AI Article Synopsis

  • Biofilms are communities of bacteria that secrete a protective matrix, rich in proteins and enzymes, but the specific roles of these enzymes in biofilm formation are not well understood.
  • The study focused on PaAP, an aminopeptidase enzyme from Pseudomonas aeruginosa, finding that its deletion enhanced initial biofilm attachment but caused significant cell death and disruption of the biofilm after 24 hours.
  • The research highlights PaAP's critical role in biofilm development and suggests that targeting this enzyme could be a potential strategy to prevent infections caused by P. aeruginosa and related biofilm issues.

Article Abstract

Biofilm bacteria are embedded within a self-secreted extracellular matrix that contains a considerable amount of proteins including many extracellular enzymes. However, little is known about the roles of such enzymes in biofilm development. Here, we studied Pseudomonas aeruginosa aminopeptidase (PaAP, encoded by PA2939 that we named the gene as paaP in this study), a quorum-sensing-regulated enzyme and one of the most abundant extracellular proteins in the biofilm matrix of this opportunistic pathogen and environmental bacterium. We found that deletion of paaP in P. aeruginosa increased initial attachment and biofilm formation at early stages of biofilm development. After 24 h growth, loss of PaAP resulted in substantial cell death and biofilm disruption. Bacterial cell death was independent of biofilm matrix polysaccharide Psl, while biofilm disruption was due to the degradation of Psl matrix by dead-bacteria-released glycosyl hydrolase PslG, thereby leading to biofilm dispersion. PaAP functioned extracellularly and aminopeptidase catalytic activity was essential for its effect on biofilm development. Our data reveal an important role of extracellular aminopeptidase in biofilm development, suggesting PaAP as a therapeutic target for preventing P. aeruginosa infection and combating biofilm-related complications.

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http://dx.doi.org/10.1111/1758-2229.12682DOI Listing

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