| Literature DB >> 33202251 |
Eva Marie Pfeil1, Julian Brands1, Nicole Merten2, Timo Vögtle3, Maddalena Vescovo2, Ulrike Rick2, Ina-Maria Albrecht2, Nina Heycke2, Kouki Kawakami4, Yuki Ono4, Francois Marie Ngako Kadji4, Suzune Hiratsuka4, Junken Aoki4, Felix Häberlein1, Michaela Matthey5, Jaspal Garg6, Stephanie Hennen2, Marie-Lise Jobin7, Kerstin Seier7, Davide Calebiro8, Alexander Pfeifer9, Akos Heinemann10, Daniela Wenzel5, Gabriele M König11, Bernhard Nieswandt3, Bernd K Fleischmann9, Asuka Inoue4, Katharina Simon12, Evi Kostenis13.
Abstract
Mechanisms that control mobilization of cytosolic calcium [Ca2+]i are key for regulation of numerous eukaryotic cell functions. One such paradigmatic mechanism involves activation of phospholipase Cβ (PLCβ) enzymes by G protein βγ subunits from activated Gαi-Gβγ heterotrimers. Here, we report identification of a master switch to enable this control for PLCβ enzymes in living cells. We find that the Gαi-Gβγ-PLCβ-Ca2+ signaling module is entirely dependent on the presence of active Gαq. If Gαq is pharmacologically inhibited or genetically ablated, Gβγ can bind to PLCβ but does not elicit Ca2+ signals. Removal of an auto-inhibitory linker that occludes the active site of the enzyme is required and sufficient to empower "stand-alone control" of PLCβ by Gβγ. This dependence of Gi-Gβγ-Ca2+ on Gαq places an entire signaling branch of G-protein-coupled receptors (GPCRs) under hierarchical control of Gq and changes our understanding of how Gi-GPCRs trigger [Ca2+]i via PLCβ enzymes.Entities:
Keywords: Ca(2+) signaling; FR900359; GPCR; GPR17; Gi; Gq; PTX; heterotrimeric G protein; phospholipase Cβ; real-time BRET-based IP(3) biosensor
Year: 2020 PMID: 33202251 DOI: 10.1016/j.molcel.2020.10.027
Source DB: PubMed Journal: Mol Cell ISSN: 1097-2765 Impact factor: 17.970