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Engineering selectivity of Cutibacterium acnes phages by epigenetic imprinting

Nastassia Knödlseder, View ORCID ProfileGuillermo Nevot, Maria-José Fábrega, View ORCID ProfileJulia Mir-Pedrol, View ORCID ProfileMarta Sanvicente-García, Nil Campamà-Sanz, Rolf Lood, View ORCID ProfileMarc Güell
doi: https://doi.org/10.1101/2021.12.19.473365
Nastassia Knödlseder
1Department of Experimental and Health Sciences, Pompeu Fabra University, Barcelona, Spain
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Guillermo Nevot
1Department of Experimental and Health Sciences, Pompeu Fabra University, Barcelona, Spain
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Maria-José Fábrega
1Department of Experimental and Health Sciences, Pompeu Fabra University, Barcelona, Spain
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Julia Mir-Pedrol
1Department of Experimental and Health Sciences, Pompeu Fabra University, Barcelona, Spain
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Marta Sanvicente-García
1Department of Experimental and Health Sciences, Pompeu Fabra University, Barcelona, Spain
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Nil Campamà-Sanz
1Department of Experimental and Health Sciences, Pompeu Fabra University, Barcelona, Spain
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Rolf Lood
2Division of Infection Medicine, Department of Clinical Sciences, Faculty of Medicine, Lund, Sweden
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Marc Güell
1Department of Experimental and Health Sciences, Pompeu Fabra University, Barcelona, Spain
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  • For correspondence: marc.guell@upf.edu
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Abstract

Cutibacterium acnes (C. acnes) is a gram-positive bacterium and a member of the human skin microbiome. Despite being the most abundant skin commensal, certain members have been associated with common inflammatory disorders such as acne vulgaris. The availability of the complete genome sequences from various C. acnes clades have enabled the identification of putative methyltransferases, some of them potentially belonging to restriction-modification (R-M) systems which protect the host of invading DNA. However, little is known on whether these systems are functional in the different C. acnes strains. To investigate the activity of these putative R-M and their relevance in host protective mechanisms, we analyzed the methylome of seven representative C. acnes strains by Oxford Nanopore Technologies (ONT) sequencing. We detected the presence of a 6-methyladenine modification at a defined DNA consensus sequence in strain KPA171202 and recombinant expression of this R-M system confirmed its methylation activity. Additionally, a R-M knockout mutant verified the loss of methylation properties of the strain. We studied the potential of one C. acnes bacteriophage (PAD20) in killing various C. acnes strains and linked an increase in its specificity to phage DNA methylation acquired upon infection of a methylation competent strain. We demonstrate a therapeutic application of this mechanism where phages propagated in R-M deficient strains selectively kill R-M deficient acne-prone clades while probiotic ones remain resistant to phage infection.

Figure

Competing Interest Statement

The authors have declared no competing interest.

  • Abbreviations

    6mA
    N6-methyladenine
    4mC
    N4-methylcytosine
    5mC
    N5-methylcytosine
    C. acnes
    Cutibacterium acnes
    CDS
    coding sequence
    CRISPR
    clustered regularly interspaced palindromic repeats
    EOP
    Efficiency of Bacteriophage plaquing
    HGT
    horizontal gene transfer
    KO
    knock out
    MTase
    methyltransferase
    ONT
    Oxford nanopore technologies
    ORF
    open reading frame
    REase
    restriction endonuclease
    R-M
    restriction methylation
    SLST
    single-locus sequence typing
    MLST
    multi-locus sequence typing
    SMRT
    single nucleotide real time sequencing
    tad
    tight adherence
  • Copyright 
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    Posted December 20, 2021.
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    Engineering selectivity of Cutibacterium acnes phages by epigenetic imprinting
    Nastassia Knödlseder, Guillermo Nevot, Maria-José Fábrega, Julia Mir-Pedrol, Marta Sanvicente-García, Nil Campamà-Sanz, Rolf Lood, Marc Güell
    bioRxiv 2021.12.19.473365; doi: https://doi.org/10.1101/2021.12.19.473365
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    Engineering selectivity of Cutibacterium acnes phages by epigenetic imprinting
    Nastassia Knödlseder, Guillermo Nevot, Maria-José Fábrega, Julia Mir-Pedrol, Marta Sanvicente-García, Nil Campamà-Sanz, Rolf Lood, Marc Güell
    bioRxiv 2021.12.19.473365; doi: https://doi.org/10.1101/2021.12.19.473365

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