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Exploring Clinical Class 1 Integrons as Valuable Targets for the Re-sensitization of Multidrug Resistant Pathogenic Bacteria Using CRISPR-Cas

Anna Berggreen Skovmand, Nicolai Juel Paaske, View ORCID ProfileArancha Peñil-Celis, Amalie Elisabeth Schønemann, Lærke Lund Hansen, View ORCID ProfileWitold Kot, View ORCID ProfileM. Pilar Garcillán-Barcia, View ORCID ProfileTue Kjærgaard Nielsen
doi: https://doi.org/10.1101/2025.03.28.645910
Anna Berggreen Skovmand
1University of Copenhagen, Department of Plant and Environmental Sciences, Frederiksberg C, Denmark
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Nicolai Juel Paaske
1University of Copenhagen, Department of Plant and Environmental Sciences, Frederiksberg C, Denmark
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Arancha Peñil-Celis
2Instituto de Biomedicina y Biotecnología de Cantabria, CSIC-Universidad de Cantabria, Cantabria, Spain
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Amalie Elisabeth Schønemann
1University of Copenhagen, Department of Plant and Environmental Sciences, Frederiksberg C, Denmark
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Lærke Lund Hansen
1University of Copenhagen, Department of Plant and Environmental Sciences, Frederiksberg C, Denmark
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Witold Kot
1University of Copenhagen, Department of Plant and Environmental Sciences, Frederiksberg C, Denmark
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M. Pilar Garcillán-Barcia
2Instituto de Biomedicina y Biotecnología de Cantabria, CSIC-Universidad de Cantabria, Cantabria, Spain
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Tue Kjærgaard Nielsen
1University of Copenhagen, Department of Plant and Environmental Sciences, Frederiksberg C, Denmark
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  • ORCID record for Tue Kjærgaard Nielsen
  • For correspondence: tkn{at}plen.ku.dk
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Abstract

The increasing prevalence of bacteria resistant to many or all types of antibiotics poses a major health crisis. Novel classes of antibiotics are only slowly being developed and alternative strategies are needed to tackle the issue. Mobile genetic elements and class 1 integrons are important facilitators for antibiotic resistance genes, with the latter being highly conserved in human pathogens. The growing prevalence of multidrug-resistant bacteria and the paucity in the development of new antibiotics underscore the urgent need for innovative approaches in the treatment of pathogens. Among these, CRISPR-Cas nucleases can be used to cleave acquired resistance genes, leading to either plasmid curing or cell death if the target is on a chromosome. In this study, we investigate the feasibility of using class 1 integrons as a target for Cas9-based cleavage leading to re-sensitizing antibiotic-resistant bacteria. We analyze the conserved and widespread integrase gene intI1 and conclude that it is a suitable target for Cas-based re-sensitization due to its high sequence conservation and its occurrence largely limited to human pathogens, alleviating the risk of targeting benign bacteria. We developed a broad host range conjugative plasmid encoding a class 1 integron-targeting Cas9 system that leads to removal of resistance plasmids in target bacteria with subsequent re-sensitization towards antibiotics. We find that 290 distinct ARGs co-occur on int1-harboring plasmids, showing the potential for re-sensitization towards a very broad range of antibiotics.

Competing Interest Statement

The authors have declared no competing interest.

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The copyright holder for this preprint is the author/funder, who has granted bioRxiv a license to display the preprint in perpetuity. It is made available under a CC-BY-NC-ND 4.0 International license.
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Posted March 28, 2025.
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Exploring Clinical Class 1 Integrons as Valuable Targets for the Re-sensitization of Multidrug Resistant Pathogenic Bacteria Using CRISPR-Cas
Anna Berggreen Skovmand, Nicolai Juel Paaske, Arancha Peñil-Celis, Amalie Elisabeth Schønemann, Lærke Lund Hansen, Witold Kot, M. Pilar Garcillán-Barcia, Tue Kjærgaard Nielsen
bioRxiv 2025.03.28.645910; doi: https://doi.org/10.1101/2025.03.28.645910
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Exploring Clinical Class 1 Integrons as Valuable Targets for the Re-sensitization of Multidrug Resistant Pathogenic Bacteria Using CRISPR-Cas
Anna Berggreen Skovmand, Nicolai Juel Paaske, Arancha Peñil-Celis, Amalie Elisabeth Schønemann, Lærke Lund Hansen, Witold Kot, M. Pilar Garcillán-Barcia, Tue Kjærgaard Nielsen
bioRxiv 2025.03.28.645910; doi: https://doi.org/10.1101/2025.03.28.645910

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