dgkh00038310.3205/dgkh000383urn:nbn:de:0183-dgkh0003837Research ArticleDetection of Serratia marcescens in neonatal intensive care units requires a rapid and comprehensive infection control response starting with the very first caseDer Nachweis bereits eines Serratia marcescens Falles auf einer neonatologischen Intensivstation bedarf schneller und umfassender HygienemaßnahmenBöhneBöhneCarolinC
Department of Pediatric Pulmonology, Allergology and Neonatology, Hannover Medical School, Hannover, GermanyDepartment of Pediatric Pulmonology, Allergology and Neonatology, Hannover Medical School, Hannover, GermanyauthorChhatwalChhatwalPatrickPInstitute for Medical Microbiology and Hospital Epidemiology, Hannover Medical School, Hannover, GermanyauthorPeterPeterCorinnaCDepartment of Pediatric Pulmonology, Allergology and Neonatology, Hannover Medical School, Hannover, GermanyauthorEbadiEbadiEllaEInstitute for Medical Microbiology and Hospital Epidemiology, Hannover Medical School, Hannover, GermanyauthorHansenHansenGesineGDepartment of Pediatric Pulmonology, Allergology and Neonatology, Hannover Medical School, Hannover, GermanyauthorSchlüterSchlüterDirkDInstitute for Medical Microbiology and Hospital Epidemiology, Hannover Medical School, Hannover, GermanyauthorBangeBangeFranz-ChristophFCInstitute for Medical Microbiology and Hospital Epidemiology, Hannover Medical School, Hannover, GermanyauthorBohnhorstBohnhorstBettinaBDepartment of Pediatric Pulmonology, Allergology and Neonatology, Hannover Medical School, Hannover, GermanyauthorBaierBaierClaasC
Institute for Medical Microbiology and Hospital Epidemiology, Hannover Medical School, Carl-Neuberg-Straße 1, 30625 Hannover, Germany, Phone: +49 511 532 8675, Fax: +49 511 532 8174Institute for Medical Microbiology and Hospital Epidemiology, Hannover Medical School, Hannover, Germanybaier.claas@mh-hannover.deauthorGerman Medical Science GMS Publishing House
Düsseldorf
610preterm infantsneonatal intensive care unitclusterinfection controloutbreakSerratia marcescensFrühgeboreneneonatologische IntensivstationHäufungAusbruchHygieneSerratia marcescens20210315englThis is an Open Access article distributed under the terms of the Creative Commons Attribution 4.0 License.Dieser Artikel ist ein Open-Access-Artikel und steht unter den Lizenzbedingungen der Creative Commons Attribution 4.0 License (Namensnennung).2196-522616GMS Hygiene and Infection ControlGMS Hyg Infect Control12Hintergrund:Serratiamarcescens ist ein wohlbekannter, herausfordernder Erreger in der neonatologischen Intensivmedizin. Er kann schwere Infektionen bei Frühgeborenen und nosokomiale Ausbrüche verursachen. Methoden: In der vorliegenden Arbeit präsentieren wir das Hygienemanagement einer Serratia marcescens Häufung auf einer tertiären neonatologischen Intensivstation. Ergebnis und Schlussfolgerungen: Das vorgestellte Hygienemanagement, das bereits mit dem ersten auftretenden Serratia marcescens Fall angewendet wird, zielt insbesondere auf die frühe Detektion und schnelle Unterbrechung von nosokomialen Transmissionsketten ab. Ein engmaschiges, sensitives mikrobiologisches Screening, eine strikte räumliche Isolation und die Stärkung der Händehygiene-Adhärenz sind zentrale Maßnahmen in diesem Konzept, welches insgesamt 8 Komponenten beinhaltet. Das Konzept war in der Lage, die Häufungssituation rasch zu kontrollieren und zu begrenzen. Background:Serratiamarcescens is a well-known and challenging pathogen in neonatal intensive care units. It is responsible for severe infections and can cause nosocomial outbreaks. Methods: We present the infection control response to a Serratiamarcescens cluster which occurred in a tertiary neonatal intensive care unit. Results and conclusions: The presented comprehensive and decisive hygiene management response starting with the very first case aims especially at early detection and immediate interruption of nosocomial transmission. Frequent and sensitive microbiological screening, rigorous spatial isolation of colonized infants, and reinforcing adherence to hand hygiene are essential in this response, which comprises eight measures. It prevented a full-blown outbreak.BackgroundSerratia