Application of Molecular Methods for Carbapenemase Detection

Anastasia Bilozor^{1

2}, Arta Balode³, Giorgi Chakhunashvili⁴, Tetyana Chumachenko⁵, Svetlana Egorova⁶, Marina Ivanova¹, Liidia Kaftyreva⁶, Siiri Kõljalg², Triinu Kõressaar⁷, Olga Lysenko⁸, Jolanta Miciuleviciene⁹, Reet Mändar², Danuta O Lis¹⁰, Monika Pomorska Wesolowska¹¹, Kaspar Ratnik¹², Maido Remm⁷, Jelena Rudzko¹², Tiiu Rööp², Mara Saule³, Epp Sepp², Julia Shyshporonok¹³, Leonid Titov¹³, David Tsereteli⁴, Paul Naaber^{2

12}

Affiliations

¹ Department of Microbiology, Central Laboratory, East-Tallinn Central Hospital, Tallinn, Estonia.
² Department of Microbiology, Institute of Biomedicine and Translational Medicine, University of Tartu, Tartu, Estonia.
³ Department of Biology and Microbiology, Riga Stradins University, Riga, Latvia.
⁴ Department of Communicable Disease, National Center for Disease Control and Public Health, Tbilisi, Georgia.
⁵ Department of Epidemiology, Kharkiv National Medical University, Kharkiv, Ukraine.
⁶ Department of Enteric Infections, St-Petersburg Pasteur Institute, Saint Petersburg, Russia.
⁷ Department of Bioinformatics, Institute of Molecular and Cell Biology, University of Tartu, Tartu, Estonia.
⁸ Department of Bacteriological Laboratory, Kyiv City Clinical Hospital, Kyiv, Ukraine.
⁹ Department of Microbiology, Vilnius City Clinical Hospital, Vilnius, Lithuania.
¹⁰ Department of Biohazards and Immunoallergology, Institute of Occupational Medicine and Environmental Health, Sosnowiec, Poland.
¹¹ Department of Microbiology, KORLAB Medical Laboratory, Ruda Slaska, Poland.
¹² SYNLAB Estonia, Tallinn, Estonia.
¹³ Department of Clinical and Experimental Microbiology, Republican Research and Practical Center for Epidemiology and Microbiology, Minsk, Belarus.

PMID: 31428068
PMCID: PMC6687770
DOI: 10.3389/fmicb.2019.01755

Application of Molecular Methods for Carbapenemase Detection

Anastasia Bilozor et al. Front Microbiol. 2019.

. 2019 Aug 2:10:1755.

doi: 10.3389/fmicb.2019.01755. eCollection 2019.

Authors

Affiliations

¹ Department of Microbiology, Central Laboratory, East-Tallinn Central Hospital, Tallinn, Estonia.
² Department of Microbiology, Institute of Biomedicine and Translational Medicine, University of Tartu, Tartu, Estonia.
³ Department of Biology and Microbiology, Riga Stradins University, Riga, Latvia.
⁴ Department of Communicable Disease, National Center for Disease Control and Public Health, Tbilisi, Georgia.
⁵ Department of Epidemiology, Kharkiv National Medical University, Kharkiv, Ukraine.
⁶ Department of Enteric Infections, St-Petersburg Pasteur Institute, Saint Petersburg, Russia.
⁷ Department of Bioinformatics, Institute of Molecular and Cell Biology, University of Tartu, Tartu, Estonia.
⁸ Department of Bacteriological Laboratory, Kyiv City Clinical Hospital, Kyiv, Ukraine.
⁹ Department of Microbiology, Vilnius City Clinical Hospital, Vilnius, Lithuania.
¹⁰ Department of Biohazards and Immunoallergology, Institute of Occupational Medicine and Environmental Health, Sosnowiec, Poland.
¹¹ Department of Microbiology, KORLAB Medical Laboratory, Ruda Slaska, Poland.
¹² SYNLAB Estonia, Tallinn, Estonia.
¹³ Department of Clinical and Experimental Microbiology, Republican Research and Practical Center for Epidemiology and Microbiology, Minsk, Belarus.

PMID: 31428068
PMCID: PMC6687770
DOI: 10.3389/fmicb.2019.01755

Abstract

This study has evaluated the correlation between different carbapenemases detection methods on carbapenem non-susceptible Klebsiella pneumoniae strains from Northern and Eastern Europe; 31 institutions in 9 countries participated in the research project, namely Finland, Estonia, Latvia, Lithuania, Russia, St. Petersburg, Poland, Belarus, Ukraine, and Georgia. During the research program, a total of 5,001 clinical K. pneumoniae isolates were screened for any carbapenem non-susceptibility by the disk diffusion method, Vitek 2 or Phoenix system following the EUCAST guideline on detection of resistance mechanisms, version 1.0. Strains isolated from outpatients and hospitalized patients from April 2015 to June 2015 were included. All types of samples (blood, pus, urine, etc.) excluding fecal screening or fecal colonization samples have been represented. In total, 171 carbapenemase screening-positive K. pneumoniae isolates (3.42%) were found and characterized. Several methods were used for detection of carbapenemases production, including Luminex assay (PCR and hybridization), whole genome sequencing, MALDI-TOF based Imipenem degradation assay, and immunochromatography testing. Minimal inhibitory concentration determination for Meropenem by agar-based gradient method was also used. Finally, 83 K. pneumoniae strains were carbapenemase negative by all confirmation methods (49.4% of all screening-positive ones), 74 - positive by three methods (44.0%), 8 - positive by two methods (4.8%) and 3 - positive by only one method (1.8%). The sensitivity of the tests was 96.3% for Whole genome sequencing and MALDI-TOF assay (both three undetected cases), and 95.1% for Luminex-Carba (4 undetected cases). The most commonly detected carbapenemases were NDM (n = 54) and OXA-48 (n = 26), followed by KPC-2, VIM-5, and OXA-72 (one case of each). Our results showed that different types of carbapenemases can be detected in the countries involved in the project. The sensitivity of our methods for carbapenemase detection (including screening as a first step and further confirmation tests) was >95%, but we would recommend using different methods to increase the sensitivity of detection and make it more precise.

Keywords: Klebsiella pneumoniae; MALDI-TOF carbapenemase assay; carbapenemases; luminex carbapenemases assay; whole genome sequencing.

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Figures

**FIGURE 1**
Distribution of Meropenem MIC values in screening-positive *Klebsiella pneumoniae* strains (n = 168). Blue boxes: susceptible strains (≤2 mg/L); blue boxes with white dotes: susceptible above screening cut-off (>0.125–≤2 mg/L); green boxes: susceptible, increased exposure (>2–8 mg/L); red boxes: resistant (>8 mg/L). Number of strains (number of strains with carbapenemase gene).

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References

1. CDC (2011). Multiplex Real-Time PCR Detection of Klebsiella pneumoniae Carbapenemase (KPC) and New Delhi metallo-β-lactamase (NDM-1). Available at: https://www.cdc.gov/hai/pdfs/labsettings/KPC-NDM-protocol-2011.pdf (accessed January 29, 2011).
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Application of Molecular Methods for Carbapenemase Detection

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Application of Molecular Methods for Carbapenemase Detection

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Abstract

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