Gβγ is a direct regulator of endogenous p101/p110γ and p84/p110γ PI3Kγ complexes in mouse neutrophils

The PI3Kγ isoform is activated by Gi-coupled GPCRs in myeloid cells, but the extent to which the two endogenous complexes of PI3Kγ, p101/p110γ and p84/p110γ, receive direct regulation through Gβγ or indirect regulation through RAS and the sufficiency of those inputs is controversial or unclear. We g...

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Veröffentlicht in:	Science signaling 2020-11, Vol.13 (656)
Hauptverfasser:	Rynkiewicz, Natalie K, Anderson, Karen E, Suire, Sabine, Collins, Daniel M, Karanasios, Eleftherios, Vadas, Oscar, Williams, Roger, Oxley, David, Clark, Jonathan, Stephens, Len R, Hawkins, Phillip T
Format:	Artikel
Sprache:	eng
Schlagworte:	Agonists Animal models Binding sites Cell activation Formyl peptides G protein-coupled receptors Inflammation Leukocyte migration Leukocytes (neutrophilic) Mutation Myeloid cells Neutrophils Peritonitis Phosphatidylinositol 3,4,5-triphosphate Regulation Regulatory subunits Signaling
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creator	Rynkiewicz, Natalie K Anderson, Karen E Suire, Sabine Collins, Daniel M Karanasios, Eleftherios Vadas, Oscar Williams, Roger Oxley, David Clark, Jonathan Stephens, Len R Hawkins, Phillip T
description	The PI3Kγ isoform is activated by Gi-coupled GPCRs in myeloid cells, but the extent to which the two endogenous complexes of PI3Kγ, p101/p110γ and p84/p110γ, receive direct regulation through Gβγ or indirect regulation through RAS and the sufficiency of those inputs is controversial or unclear. We generated mice with point mutations that prevent Gβγ binding to p110γ (RK552DD) or to p101 (VVKR777AAAA) and investigated the effects of these mutations in primary neutrophils and in mouse models of neutrophilic inflammation. Loss of Gβγ binding to p110γ substantially reduced the activation of both p101/p110γ and p84/p110γ in neutrophils by various GPCR agonists. Loss of Gβγ binding to p101 caused more variable effects, depending on both the agonist and cellular response, with the biggest reductions seen in PIP production by primary neutrophils in response to LTB4 and MIP-2 and in the migration of neutrophils during thioglycolate-induced peritonitis or MIP2-induced ear pouch inflammation. We also observed that p101 neutrophils showed enhanced p84-dependent ROS responses to MLP and C5a, suggesting that competition may exist between p101/p110γ and p84/p110γ for Gβγ subunits downstream of GPCR activation. GPCRs did not activate p110γ in neutrophils from mice lacking both the p101 and p84 regulatory subunits, indicating that RAS binding to p110γ is insufficient to support GPCR activation in this cell type. These findings define a direct role for Gβγ subunits in activating both of the endogenous PI3Kγ complexes and indicate that the regulatory PI3Kγ subunit biases activation toward different GPCRs.
doi_str_mv	10.1126/scisignal.aaz4003
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We generated mice with point mutations that prevent Gβγ binding to p110γ (RK552DD) or to p101 (VVKR777AAAA) and investigated the effects of these mutations in primary neutrophils and in mouse models of neutrophilic inflammation. Loss of Gβγ binding to p110γ substantially reduced the activation of both p101/p110γ and p84/p110γ in neutrophils by various GPCR agonists. Loss of Gβγ binding to p101 caused more variable effects, depending on both the agonist and cellular response, with the biggest reductions seen in PIP production by primary neutrophils in response to LTB4 and MIP-2 and in the migration of neutrophils during thioglycolate-induced peritonitis or MIP2-induced ear pouch inflammation. We also observed that p101 neutrophils showed enhanced p84-dependent ROS responses to MLP and C5a, suggesting that competition may exist between p101/p110γ and p84/p110γ for Gβγ subunits downstream of GPCR activation. GPCRs did not activate p110γ in neutrophils from mice lacking both the p101 and p84 regulatory subunits, indicating that RAS binding to p110γ is insufficient to support GPCR activation in this cell type. These findings define a direct role for Gβγ subunits in activating both of the endogenous PI3Kγ complexes and indicate that the regulatory PI3Kγ subunit biases activation toward different GPCRs.