marcescens (Sm) is associated with nosocomial outbreaks in neonatal intensive care units (NICUs) , , , , . Preterm infants bear a particular risk for severe infections caused by Sm due to their immature immune system. Besides bloodstream infections (BSIs), Sm can also cause meningitis/brain abscess or conjunctivitis . Overall, the occurrence of Sm in an NICU requires a fast and decisive response to prevent or contain nosocomial spread. Here, we present and discuss a comprehensive infection control response, which was successfully implemented in a tertiary NICU to rapidly control a Sm cluster. MethodsThe cluster occurred in an NICU of a German university hospital in May/June 2020. The NICU had 10 beds in three two-bed rooms and one four-bed room. The regular nurse-to-patient ratio was 1:1 to 1:3. Assigned cleaning and healthcare staff serviced the ward. The ward was disinfected twice daily. The incubators were changed weekly and disinfected at a central facility.According to the recommendations of the Commission for Hospital Hygiene and Infection Prevention at the German Robert Koch Institute, preterm infants were regularly screened for colonization of various bacteria, including Gram-negative rods, during their stay at the NICU. The screening included rectal and respiratory specimens and was performed upon admission and once a week afterwards (every Monday). Sm isolates were molecularly characterized by pulsed-field gel electrophoresis (PFGE) according to an in-house protocol (restriction enzyme SpeI) in a hygiene laboratory that is accredited according to ISO/IEC 17025 by the German national accreditation body. PFGE patterns were compared visually. The Sm cluster was investigated in line with the ORION statement. The institution’s ethics committee approved the analysis (number 9264_BO_K_2020).ResultsThe cluster affected four preterm infants (two pairs of twins). They had a birth weight of 1,150 g and 1,350 g (30+2 weeks) and 1,450 g and 1,590 g (32+1 weeks). All the children tested positive within one week and Sm acquisition was assumed to be nosocomial. Each pair of twins shared one room. All infants were colonized rectally, including three who additionally had positive respiratory specimens. The isolates shared an identical phenotypic antimicrobial susceptibility pattern (susceptible to third-generation cephalosporins, fluoroquinolones and carbapenems). The first patient with Sm was detected by routine weekly colonization screening in the NICU. After Sm detection in this first patient, the following measures were implemented immediately: Frequent screening targeting Sm. Another weekly screening day (Thursday) was therefore established. These screening specimens were processed on standard MacConkey agar with a colistin disk to increase sensitivity for Sm. Figure 1 shows this approach. Establishment of an interdisciplinary task force to ensure proper and timely information to all stakeholders (neonatologists, infection control staff, microbiologists).Strict spatial isolation (single room or cohort) and contact precautions (gloves, gown). Moreover, the nursing staff were exclusively assigned and did not care for other infants (as far as possible). Discharge or transfer of Sm patients as soon as possible. Reinforcement of adherence to hand hygiene by staff (including external personnel) and parents by frequent on-site training.Clinical alertness towards the development of Sm infection in colonized patients. Molecular characterization to i) verify (or falsify), ii) better understand, and iii) visualize potential transmission. Environmental source search (e.g., the microbiologic examination of inanimate surfaces and medical equipment with contact plates and swabs or microbiologic examination of disinfectant solution and nutrition, including breastmilk). Sm colonization of the three other patients was detected within one week following the index case. Fortunately, one pair of twins was successfully transferred from the NICU within one week of Sm detection. The other pair of twins, however, stayed in the NICU for a total of 43 days. Sm was not detected in this pair of twins by the end of their hospital