Dynamics of the formation of flat clathrin lattices in response to growth factor stimulus.

Clathrin assemblies on the cell membrane are critical for endocytosis and signal transduction in cells. Specifically, -shaped clathrin assemblies function as the coat of endocytic vesicles, while flat clathrin assemblies, also known as flat clathrin lattices, serve as signaling hubs for various signaling pathways. Multiple flat clathrin lattices exist on the cell membrane, and these lattices grow after epidermal growth factor stimulation (EGF) and then return to baseline. In this work, we used a particle-based model to simulate the assembly and disassembly of flat clathrin lattices to capture these dynamics. We found that the formation of flat clathrin lattices is highly dynamic, that is, cluster number, size and dwelling time often change even in the absence of any stimulus. Moreover, these key features are affected by adaptor protein 2 (AP-2) number, clathrin-clathrin binding rate, and clathrin diffusion coefficient. Specifically, an increase in AP-2 number leads to the transition from no cluster, short-lasting multiple small clusters, to a long-lasting single giant cluster. An increased clathrin-clathrin binding rate or decreased clathrin diffusion coefficient both result in an increased cluster number, reduced cluster size, and shortened dwelling time. Furthermore, we also predicted that under EGF stimulation, simultaneous changes in the AP-2 number, the clathrin-clathrin binding rate, and the clathrin diffusion coefficient can reproduce the experimentally observed trend of FCLs: an increase in cluster number and size in the first 30 minutes, followed by a decrease after 30 minutes. These findings reveal kinetic mechanisms underlying the formation of multiple FCLs and how EGF regulates FCL dynamics.