</description><identifier>ISSN: 1945-0877</identifier><identifier>EISSN: 1937-9145</identifier><identifier>DOI: 10.1126/scisignal.aaz4003</identifier><identifier>PMID: 33144519</identifier><language>eng</language><publisher>United States: The American Association for the Advancement of Science</publisher><subject>Agonists ; Animal models ; Binding sites ; Cell activation ; Formyl peptides ; G protein-coupled receptors ; Inflammation ; Leukocyte migration ; Leukocytes (neutrophilic) ; Mutation ; Myeloid cells ; Neutrophils ; Peritonitis ; Phosphatidylinositol 3,4,5-triphosphate ; Regulation ; Regulatory subunits ; Signaling</subject><ispartof>Science signaling, 2020-11, Vol.13 (656)</ispartof><rights>Copyright © 2020 The Authors, some rights reserved; exclusive licensee American Association for the Advancement of Science. 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We generated mice with point mutations that prevent Gβγ binding to p110γ (RK552DD) or to p101 (VVKR777AAAA) and investigated the effects of these mutations in primary neutrophils and in mouse models of neutrophilic inflammation. Loss of Gβγ binding to p110γ substantially reduced the activation of both p101/p110γ and p84/p110γ in neutrophils by various GPCR agonists. Loss of Gβγ binding to p101 caused more variable effects, depending on both the agonist and cellular response, with the biggest reductions seen in PIP production by primary neutrophils in response to LTB4 and MIP-2 and in the migration of neutrophils during thioglycolate-induced peritonitis or MIP2-induced ear pouch inflammation. We also observed that p101 neutrophils showed enhanced p84-dependent ROS responses to MLP and C5a, suggesting that competition may exist between p101/p110γ and p84/p110γ for Gβγ subunits downstream of GPCR activation. GPCRs did not activate p110γ in neutrophils from mice lacking both the p101 and p84 regulatory subunits, indicating that RAS binding to p110γ is insufficient to support GPCR activation in this cell type. 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We generated mice with point mutations that prevent Gβγ binding to p110γ (RK552DD) or to p101 (VVKR777AAAA) and investigated the effects of these mutations in primary neutrophils and in mouse models of neutrophilic inflammation. Loss of Gβγ binding to p110γ substantially reduced the activation of both p101/p110γ and p84/p110γ in neutrophils by various GPCR agonists. Loss of Gβγ binding to p101 caused more variable effects, depending on both the agonist and cellular response, with the biggest reductions seen in PIP production by primary neutrophils in response to LTB4 and MIP-2 and in the migration of neutrophils during thioglycolate-induced peritonitis or MIP2-induced ear pouch inflammation. We also observed that p101 neutrophils showed enhanced p84-dependent ROS responses to MLP and C5a, suggesting that competition may exist between p101/p110γ and p84/p110γ for Gβγ subunits downstream of GPCR activation. GPCRs did not activate p110γ in neutrophils from mice lacking both the p101 and p84 regulatory subunits, indicating that RAS binding to p110γ is insufficient to support GPCR activation in this cell type. These findings define a direct role for Gβγ subunits in activating both of the endogenous PI3Kγ complexes and indicate that the regulatory PI3Kγ subunit biases activation toward different GPCRs.</abstract><cop>United States</cop><pub>The American Association for the Advancement of Science</pub><pmid>33144519</pmid><doi>10.1126/scisignal.aaz4003</doi><orcidid>https://orcid.org/0000-0003-3172-0222</orcidid><orcidid>https://orcid.org/0000-0002-6787-8534</orcidid><orcidid>https://orcid.org/0000-0002-2771-3487</orcidid><orcidid>https://orcid.org/0000-0003-3511-6479</orcidid><orcidid>https://orcid.org/0000-0002-7394-6660</orcidid><orcidid>https://orcid.org/0000-0001-7754-4207</orcidid><orcidid>https://orcid.org/0000-0002-6979-0464</orcidid><oa>free_for_read</oa></addata></record>
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subjects	Agonists Animal models Binding sites Cell activation Formyl peptides G protein-coupled receptors Inflammation Leukocyte migration Leukocytes (neutrophilic) Mutation Myeloid cells Neutrophils Peritonitis Phosphatidylinositol 3,4,5-triphosphate Regulation Regulatory subunits Signaling
title	Gβγ is a direct regulator of endogenous p101/p110γ and p84/p110γ PI3Kγ complexes in mouse neutrophils
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