stay. The index patient developed an Sm BSI after initial rectal colonization. Empiric antibiotic therapy included meropenem and tobramycin. The patient recovered quickly with no foreseeable long-term effects to date. An initial PFGE was performed within two weeks that included the colonizing strains of all four patients. The isolates had an identical PFGE pattern. Figure 2 shows the result of a PFGE comprising the blood culture isolate of the first patient. In addition, breastmilk from the mother of the first patient was examined; however, Sm was not detected. No further cases occurred in the NICU with a turnover of 29 new admissions and 18 transfers by the time the remaining pair of twins with Sm were discharged from the NICU. All measures were continued until this discharge. However, the additional weekly screening targeting Sm was performed for another two weeks thereafter.DiscussionImplementation of this multimodal infection control response led to the immediate containment of the cluster. The response targeted various elements. Frequent and sensitive microbiological screening to quickly detect positive patients and monitor potentially ongoing transmission was essential. Repeated screening has also been described in other Sm clusters and is an important tool in outbreak control , . To increase sensitivity, we made use of the intrinsic resistance of Sm against colistin. A similar approach using an enrichment broth containing colistin has been described . In contrast to the use of an enrichment broth, the colistin disk allows a matrix-assisted laser desorption/ionization time-of-flight mass spectrometry-based identification of colonies growing in the inhibition zone after incubation for 18–24 h.All stakeholders were involved to guarantee a prompt and continuous flow of information by implementing an interdisciplinary task force.The following measures, which are often reported in outbreak literature, are specifically aimed at interrupting transmission: spatial isolation (e.g., private room), exclusively assigned staff for Sm positive patients, strengthening hand hygiene, and discharge of Sm carriers , , , . Reinforcing hand hygiene appears to be of particular importance , , as contaminated hands are a relevant route of transmission . Contaminated hands might have also played a role in this cluster, as the pairs of twins were each located in different rooms, but cared for by the same staff prior to Sm detection. Timely discharge and transfer of Sm positive patients is important to remove or minimize a potential source of transmission. It is noteworthy that one pair of twins stayed in the NICU for a total of 43 days. Due to this long period, transmission control was a challenge, considering all patient admissions and transfers.Clinical alertness towards the development of infections, especially BSI, is essential to ensure early administration of adequate empiric antibiotic therapy for suspected invasive infection in Sm-colonized patients. Here, one of the four infants developed BSI, which is a known and feared phenomenon in Sm clusters . Molecular characterization of bacterial isolates in a cluster is crucial for a better understanding of the transmission process. PFGE was used in this case. Sequencing-based methods are also emerging for Sm , . One benefit of sequencing-based methods with a standardized nomenclature (e.g., core genome multilocus sequence typing) is that data generated from different settings (e.g., different outbreaks) can be compared quite easily.Sm might persist in the environment; it was found in environmental samples from Sm clusters . Therefore, environmental microbiological sampling should be performed – especially when the epidemiological pattern suggests a point source rather than patient-to-patient transmission. We had planned to examine inanimate surfaces (e.g., incubators, ultrasound equipment) and disinfectant solution in dispensers if more cases arose. In the present case, the frequency of regular cleaning was already quite high. However, intensified cleaning is reported as an outbreak control measure , . We refrained from testing staff. Complete or partial closure of an