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C-terminal phosphorylation modulates ERM-1 localization and dynamics to control cortical actin organization and support lumen formation during <i>Caenorhabditis</i>   <i>elegans</i> development

João J. Ramalho, Jorian J. Sepers, Ophélie Nicolle, Ruben Schmidt, Janine Cravo, Grégoire Michaux, Mike Boxem

2020Development41 citationsDOIOpen Access PDF

Abstract

ABSTRACT ERM proteins are conserved regulators of cortical membrane specialization that function as membrane-actin linkers and molecular hubs. The activity of ERM proteins requires a conformational switch from an inactive cytoplasmic form into an active membrane- and actin-bound form, which is thought to be mediated by sequential PIP2 binding and phosphorylation of a conserved C-terminal threonine residue. Here, we use the single Caenorhabditis elegans ERM ortholog, ERM-1, to study the contribution of these regulatory events to ERM activity and tissue formation in vivo. Using CRISPR/Cas9-generated erm-1 mutant alleles, we demonstrate that a PIP2-binding site is crucially required for ERM-1 function. By contrast, dynamic regulation of C-terminal T544 phosphorylation is not essential but modulates ERM-1 apical localization and dynamics in a tissue-specific manner, to control cortical actin organization and support lumen formation in epithelial tubes. Our work highlights the dynamic nature of ERM protein regulation during tissue morphogenesis and the importance of C-terminal phosphorylation in fine-tuning ERM activity in a tissue-specific context.

Topics & Concepts

BiologyCaenorhabditis elegansCell biologyTerminal (telecommunication)PhosphorylationLumen (anatomy)ActinBiochemistryGeneComputer scienceTelecommunicationsGenetics, Aging, and Longevity in Model OrganismsCellular Mechanics and InteractionsGene Regulatory Network Analysis
C-terminal phosphorylation modulates ERM-1 localization and dynamics to control cortical actin organization and support lumen formation during <i>Caenorhabditis</i>   <i>elegans</i> development | Litcius