon, Mathers and Cheong2,Reference Mathers, Vegesana and German Mesner3 Although recovery of CPOs from wastewater plumbing does not indicate directionality of spread, Reference Landelle, Legrand and Lesprit26 several factors increase the plausibility of CPO transmission from wastewater plumbing to patients at LTACH A. These include cleaning practices that disseminated contaminants from the sink basin to surrounding area, recovery of CPOs from the sink splash zone where supplies were stored, and control of transmission following improved adherence to sink hygiene. Additionally, risk factors identified in the cohort study, the presence of a feeding tube and receipt of oral vancomycin, were linked to observed sink hygiene gaps: storage of syringes for feeding tube flushes within the sink and swivette toilet splash zones and compounding of oral vancomycin adjacent to a pharmacy sink drain from which KPC-CRE was recovered. Although wastewater plumbing is hypothesized to have been the source of many transmissions, person-to-person CPO transmission also contributed, as demonstrated by some geographic clustering of cases (data not shown) and epidemiologic links to specialty care services (eg, hemodialysis), particularly early in the outbreak when adherence to hand hygiene and PPE use was low.
The index case was the first VIM-CRPA reported in Florida. Reference Rankin, Caicedo, Dotson, Gable and Chu13 LTACH-A VIM-CRPA isolates, however, showed surprising diversity in alleles and strain types, indicating that VIM-CRPA may be more common in central Florida than previously recognized. Supporting this finding, ∼1% of patients screened at admission carried bla VIM. Furthermore, some patient and environmental isolates harbored an allele, bla VIM-61, that appears to be unique to central Florida and has been identified in patients without epidemiologic linkages to LTACH-A. These findings emphasize the value of admission screening and collaboration with other healthcare facilities and public health partners to prevent further spread of CPOs in the central Florida region.
Our investigation had several limitations. First, we used paper procedure logs to identify exposure risk factors in the cohort study, and we were unable to evaluate some potential confounders, such as comorbid conditions and antibiotic receipt for noncases. For many cases, we were unable to conclusively determine whether they were acquired at LTACH A because they were identified before implementation of admission screening. Finally, we selected a subset of isolates representing varied PFGE patterns and specimen sources for WGS to infer isolate relatedness; however, it is possible that isolates with related PFGE patterns could harbor different carbapenemase alleles or plasmid markers. Isolates with plasmids sharing the same replicon and carbapenemase allele could represent plasmids from different sources and may indicate evolution of plasmid genes during the outbreak or unique plasmids introduced to LTACH A.
Through epidemiologic and molecular investigations, we identified concurrent outbreaks of carbapenemase-producing organisms. The primary reservoirs and modes of transmission may have varied among the different alleles and organisms and at different stages of the outbreak. This investigation illustrates how sustained public health and healthcare facility collaboration can control spread of emerging resistance in high-acuity postacute care facilities.
Supplementary material
To view supplementary material for this article, please visit https://doi.org/10.1017/ice.2023.231
Acknowledgments
We thank Dr Janet Glowicz, Dr Kim Skrobarcek, Dr Nailah Smith, Dr Marion A. Kainer, Craig Gillen, Jennifer Jackson, Danielle Knight, Taylor Langston, Anne Marie Chase, Hollis Houston, Lori Spicer, Mandy Lyons, and Tracey Woodard for their contributions in assisting with direct observations, laboratory testing, and specimen shipping, and data entry. We thank Justin Lee, Erisa Sula, and the CDC Genomics Sequencing Lab; Erin Breaker and Jonathon Daniels for sequencing work, and Nicholas Vlachos, Richard Stanton, and Magdalena Medrizycki for bioinformatics. In addition, we thank the healthcare personnel, the facility infection preventionist, the chief nursing officer, and the regional infection preventionist for their collaboration and dedication to containing this outbreak for the safety of their patients. The findings and conclusions in this article are those of the authors and do not necessarily represent the official position of the Centers for Disease Control and Prevention. Use of trade names is for identification only and does not imply endorsement by the Public Health Service or by the US Department of Health and Human Services. Sequence read data are available in Genbank Nucleotide Database and can be accessed under BioProject PRJNA288601 with accessions SAMN30974092 to SAMN30974118.
Financial support
No funding external to the Centers for Disease Control and Prevention was provided for this study.
Competing interests
All authors report no conflicts of interest relevant to this article.
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