NICU is an ultima ratio measure in Sm outbreaks . However, it is highly disruptive and often not feasible. Fortunately, this was not necessary in our case. In conclusion, rapid implementation of a comprehensive and multimodal infection control response starting immediately with the first identified Sm patient is required to avoid a full-blown outbreak. Frequent and sensitive microbiological screening of all patients, rigorous spatial isolation of colonized infants and reinforcing adherence to hand hygiene are essential. De-escalation of measures is possible once the last Sm patient has been discharged.NotesCompeting interestsThe authors declare that they have no competing interests.FundingThis research did not receive any specific grant from funding agencies in the public, commercial, or non-profit sectors.Authors’ contributionsAll authors contributed to the manuscript according to the ICMJE (International Committee of Medical Journal Editors) recommendations and were involved in data acquisition, analysis and interpretation. CB, PC, CBO and F-CB prepared the manuscript. CB organized the drafting process. BB, CP, CB, EE and F-CB supervised the infection control response on the ward. PC and DS were involved in microbiologic diagnostics. All authors critically revised the manuscript, account for accuracy and correctness and have read and agreed to the final draft before submission. CBO and PC are contributed equally as first author. Jang TNFung CPYang TLShen SHHuang CSLee SHUse of pulsed-field gel electrophoresis to investigate an outbreak of Serratia marcescens infection in a neonatal intensive care unit2001J Hosp Infect13-9Jang TN, Fung CP, Yang TL, Shen SH, Huang CS, Lee SH. Use of pulsed-field gel electrophoresis to investigate an outbreak of Serratia marcescens infection in a neonatal intensive care unit. J Hosp Infect. 2001 May;48(1):13-9. DOI: 10.1053/jhin.2001.0947https://doi.org/10.1053/jhin.2001.0947Redondo-Bravo LGutiérrez-González ESan Juan-Sanz IFernández-Jiménez IRuiz-Carrascoso GGallego-Lombardo SSánchez-García LElorza-Fernández DPellicer-Martínez AOmeñaca FRobustillo-Rodela ASerratia marcescens outbreak in a neonatology unit of a Spanish tertiary hospital: Risk factors and control measures2019Am J Infect Control271-9Redondo-Bravo L, Gutiérrez-González E, San Juan-Sanz I, Fernández-Jiménez I, Ruiz-Carrascoso G, Gallego-Lombardo S, Sánchez-García L, Elorza-Fernández D, Pellicer-Martínez A, Omeñaca F, Robustillo-Rodela A. Serratia marcescens outbreak in a neonatology unit of a Spanish tertiary hospital: Risk factors and control measures. Am J Infect Control. 2019 Mar;47(3):271-9. DOI: 10.1016/j.ajic.2018.08.026https://doi.org/10.1016/j.ajic.2018.08.026Yeo KTOctavia SLim KLin CLin RThoon KCTee NWSYung CFSerratia marcescens in the neonatal intensive care unit: A cluster investigation using molecular methods2020J Infect Public Health1006-11Yeo KT, Octavia S, Lim K, Lin C, Lin R, Thoon KC, Tee NWS, Yung CF. Serratia marcescens in the neonatal intensive care unit: A cluster investigation using molecular methods. J Infect Public Health. 2020 Jul;13(7):1006-11. DOI: 10.1016/j.jiph.2019.12.003https://doi.org/10.1016/j.jiph.2019.12.003Åttman EKorhonen PTammela OVuento RAittoniemi JSyrjänen JMattila EÖsterblad MHuttunen RA Serratia marcescens outbreak in a neonatal intensive care unit was successfully managed by rapid hospital hygiene interventions and screening2018Acta Paediatr425-9Åttman E, Korhonen P, Tammela O, Vuento R, Aittoniemi J, Syrjänen J, Mattila E, Österblad M, Huttunen R. A Serratia marcescens outbreak in a neonatal intensive care unit was successfully managed by rapid hospital hygiene interventions and screening. Acta Paediatr. 2018 Mar;107(3):425-9. DOI: 10.1111/apa.14132https://doi.org/10.1111/apa.14132Zingg WSoulake IBaud DHuttner BPfister RRenzi GPittet DSchrenzel JFrancois PManagement and investigation of a Serratia marcescens outbreak in a neonatal unit in Switzerland – the role of hand hygiene and whole genome sequencing2017Antimicrob Resist Infect Control125Zingg W, Soulake I, Baud D, Huttner B, Pfister R, Renzi G, Pittet D, Schrenzel J, Francois P. Management and investigation of a Serratia marcescens outbreak in a neonatal unit in Switzerland – the role of hand hygiene and whole genome sequencing. Antimicrob Resist Infect Control. 