Identification of novel species-selective agonists of the G-protein-coupled receptor GPR35 that promote recruitment of β-arrestin-2 and activate Gα13

Jenkins, Laura; Brea, José; Smith, Nicola J.; Hudson, Brian D.; Reilly, Graeme; Bryant, Nia J.; Castro, Marián; Loza, María‐Isabel; Milligan, Graeme

doi:10.1042/bj20101287

Cited by 93 publications

(166 citation statements)

References 26 publications

(33 reference statements)

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“…mFFA4-Arrestin 3 Interaction Assay. Arrestin 3 recruitment to mFFA4 was assessed using a bioluminescence resonance energy transfer (BRET) assay (Jenkins et al, 2010;Butcher et al, 2014;Hudson et al, 2014;MacKenzie et al, 2014). Briefly, human embryonic kidney 293T (HEK293T) cells were cotransfected with arrestin 3-Renilla luciferase and eYFP-tagged receptor plasmids in a 1:4 ratio using polyethyleneimine.…”

Section: Methodsmentioning

confidence: 99%

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

et al. 2016

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It is established that long-chain free fatty acids including v-3 fatty acids mediate an array of biologic responses through members of the free fatty acid (FFA) receptor family, which includes FFA4. However, the signaling mechanisms and modes of regulation of this receptor class remain unclear. Here, we employed mass spectrometry to determine that phosphorylation of mouse (m) FFAR4 occurs at five serine and threonine residues clustered in two separable regions of the C-terminal tail, designated cluster 1 (Thr 347 , Thr 349 , and Ser 350 ) and cluster 2 (Ser 357 and Ser 361 ). Mutation of these phosphoacceptor sites to alanine completely prevented phosphorylation of mFFA4 but did not limit receptor coupling to extracellular signal regulated protein kinase 1 and 2 (ERK1/2) activation. Rather, an inhibitor of G q / 11 proteins completely prevented receptor signaling to ERK1/2. By contrast, the recruitment of arrestin 3, receptor internalization, and activation of Akt were regulated by mFFA4 phosphorylation. The analysis of mFFA4 phosphorylation-dependent signaling was extended further by selective mutations of the phosphoacceptor sites. Mutations within cluster 2 did not affect agonist activation of Akt but instead significantly compromised receptor internalization and arrestin 3 recruitment. Distinctly, mutation of the phosphoacceptor sites within cluster 1 had no effect on receptor internalization and had a less extensive effect on arrestin 3 recruitment but significantly uncoupled the receptor from Akt activation. These unique observations define differential effects on signaling mediated by phosphorylation at distinct locations. This hallmark feature supports the possibility that the signaling outcome of mFFA4 activation can be determined by the pattern of phosphorylation (phosphorylation barcode) at the C terminus of the receptor.

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Section: Methodsmentioning

confidence: 99%

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

et al. 2016

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“…Although GPR35 is indicated to be a receptor responsive to the endogenously produced tryptophan metabolite kynurenic acid (Wang et al, 2006), lack of convergence on this issue has resulted in a number of efforts to identify surrogate agonist ligands that might be used to help further define the roles of this receptor. Although a number of such ligands have been identified (Taniguchi et al, 2006;Jenkins et al, 2010;Zhao et al, 2010;Deng et al, 2012;Funke et al, 2013;Neetoo-Isseljee et al, 2013), many of these are either of modest potency and/or display markedly different potency at human and rodent orthologs of GPR35 (Jenkins et al, 2010;Funke et al, 2013;Neetoo-Isseljee et al, 2013). This has posed challenges both in efforts to define the orthosteric binding pocket of the receptor and to use rodents and cell lines derived from such animals to further explore the function of GPR35.…”

Section: Introductionmentioning

confidence: 99%

“…The antiasthma and antiallergic agents cromolyn disodium (Jenkins et al, 2010;Yang et al, 2010) and nedocromil sodium (Yang et al, 2010) were recently shown to act as moderately potent agonists of GPR35. These ligands are both di-acids with marked mirror image symmetry (Fig.…”

