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Elements of the Endomucin Extracellular Domain Essential for VEGF-Induced VEGFR2 Activity
Elements of the Endomucin Extracellular Domain Essential for VEGF-Induced VEGFR2 Activity
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Elements of the Endomucin Extracellular Domain Essential for VEGF-Induced VEGFR2 Activity
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Elements of the Endomucin Extracellular Domain Essential for VEGF-Induced VEGFR2 Activity
Elements of the Endomucin Extracellular Domain Essential for VEGF-Induced VEGFR2 Activity

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Elements of the Endomucin Extracellular Domain Essential for VEGF-Induced VEGFR2 Activity
Elements of the Endomucin Extracellular Domain Essential for VEGF-Induced VEGFR2 Activity
Journal Article

Elements of the Endomucin Extracellular Domain Essential for VEGF-Induced VEGFR2 Activity

2020
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Overview
Endomucin (EMCN) is the type I transmembrane glycoprotein, mucin-like component of the endothelial cell glycocalyx. We have previously shown that EMCN is necessary for vascular endothelial growth factor (VEGF)-induced VEGF receptor 2 (VEGFR2) internalization and downstream signaling. To explore the structural components of EMCN that are necessary for its function and the molecular mechanism of EMCN in VEGF-induced endothelial functions, we generated a series of mouse EMCN truncation mutants and examined their ability to rescue VEGF-induced endothelial functions in human primary endothelial cells (EC) in which endogenous EMCN had been knocked down using siRNA. Expression of the mouse full-length EMCN (FL EMCN) and the extracellular domain truncation mutants ∆21-81 EMCN and ∆21-121 EMCN, but not the shortest mutant ∆21-161 EMCN, successfully rescued the VEGF-induced EC migration, tube formation, and proliferation. ∆21-161 EMCN failed to interact with VEGFR2 and did not facilitate VEGFR2 internalization. Deletion of COSMC (C1GalT1C1) revealed that the abundant mucin-type O-glycans were not required for its VEGFR2-related functions. Mutation of the two N-glycosylation sites on ∆21-121 EMCN abolished its interaction with VEGFR2 and its function in VEGFR2 internalization. These results reveal ∆21-121 EMCN as the minimal extracellular domain sufficient for VEGFR2-mediated endothelial function and demonstrate an important role for N-glycosylation in VEGFR2 interaction, internalization, and angiogenic activity.