Cooperation between coagulase and von willebrand factor binding protein in Staphylococcus aureus fibrin pseudocapsule formation

Dominique C S Evans; Amanda B Khamas; Alex Payne-Dwyer; Adam J M Wollman; Kristian S Rasmussen; Janne K Klitgaard; Birgitte Kallipolitis; Mark C Leake; Rikke L Meyer

doi:10.1016/j.bioflm.2024.100233

Cooperation between coagulase and von willebrand factor binding protein in Staphylococcus aureus fibrin pseudocapsule formation

Biofilm. 2024 Oct 23:8:100233. doi: 10.1016/j.bioflm.2024.100233. eCollection 2024 Dec.

Authors

Affiliations

¹ School of Physics, Engineering and Technology, University of York, York, UK.
² Interdisciplinary Nanoscience Centre, Aarhus University, Aarhus, Denmark.
³ Department of Biology, University of York, York, UK.
⁴ Department of Biochemistry and Molecular Biology, University of Southern Denmark, Odense, Denmark.

Abstract

The major human pathogen Staphylococcus aureus forms biofilms comprising of a fibrin network that increases attachment to surfaces and shields bacteria from the immune system. It secretes two coagulases, Coagulase (Coa) and von Willebrand factor binding protein (vWbp), which hijack the host coagulation cascade and trigger the formation of this fibrin clot. However, it is unclear how Coa and vWbp contribute differently to the localisation and dynamics of clot assembly in growing biofilms. Here, we address this question using high-precision time-resolved confocal microscopy of fluorescent fibrin to establish the spatiotemporal dynamics of fibrin clot formation in functional biofilms. We also use fluorescent fusion proteins to visualise the locations of Coa and vWbp in biofilms using both confocal laser scanning and high resolution highly inclined and laminated optical sheet microscopy. We visualise and quantify the spatiotemporal dynamics of fibrin production during initiation of biofilms in plasma amended with fluorescently labelled fibrinogen. We find that human serum stimulates coagulase production, and that Coa and vWbp loosely associate to the bacterial cell surface. Coa localises to cell surfaces to produce a surface-attached fibrin pseudocapsule but can diffuse from cells to produce matrix-associated fibrin. vWbp produces matrix-associated fibrin in the absence of Coa, and furthermore accelerates pseudocapsule production when Coa is present. Finally, we observe that fibrin production varies across the biofilm. A sub-population of non-dividing cells does not produce any pseudocapsule but remains within the protective extended fibrin network, which could be important for the persistence of S. aureus biofilm infections as antibiotics are more effective against actively growing cells. Our findings indicate a more cooperative role between Coa and vWbp in building fibrin networks than previously thought, and a bet-hedging cell strategy where some cells produce biofilm matrix while others do not, but instead assume a dormant phenotype that could be associated with antibiotic tolerance.

Keywords: Biofilm; CLIP tag; Confocal microscopy; Extracellular matrix; HILO; Monomeric superfolder GFP; SNAP tag.