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The GPIbα intracellular tail - role in transducing VWF- and collagen/GPVI-mediated signaling.
Constantinescu-Bercu, Adela; Wang, Yuxiao A; Woollard, Kevin J; Mangin, Pierre; Vanhoorelbeke, Karen; Crawley, James T B; Salles-Crawley, Isabelle I.
Affiliation
  • Constantinescu-Bercu A; Centre for Haematology, Department of Immunology and Inflammation, Imperial College London, London, UK.
  • Wang YA; Centre for Haematology, Department of Immunology and Inflammation, Imperial College London, London, UK.
  • Woollard KJ; Centre for Inflammatory Disease, Department of Immunology and Inflammation, Imperial College London, London, UK.
  • Mangin P; Université de Strasbourg, INSERM, EFS Grand-Est, BPPS UMR-S 1255, FMTS, Strasbourg, France.
  • Vanhoorelbeke K; Laboratory for Thrombosis Research, KU Leuven, Kortrijk, Belgium.
  • Crawley JTB; Centre for Haematology, Department of Immunology and Inflammation, Imperial College London, London, UK.
  • Salles-Crawley II; Centre for Haematology, Department of Immunology and Inflammation, Imperial College London, London, UK. i.salles@imperial.ac.uk.
Haematologica ; 107(4): 933-946, 2022 04 01.
Article in En | MEDLINE | ID: mdl-34134470
The GPIbT-VWF A1 domain interaction is essential for platelet tethering under high shear. Synergy between GPIbα and GPVI signaling machineries has been suggested previously, however its molecular mechanism remains unclear. We generated a novel GPIbα transgenic mouse (GpIbαΔsig/Δsig) by CRISPR-Cas9 technology to delete the last 24 residues of the GPIbα intracellular tail that harbors the 14-3-3 and phosphoinositide-3 kinase binding sites. GPIbαΔsig/Δsig platelets bound VWF normally under flow. However, they formed fewer filopodia on VWF/botrocetin in the presence of a oIIbI3 blocker, demonstrating that despite normal ligand binding, VWF-dependent signaling is diminished. Activation of GpIbαΔsig/Δsig platelets with ADP and thrombin was normal, but GpIbαΔsig/Δsig platelets stimulated with collagen-related-peptide (CRP) exhibited markedly decreased P-selectin exposure and eIIbI3 activation, suggesting a role for the GpIbaaintracellular tail in GPVI-mediated signaling. Consistent with this, while haemostasis was normal in GPIbαΔsig/Δsig mice, diminished tyrosine-phosphorylation, (particularly pSYK) was detected in CRP-stimulated GpIbαΔsig/Δsig platelets as well as reduced platelet spreading on CRP. Platelet responses to rhodocytin were also affected in GpIbαΔsig/Δsig platelets but to a lesser extent than those with CRP. GpIbαΔsig/Δsig platelets formed smaller aggregates than wild-type platelets on collagen-coated microchannels at low, medium and high shear. In response to both VWF and collagen binding, flow assays performed with plasma-free blood or in the presence of bIIbI3- or GPVI-blockers suggested reduced bIIbI3 activation contributes to the phenotype of the GpIbαΔsig/Δsig platelets. Together, these results reveal a new role for the intracellular tail of GPIbiiin transducing both VWF-GPIbGGand collagen-GPVI signaling events in platelets.
Subject(s)

Full text: 1 Collection: 01-internacional Database: MEDLINE Main subject: Blood Platelets / Von Willebrand Factor Limits: Animals / Humans Language: En Journal: Haematologica Year: 2022 Document type: Article Country of publication: Italy

Full text: 1 Collection: 01-internacional Database: MEDLINE Main subject: Blood Platelets / Von Willebrand Factor Limits: Animals / Humans Language: En Journal: Haematologica Year: 2022 Document type: Article Country of publication: Italy