Biased receptor signalling and intracellular trafficking profiles of structurally distinct formylpeptide receptor 2 agonists

Cheng Peng; Elizabeth A Vecchio; Anh T N Nguyen; Mia De Seram; Ruby Tang; Peter Keov; Owen L Woodman; Yung-Chih Chen; Jonathan Baell; Lauren T May; Peishen Zhao; Rebecca H Ritchie; Cheng Xue Qin

doi:10.1111/bph.17310

Biased receptor signalling and intracellular trafficking profiles of structurally distinct formylpeptide receptor 2 agonists

Br J Pharmacol. 2024 Nov;181(22):4677-4692. doi: 10.1111/bph.17310. Epub 2024 Aug 18.

Authors

Affiliations

¹ Drug Discovery Biology, Monash Institute of Pharmaceutical Sciences, Monash University, Melbourne, Victoria, Australia.
² Monash Victorian Heart Institute, Blackburn Road Clayton, Monash University, Melbourne, Victoria, Australia.
³ Medicinal Chemistry, Monash Institute of Pharmaceutical Sciences, Monash University, Melbourne, Vitoria, Australia.

PMID: 39154373
DOI: 10.1111/bph.17310

Abstract

Background: There is increasing interest in developing FPR2 agonists (compound 43, ACT-389949 and BMS-986235) as potential pro-resolving therapeutics, with ACT-389949 and BMS-986235 having entered phase I clinical development. FPR2 activation leads to diverse downstream outputs. ACT-389949 was observed to cause rapid tachyphylaxis, while BMS-986235 and compound 43 induced cardioprotective effects in preclinical models. We aim to characterise the differences in ligand-receptor engagement and downstream signalling and trafficking bias profile.

Experimental approach: Concentration-response curves to G protein dissociation, β-arrestin recruitment, receptor trafficking and second messenger signalling were generated using FPR2 ligands (BMS-986235, ACT-389949, compound 43 and WKYMVm), in HEK293A cells. Log(τ/K_A) was obtained from the operational model for bias analysis using WKYMVm as a reference ligand. Docking of FPR2 ligands into the active FPR2 cryoEM structure (PDBID: 7T6S) was performed using ICM pro software.

Key results: Bias analysis revealed that WKYMVm and ACT-389949 shared a very similar bias profile. In comparison, BMS-986235 and compound 43 displayed approximately 5- to 50-fold bias away from β-arrestin recruitment and trafficking pathways, while being 35- to 60-fold biased towards cAMP inhibition and pERK1/2. Molecular docking predicted key amino acid interactions at the FPR2 shared between WKYMVm and ACT-389949, but not with BMS-986235 and compound 43.

Conclusion and implications: In vitro characterisation demonstrated that WKYMVm and ACT-389949 differ from BMS-986235 and compound 43 in their signalling and protein coupling profile. This observation may be explained by differences in the ligand-receptor interactions. In vitro characterisation provided significant insights into identifying the desired bias profile for FPR2-based pharmacotherapy.

Keywords: Aspirin triggered lipoxin A4; FPR2; internalisation; receptor trafficking; resolution of inflammation; β‐arrestin‐2.

MeSH terms

Dose-Response Relationship, Drug
HEK293 Cells
Humans
Ligands
Molecular Docking Simulation
Protein Transport* / drug effects
Receptors, Formyl Peptide* / agonists
Receptors, Formyl Peptide* / metabolism
Receptors, Lipoxin* / agonists
Receptors, Lipoxin* / metabolism
Signal Transduction* / drug effects
beta-Arrestins / metabolism

Substances

Receptors, Formyl Peptide
Receptors, Lipoxin
FPR2 protein, human
beta-Arrestins
Ligands

Abstract

MeSH terms

Substances

Grants and funding