2017;6:125. DOI: 10.1186/s13756-017-0285-xhttps://doi.org/10.1186/s13756-017-0285-xFleisch FZimmermann-Baer UZbinden RBischoff GArlettaz RWaldvogel KNadal DRuef CThree consecutive outbreaks of Serratia marcescens in a neonatal intensive care unit2002Clin Infect Dis767-73Fleisch F, Zimmermann-Baer U, Zbinden R, Bischoff G, Arlettaz R, Waldvogel K, Nadal D, Ruef C. Three consecutive outbreaks of Serratia marcescens in a neonatal intensive care unit. Clin Infect Dis. 2002 Mar;34(6):767-73. DOI: 10.1086/339046https://doi.org/10.1086/339046Ferreira RLRezende GSDamas MSFOliveira-Silva MPitondo-Silva ABrito MCALeonardecz Ede Góes FRCampanini EBMalavazi Ida Cunha AFPranchevicius MDSCharacterization of KPC-Producing in an Intensive Care Unit of a Brazilian Tertiary Hospital2020Front Microbiol956Ferreira RL, Rezende GS, Damas MSF, Oliveira-Silva M, Pitondo-Silva A, Brito MCA, Leonardecz E, de Góes FR, Campanini EB, Malavazi I, da Cunha AF, Pranchevicius MDS. Characterization of KPC-Producing in an Intensive Care Unit of a Brazilian Tertiary Hospital. Front Microbiol. 2020;11:956. DOI: 10.3389/fmicb.2020.00956https://doi.org/10.3389/fmicb.2020.00956Giles MHarwood HMGosling DAHennessy DPearce CTDaley AJWhat is the best screening method to detect Serratia marcescens colonization during an outbreak in a neonatal intensive care nursery?2006J Hosp Infect349-52Giles M, Harwood HM, Gosling DA, Hennessy D, Pearce CT, Daley AJ. What is the best screening method to detect Serratia marcescens colonization during an outbreak in a neonatal intensive care nursery? J Hosp Infect. 2006 Mar;62(3):349-52. DOI: 10.1016/j.jhin.2005.09.015https://doi.org/10.1016/j.jhin.2005.09.015Montagnani CCocchi PLega LCampana SBiermann KPBraggion CPecile PChiappini Ede Martino MGalli LSerratia marcescens outbreak in a neonatal intensive care unit: crucial role of implementing hand hygiene among external consultants2015BMC Infect Dis11Montagnani C, Cocchi P, Lega L, Campana S, Biermann KP, Braggion C, Pecile P, Chiappini E, de Martino M, Galli L. Serratia marcescens outbreak in a neonatal intensive care unit: crucial role of implementing hand hygiene among external consultants. BMC Infect Dis. 2015 Jan;15:11. DOI: 10.1186/s12879-014-0734-6https://doi.org/10.1186/s12879-014-0734-6Rossen JWADombrecht JVanfleteren DDe Bruyne Kvan Belkum ARosema SLokate MBathoorn EReuter SGrundmann HErtel JHiggins PGSeifert HEpidemiological Typing of Serratia marcescens Isolates by Whole-Genome Multilocus Sequence Typing2019J Clin Microbiole01652-18Rossen JWA, Dombrecht J, Vanfleteren D, De Bruyne K, van Belkum A, Rosema S, Lokate M, Bathoorn E, Reuter S, Grundmann H, Ertel J, Higgins PG, Seifert H. Epidemiological Typing of Serratia marcescens Isolates by Whole-Genome Multilocus Sequence Typing. J Clin Microbiol. 2019 Apr;57(4):e01652-18. DOI: 10.1128/JCM.01652-18https://doi.org/10.1128/JCM.01652-18011
Figure 1: Serratia marcescens microbiological screeningA: MacConkey agar with a colistin disk showing the growth of Klebsiella oxytoca (white arrows) and Serratiamarcescens (black arrows); Serratia marcescens colonies are only visible within the colistin inhibition zone; B: Colistin inhibition zone with Serratia marcescens colonies in detail; C: Example of MacConkey agar without a colistin disk; Serratia marcescens colonies are masked by the more abundant species (Klebsiella oxytoca); D: Pure culture of Serratia marcescens, which is not inhibited by colistin due to intrinsic resistance.
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Figure 2: Pulsed-field gel electrophoresis C=Staphylococcus aureus quality control strain NCTC® 8325; R=In-house Serratia marcescens reference strain; 1a, 2, 3 and 4=Serratia marcescens isolates (rectal specimens) of the four cluster patients showing the identical pulsotype (monoclonal pattern); 1b=Serratia marcescens blood culture isolate of patient 1 showing the same pattern as the rectal colonization isolate (1a); 5=Serratia marcescens isolate of a patient not belonging to the cluster.