The molecular detection of carbapenem markers with a two-levels amplification screening protocol: epidemiological and resistome insights

Maddalena Calvo; Giuseppe Migliorisi; Gaetano Maugeri; Dafne Bongiorno; Carmelo Bonomo; Emanuele Nicitra; Guido Scalia; Stefania Stefani

doi:10.3389/fmicb.2024.1346442

The molecular detection of carbapenem markers with a two-levels amplification screening protocol: epidemiological and resistome insights

Front Microbiol. 2024 Feb 23:15:1346442. doi: 10.3389/fmicb.2024.1346442. eCollection 2024.

Authors

Maddalena Calvo¹, Giuseppe Migliorisi¹, Gaetano Maugeri^{1

2}, Dafne Bongiorno², Carmelo Bonomo², Emanuele Nicitra², Guido Scalia^{1

2}, Stefania Stefani^{1

2}

Affiliations

¹ U.O.C. Laboratory Analysis Unit, A.O.U. "Policlinico-San Marco", Catania, Italy.
² Department of Biomedical and Biotechnological Sciences (BIOMETEC), University of Catania, Catania, Italy.

Abstract

Objectives: Carbapenem-resistance is a challenging healthcare concern and require specific stewardship programs. Monitoring workflows include the identification from surveillance samples, such as rectal swabs. Although culture assays represent the gold standard, data report a significant effectiveness in detecting carbapenemases genes directly from rectal swabs. The aim of this study was to evaluate the REALQUALITY Carba-Screen kit (AB ANALITICA, Padova, Italy) in detecting carbapenemases genes directly from rectal swabs, also comparing its effectiveness to culture assays results. A next-generation sequencing (NGS) was performed to investigate the positive samples about resistance markers and sequence type (ST).

Methods: A number of 136 rectal swabs were collected from the University Hospital Policlinico of Catania critical wards. The samples simultaneously underwent culture and molecular assays (REALQUALITY Carba-Screen kit). The molecular method included two-steps. The first step (1 h and 6 min) rapidly excluded negative samples, while the second one (1 h and 6 min) included only positive samples for a resistance confirmation. All the positive culture samples underwent NGS analysis.

Results: Statistical evaluations demonstrated high sensitivity (100%) and detection rates (92.6%) for the REALQUALITY Carba-Screen kit, which mostly correlated to the standard workflow. All the culture positive results matched the positive molecular results, which were mainly confirmed by the NGS resistome analysis. The identified ST appeared to be diversified and different from the clinically significative strains of the same setting, furnishing interesting epidemiological evidence.

Conclusion: The molecular detection allowed a coordinate approach in a high-prevalence multi-drug-resistance area. The rapid identification with a multi-step procedure accelerated the infection control procedures, while the preliminary negative results reduced the overtreatment episodes. The molecular method efficacy was confirmed through the NGS. In conclusion, the molecular screening could initially lead to a more conservative approach, which may be reevaluated after a culture result about the microorganisms' identification and susceptibility profile.

Keywords: carbapenem-resistance; infection control measures; molecular assays; resistome analysis; screening protocol.

Grants and funding

The author(s) declare financial support was received for the research, authorship, and/or publication of this article. This research was partially supported by EU funding with the MUR PNRR Extended Partnership Initiative of Emerging Infection Disease Project n. PE 00000007 INF-ACT.