Single-molecule analysis of the entire perfringolysin O pore formation pathway.
Conall McGuinnessJames C WalshCharles Bayly-JonesMichelle A DunstoneMichelle P ChristieCraig J MortonMichael W ParkerTill BoeckingPublished in: eLife (2022)
The cholesterol-dependent cytolysin perfringolysin O (PFO) is secreted by Clostridium perfringens as a bacterial virulence factor able to form giant ring-shaped pores that perforate and ultimately lyse mammalian cell membranes. To resolve the kinetics of all steps in the assembly pathway, we have used single-molecule fluorescence imaging to follow the dynamics of PFO on dye-loaded liposomes that lead to opening of a pore and release of the encapsulated dye. Formation of a long-lived membrane-bound PFO dimer nucleates the growth of an irreversible oligomer. The growing oligomer can insert into the membrane and open a pore at stoichiometries ranging from tetramers to full rings (~35 mers), whereby the rate of insertion increases linearly with the number of subunits. Oligomers that insert before the ring is complete continue to grow by monomer addition post insertion. Overall, our observations suggest that PFO membrane insertion is kinetically controlled.
Keyphrases
- single molecule
- fluorescence imaging
- living cells
- atomic force microscopy
- drug delivery
- pseudomonas aeruginosa
- escherichia coli
- sars cov
- photodynamic therapy
- staphylococcus aureus
- single cell
- minimally invasive
- highly efficient
- stem cells
- cell therapy
- cancer therapy
- aqueous solution
- antimicrobial resistance
- cystic fibrosis
- bone marrow
- mesenchymal stem cells
- coronavirus disease
- rare case
- high speed
- liquid chromatography
- tandem mass spectrometry