Phosphoproteomic analysis of protease-activated receptor-1 biased signaling reveals unique modulators of endothelial barrier function

Abstract: Thrombin, a procoagulant protease, cleaves and activates protease-activated receptor-1 (PAR1) to promote inflammatory responses and endothelial dysfunction. In contrast, activated protein C (APC), an anticoagulant protease, activates PAR1 through a distinct cleavage site and promotes anti-inflammatory responses, prosurvival, and endothelial barrier stabilization. The distinct tethered ligands formed through cleavage of PAR1 by thrombin versus APC result in unique active receptor conformations that bias PAR1 si… Show more

“…Phosphoproteomics is an alternative approach to understand how GPCR activation changes kinase and phosphatase activity in the cell. One advantage to phosphoproteomics is that it can be used to detect and identify thousands of phosphosites; thus, examining GPCR activity from the “cellular perspective.” For example, GPCR activation is estimated to change 1–10% of all phosphorylation sites in the cell 46–49 . As a comparison, an estimated 16–20% of phosphosites can be regulated upon receptor tyrosine kinase (RTK) stimulation 50,51 …”

“…A more recent study examined how the cellular phosphoproteome was remodeled by activation of the protease‐activated receptor‐1 (PAR1) with thrombin or anticoagulant protease (APC) 49 . Thrombin cleavage of PAR1 causes coupling to Gα12/13, Gαq, and β‐arrestin while APC causes PAR1 to couple to β‐arrestin 58–61 .…”

“…Thrombin cleavage of PAR1 causes coupling to Gα12/13, Gαq, and β‐arrestin while APC causes PAR1 to couple to β‐arrestin 58–61 . Phosphoproteomic comparison of PAR1 signaling in endothelial cell derived EA.hy926 cells revealed broadly different targets of thrombin and APC‐induced activity 49 . Targets of thrombin activated PAR1 signaling were enriched in proteins linked to endothelial barrier function and adherens junctions while APC‐induced signaling modulated phosphorylation of proteins linked to gene transcription 49 .…”

“…Phosphoproteomic comparison of PAR1 signaling in endothelial cell derived EA.hy926 cells revealed broadly different targets of thrombin and APC‐induced activity 49 . Targets of thrombin activated PAR1 signaling were enriched in proteins linked to endothelial barrier function and adherens junctions while APC‐induced signaling modulated phosphorylation of proteins linked to gene transcription 49 . Additionally, APC modulated a much smaller number of phosphosites than the full agonist thrombin 47,49 .…”

“…Targets of thrombin activated PAR1 signaling were enriched in proteins linked to endothelial barrier function and adherens junctions while APC‐induced signaling modulated phosphorylation of proteins linked to gene transcription 49 . Additionally, APC modulated a much smaller number of phosphosites than the full agonist thrombin 47,49 . Thus, certain biased agonist/GPCR pairs can greatly change the cellular phosphoproteome—and consequently cellular function—compared to their unbiased counterparts.…”

A cellular perspective of bias at G protein‐coupled receptors

“…Phosphoproteomics is an alternative approach to understand how GPCR activation changes kinase and phosphatase activity in the cell. One advantage to phosphoproteomics is that it can be used to detect and identify thousands of phosphosites; thus, examining GPCR activity from the “cellular perspective.” For example, GPCR activation is estimated to change 1–10% of all phosphorylation sites in the cell 46–49 . As a comparison, an estimated 16–20% of phosphosites can be regulated upon receptor tyrosine kinase (RTK) stimulation 50,51 …”

“…A more recent study examined how the cellular phosphoproteome was remodeled by activation of the protease‐activated receptor‐1 (PAR1) with thrombin or anticoagulant protease (APC) 49 . Thrombin cleavage of PAR1 causes coupling to Gα12/13, Gαq, and β‐arrestin while APC causes PAR1 to couple to β‐arrestin 58–61 .…”

“…Thrombin cleavage of PAR1 causes coupling to Gα12/13, Gαq, and β‐arrestin while APC causes PAR1 to couple to β‐arrestin 58–61 . Phosphoproteomic comparison of PAR1 signaling in endothelial cell derived EA.hy926 cells revealed broadly different targets of thrombin and APC‐induced activity 49 . Targets of thrombin activated PAR1 signaling were enriched in proteins linked to endothelial barrier function and adherens junctions while APC‐induced signaling modulated phosphorylation of proteins linked to gene transcription 49 .…”

“…Phosphoproteomic comparison of PAR1 signaling in endothelial cell derived EA.hy926 cells revealed broadly different targets of thrombin and APC‐induced activity 49 . Targets of thrombin activated PAR1 signaling were enriched in proteins linked to endothelial barrier function and adherens junctions while APC‐induced signaling modulated phosphorylation of proteins linked to gene transcription 49 . Additionally, APC modulated a much smaller number of phosphosites than the full agonist thrombin 47,49 .…”

“…Targets of thrombin activated PAR1 signaling were enriched in proteins linked to endothelial barrier function and adherens junctions while APC‐induced signaling modulated phosphorylation of proteins linked to gene transcription 49 . Additionally, APC modulated a much smaller number of phosphosites than the full agonist thrombin 47,49 . Thus, certain biased agonist/GPCR pairs can greatly change the cellular phosphoproteome—and consequently cellular function—compared to their unbiased counterparts.…”

A cellular perspective of bias at G protein‐coupled receptors

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Phosphoproteomic analysis of thrombin- and p38 MAPK-regulated signaling networks in endothelial cells