Distinct Phosphorylation Clusters Determine the Signaling Outcome of Free Fatty Acid Receptor 4/G Protein–Coupled Receptor 120

Prihandoko, Rudi; Álvarez-Curto, Elisa; Hudson, Brian D.; Butcher, Adrian J.; Ulven, Trond; Miller, Ashley M.; Tobin, Andrew B.; Milligan, Graeme

doi:10.1124/mol.115.101949

Cited by 52 publications

(69 citation statements)

References 49 publications

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“…We recently defined the sites of agonist-regulated phosphorylation within the C-terminal tail of both mouse (m)FFA4 and human (h)FFA4 and defined that conversion of these serine and threonine residues to alanines produces phosphorylation-deficient (PD) forms of the receptor orthologs (21, 22). We also recently proposed that detection of agonist-regulated GPCR phosphorylation using phospho-specific antibodies could be used as a biomarker for receptor activation (24).…”

Section: Resultsmentioning

confidence: 99%

“…We also recently proposed that detection of agonist-regulated GPCR phosphorylation using phospho-specific antibodies could be used as a biomarker for receptor activation (24). Here we used phospho-specific antibodies against the agonist-regulated phosphorylation sites Thr 347 and Ser 350 (21, 22) as a marker for FFA4 activation in genome-edited HEK293 cells. After stable expression of mFFA4-eYFP in each of parental HEK293 cells and the Gα q /Gα 11 or arrestin2/3 genome-edited cell lines and selection of individual clones, activation of mFFA4 by the agonist TUG-891 (25–27) was produced no-matter the genetic status of the cells (parental or genome-edited) (Fig.…”

Section: Resultsmentioning

confidence: 99%

“…Each of these lines was then further transfected to stably express either wild type FFA4 or a form of this receptor that cannot be phosphorylated in response to an agonist ligand because each of the residues in the C-terminal tail that becomes phosphorylated in the wild type receptor has been mutated to alanine (21, 22). We show that either restricting interaction of FFA4 with arrestins via this mutational strategy or eliminating expression of the arrestins results in prolongation of Ca 2+ signaling via FFA4, whereas we also show that arrestins do not contribute directly to FFA4-mediated ERK1/2 MAP kinase phosphorylation/activation in HEK293 cells.…”

Section: Introductionmentioning

confidence: 99%

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Targeted Elimination of G Proteins and Arrestins Defines Their Specific Contributions to Both Intensity and Duration of G Protein-coupled Receptor Signaling

Álvarez-Curto

Inoue

Jenkins

et al. 2016

Journal of Biological Chemistry

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152

170

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G protein-coupled receptors (GPCRs) can initiate intracellular signaling cascades by coupling to an array of heterotrimeric G proteins and arrestin adaptor proteins. Understanding the contribution of each of these coupling options to GPCR signaling has been hampered by a paucity of tools to selectively perturb receptor function. Here we employ CRISPR/Cas9 genome editing to eliminate selected G proteins (Gαq and Gα11) or arrestin2 and arrestin3 from HEK293 cells together with the elimination of receptor phosphorylation sites to define the relative contribution of G proteins, arrestins, and receptor phosphorylation to the signaling outcomes of the free fatty acid receptor 4 (FFA4). A lack of FFA4-mediated elevation of intracellular Ca2+ in Gαq/Gα11-null cells and agonist-mediated receptor internalization in arrestin2/3-null cells confirmed previously reported canonical signaling features of this receptor, thereby validating the genome-edited HEK293 cells. FFA4-mediated ERK1/2 activation was totally dependent on Gq/11 but intriguingly was substantially enhanced for FFA4 receptors lacking sites of regulated phosphorylation. This was not due to a simple lack of desensitization of Gq/11 signaling because the Gq/11-dependent calcium response was desensitized by both receptor phosphorylation and arrestin-dependent mechanisms, whereas a substantially enhanced ERK1/2 response was only observed for receptors lacking phosphorylation sites and not in arrestin2/3-null cells. In conclusion, we validate CRISPR/Cas9 engineered HEK293 cells lacking Gq/11 or arrestin2/3 as systems for GPCR signaling research and employ these cells to reveal a previously unappreciated interplay of signaling pathways where receptor phosphorylation can impact on ERK1/2 signaling through a mechanism that is likely independent of arrestins.

