Profilin Interacts with the Gly-Pro-Pro-Pro-Pro-Pro Sequences of Vasodilator-Stimulated Phosphoprotein (VASP): Implications for Actin-Based Listeria Motility

Abstract

Intracellular actin-based motility of Listeria monocytogenes requires protein−protein interactions involving two different proline-rich sequences: first, the tightly bound bacterial surface protein ActA uses its multiple oligoproline registers [consensus sequence = FE(D)FPPPPTD(E)E(D)] to tether vasodilator-stimulated phosphoprotein (VASP) to the bacterial surface; and second, VASP then deploys its own multiple GPPPPP (or GP₅) registers to localize the actin−regulatory protein profilin to promote actin polymerization. We now report that fluorescence titration showed that GP₅GP₅GP₅ peptide binds to profilin (K_D of 84 μM), and the peptide weakly inhibits exchange of actin-bound nucleotide in the absence or presence of profilin. Microinjection of synthetic GPPPPP triplet into Listeria-infected PtK2 cells promptly arrested motility at an intracellular concentration of 10 μM. This inhibition was completely neutralized when equimolar concentrations of profilin and GP₅GP₅GP₅ were simultaneously microinjected. Fluorescence studies with [His-133-Ser]-profilin, a site-directed mutant previously shown to be defective in binding poly-l-proline [Bjorkegren, C., Rozycki, M., Schutt, C. E., Lindberg, U., & Karlsson, R. (1993) FEBS Lett. 333, 123−126], exhibits little or no evidence of saturable GP₅GP₅GP₅ binding. When an equimolar concentration of this [His-133-Ser]-profilin mutant was co-injected with GP₅GP₅GP₅, the peptide's inhibitory action remained completely unaffected, indicating that GP₅GP₅GP₅ binding to wild-type profilin represents a key step in actin-based pathogen motility. We also present a model that shows how the focal binding of VASP with its GPPPPP registers can greatly increase the local concentration of profilin and/or profilin−actin−ATP complex at the bacteria/rocket-tail interface.