Section: Introductionmentioning

confidence: 99%

“…Zaprinast (Taniguchi et al, 2006;Jenkins et al, 2010Jenkins et al, , 2011 has become the standard surrogate agonist of GPR35 and, akin to zaprinast, a number of mast cell stabilizers also contain an acid bioisostere. Because zaprinast is an example of a ligand that displays marked variation in potency between rodent and human GPR35 (Taniguchi et al, 2006;Jenkins et al, 2010Jenkins et al, , 2011, this also encouraged us to also explore the contributions of a series of nonmaintained arginine residues within regions of the receptor species orthologs that are predicted to define the ligand binding pocket. Cross-species alterations of such residues provided novel insights into the binding pocket.…”

Section: Introductionmentioning

confidence: 99%

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The Antiallergic Mast Cell Stabilizers Lodoxamide and Bufrolin as the First High and Equipotent Agonists of Human and Rat GPR35

Mackenzie¹,

Caltabiano

Kent

et al. 2013

Mol Pharmacol

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Lack of high potency agonists has restricted analysis of the G protein-coupled receptor GPR35. Moreover, marked variation in potency and/or affinity of current ligands between human and rodent orthologs of GPR35 has limited their productive use in rodent models of physiology. Based on the reported modest potency of the antiasthma and antiallergic ligands cromolyn disodium and nedocromil sodium, we identified the related compounds lodoxamide and bufrolin as high potency agonists of human GPR35. Unlike previously identified high potency agonists that are highly selective for human GPR35, both lodoxamide and bufrolin displayed equivalent potency at rat GPR35. Further synthetic antiallergic ligands, either sharing features of the standard surrogate agonist zaprinast, or with lodoxamide and bufrolin, were also shown to display agonism at either human or rat GPR35. Because both lodoxamide and bufrolin are symmetric di-acids, their potential mode of binding was explored via mutagenesis based on swapping between the rat and human ortholog nonconserved arginine residues within proximity of a key conserved arginine at position 3.36. Computational modeling and ligand docking predicted the contributions of different arginine residues, other than at 3.36, in human GPR35 for these two ligands and were consistent with selective loss of potency of either bufrolin or lodoxamide at distinct arginine mutants. The computational models also suggested that bufrolin and lodoxamide would display reduced potency at a low-frequency human GPR35 single nucleotide polymorphism. This prediction was confirmed experimentally.

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“…50 Niflumic acid has also been found to be an activator of GPR (G-protein coupled receptor) 35, a protein implicated in a number of conditions including inflammatory pain, asthma, heart disease, cancer, and metabolic diseases, and regarded as a promising therapeutic target. 51 Preclinical studies have shown that morniflumate has marked anti-inflammatory activity, comparable with niflumic acid.…”

Section: Pharmacodynamic Profilementioning

confidence: 99%

Efficacy and Safety of Morniflumate for the Treatment of Symptoms Associated with Soft Tissue Inflammation

Cremonesi

Cavalieri

2015

J Int Med Res

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The effectiveness of nonsteroidal antiinflammatory drugs (NSAIDs) for the management of pain in osteoarthritis and other musculoskeletal diseases is well documented. The role of NSAIDs is less clear in the treatment of conditions involving soft tissue inflammation, including the airways, earnose-throat (ENT) system and urogenital tract. These conditions are often treated inappropriately with antibiotics. Morniflumate, the ß-morpholinoethyl ester of niflumic acid, is a member of the fenamate family of NSAIDs indicated for the treatment of inflammatory conditions (with or without pain) affecting airways, the ENT system, urogenital tract and the osteoarticular system. Morniflumate has a 30-year history of clinical use, particularly for the treatment of pain associated with paediatric ENT infection. This article reviews evidence supporting the efficacy and safety of morniflumate. Based on available evidence and the favourable tolerability profile emerging from extensive clinical use, morniflumate appears to be a valid and well-tolerated alternative to other NSAIDs, or to antibiotics, for the treatment of pain and other symptoms of soft tissue inflammation.

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Identification of novel species-selective agonists of the G-protein-coupled receptor GPR35 that promote recruitment of β-arrestin-2 and activate Gα13

Cited by 93 publications

References 26 publications

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

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

The Antiallergic Mast Cell Stabilizers Lodoxamide and Bufrolin as the First High and Equipotent Agonists of Human and Rat GPR35

Efficacy and Safety of Morniflumate for the Treatment of Symptoms Associated with Soft Tissue Inflammation

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