RT Journal Article SR Electronic T1 Fast activation cycles of Rac1 at the lamellipodium tip trigger membrane protrusion JF bioRxiv FD Cold Spring Harbor Laboratory SP 130849 DO 10.1101/130849 A1 Amine Mehidi A1 Olivier Rossier A1 Anaël Chazeau A1 Fabien Binamé A1 Amanda Remorino A1 Mathieu Coppey A1 Zeynep Karatas A1 Jean-Baptiste Sibarita A1 Violaine Moreau A1 Grégory Giannone YR 2017 UL http://biorxiv.org/content/early/2017/04/27/130849.abstract AB The spatiotemporal coordination of actin regulators in the lamellipodium determines the dynamics and architecture of branched F-actin networks during cell migration. The WAVE complex, effector of Rac1 during cell protrusion, is concentrated at the lamellipodium tip. Yet, correlation of Rho GTPases activation with cycles of membrane protrusions, suggested that Rac1 activation is not synchronized with membrane protrusion and occurs behind the lamellipodium. However, RhoA activation is maximal at the cell edge and synchronized with edge progression. Combining single protein tracking (SPT) and super-resolution imaging with loss- or gain-of-function of Rho GTPases mutants, we demonstrate that Rac1 immobilizations at the lamellipodium tip are correlated with Rac1 activation, on the contrary to RhoA. We show that Rac1 effector WAVE and Rac1 regulator IRSp53 accumulate at the lamellipodium tip by membrane free-diffusion and trapping. Nevertheless, wild-type Rac1, which directly interacts with WAVE and IRSp53, only displays slower diffusion at the lamellipodium tip, suggesting fast local activation/inactivation cycles. Local optogenetic activation of Rac1, triggered by Tiam1 membrane recruitment, proves that Rac1 activation must occur at the lamellipodium tip and not behind the lamellipodium to trigger efficient membrane protrusion. Furthermore, coupling tracking with optogenetic activation of Rac1 demonstrates that Rac1-WT diffusive properties are unchanged despite enhanced lamellipodium protrusion. Taken together, our results support a model where Rac1 is rapidly switching between activation and inhibition at the lamellipodium tip, ensuring a local and fast control of Rac1 actions on its targets.Significance Rac1 and RhoA GTPases are molecular switches controlling the actin cytoskeletal during cell migration. WAVE, Rac1 effector during cell protrusion, is concentrated at the lamellipodium tip. But, recent biosensor imaging studies suggested that Rac1 activation occurs behind the lamellipodium, while RhoA activation is maximal at the cell edge. Using single-molecule imaging and optogentics Rac1 activation we solved this apparent contradiction. We revealed a strong correlation between Rac1 activation and transient immobilizations at the lamellipodium tip, unlike RhoA. Furthermore, we demonstrated that Rac1 must be activated at the lamellipodium tip and not away from it to stimulate protrusion. Thus, fast cycling between activation and inhibition at the proximity of Rac1 targets ensures a local and fast control over Rac1 actions.Arp2/3actin related proteins 2/3Ddiffusion coefficientF-actinactin filamentsFMNL2formin-like protein-2FNfibronectinGAPGTPase-activating proteinGDIGuanine-nucleotide Dissociation InhibitorGEFGuanine-nucleotide Exchange FactorIRSp53insulin receptor tyrosine kinase substrate p53LMlamellipodiumNPFnucleation promoting factorMSDmean squared displacementPALMphotoactivation localization microscopyPSDpost synaptic densityrconfconfinement radiussptsingle protein trackingVASPvasodilator-stimulated phosphoproteinWAVEWASP-family verprolin homologue