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Section: Resultsmentioning

confidence: 99%

Section: Resultsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Targeted Elimination of G Proteins and Arrestins Defines Their Specific Contributions to Both Intensity and Duration of G Protein-coupled Receptor Signaling

Álvarez-Curto

Inoue

Jenkins

et al. 2016

Journal of Biological Chemistry

Self Cite

152

170

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show abstract

“…These changes in receptor conformation are detected by G protein-coupled receptor kinases (GRKs), resulting in specific phosphorylation patterns at receptor intracellular domains. Quantitative mass spectrometry approaches, combined with phosphospecific antibodies, have shown that ligand-induced receptor phosphorylation is tissue and ligand specific and can be associated with specific signaling cascades; this supports a phosphorylation barcode hypothesis (Butcher et al, 2011;Liggett, 2011;Nobles et al, 2011;Prihandoko et al, 2016). Receptor phosphorylation is recognized by b-arrestins, which are recruited to the plasma membrane and sterically hinder G protein association while initiating b-arrestin-mediated internalization and signaling (Nobles et al, 2011;Liggett, 2011).…”

Section: Cb 1 Rs and B-arrestin-mediated Signalingmentioning

confidence: 92%

The Multiple Waves of Cannabinoid 1 Receptor Signaling

Nogueras-Ortiz

Yudowski

2016

Mol Pharmacol

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The cannabinoid 1 receptor (CB 1 R) is one of the most abundant G protein-coupled receptors (GPCRs) in the central nervous system, with key roles during neurotransmitter release and synaptic plasticity. Upon ligand activation, CB 1 Rs may signal in three different spatiotemporal waves. The first wave, which is transient (,10 minutes) and initiated by heterotrimeric G proteins, is followed by a second wave (.5 minutes) that is mediated by b-arrestins. The third and final wave occurs at intracellular compartments and could be elicited by G proteins or b-arrestins. This complexity presents multiple challenges, including the correct classification of receptor ligands, the identification of the signaling pathways regulated by each wave, and the underlying molecular mechanisms and physiologic impacts of these waves. Simultaneously, it provides new opportunities to harness the therapeutic potential of the cannabinoid system and other GPCRs. Over the last several years, we have significantly expanded our understanding of the mechanisms and pathways downstream from the CB 1 R. The identification of receptor mutations that can bias signaling to specific pathways and the use of siRNA technology have been key tools to identifying which signaling cascades are controlled by G proteins or b-arrestins. Here, we review our current knowledge on CB 1 R signaling, with particular emphasis on the mechanisms and cascades mediated by b-arrestins downstream from the CB 1 R.

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“…These bar-codes are finely tuned and define which signaling cascades are activated, thus opening up a spectrum of possibilities frequently defined as functional selectivity or ligand bias (Liggett, 2011; Nobles et al, 2011; Prihandoko et al, 2016). However, careful consideration must be taken when interpreting results obtained from heterologous systems, particularly when signaling can be significantly affected (biased) by the different levels of protein expression across different cell types (Bosier et al, 2010; Atwood et al, 2011; Straiker et al, 2012).…”

Section: The Endocannabinoid System In the Cnsmentioning

confidence: 99%

Cannabinoid Receptors in the Central Nervous System: Their Signaling and Roles in Disease

Kendall

Yudowski

2017

Front. Cell. Neurosci.

236

208

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The identification and cloning of the two major cannabinoid (CB1 and CB2) receptors together with the discovery of their endogenous ligands in the late 80s and early 90s, resulted in a major effort aimed at understanding the mechanisms and physiological roles of the endocannabinoid system (ECS). Due to its expression and localization in the central nervous system (CNS), the CB1 receptor together with its endogenous ligands (endocannabinoids (eCB)) and the enzymes involved in their synthesis and degradation, has been implicated in multiple pathophysiological events ranging from memory deficits to neurodegenerative disorders among others. In this review, we will provide a general overview of the ECS with emphasis on the CB1 receptor in health and disease. We will describe our current understanding of the complex aspects of receptor signaling and trafficking, including the non-canonical signaling pathways such as those mediated by β-arrestins within the context of functional selectivity and ligand bias. Finally, we will highlight some of the disorders in which CB1 receptors have been implicated. Significant knowledge has been achieved over the last 30 years. However, much more research is still needed to fully understand the complex roles of the ECS, particularly in vivo and to unlock its true potential as a source of therapeutic targets.

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Distinct Phosphorylation Clusters Determine the Signaling Outcome of Free Fatty Acid Receptor 4/G Protein–Coupled Receptor 120

Cited by 52 publications

References 49 publications

Targeted Elimination of G Proteins and Arrestins Defines Their Specific Contributions to Both Intensity and Duration of G Protein-coupled Receptor Signaling

Targeted Elimination of G Proteins and Arrestins Defines Their Specific Contributions to Both Intensity and Duration of G Protein-coupled Receptor Signaling

The Multiple Waves of Cannabinoid 1 Receptor Signaling

Cannabinoid Receptors in the Central Nervous System: Their Signaling and Roles in Disease

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