Molecular dissection of the human A3 adenosine receptor coupling with β-arrestin2

Jolien Storme; Annelies Cannaert; Kathleen Van Craenenbroeck; Christophe P Stove

doi:10.1016/j.bcp.2018.01.008

Molecular dissection of the human A₃ adenosine receptor coupling with β-arrestin2

Biochem Pharmacol. 2018 Feb:148:298-307. doi: 10.1016/j.bcp.2018.01.008. Epub 2018 Jan 5.

Authors

Jolien Storme¹, Annelies Cannaert¹, Kathleen Van Craenenbroeck¹, Christophe P Stove²

Affiliations

¹ Laboratory of Toxicology, Department of Bioanalysis, Faculty of Pharmaceutical Sciences, Ghent University, Ottergemsesteenweg 460, 9000 Ghent, Belgium.
² Laboratory of Toxicology, Department of Bioanalysis, Faculty of Pharmaceutical Sciences, Ghent University, Ottergemsesteenweg 460, 9000 Ghent, Belgium. Electronic address: Christophe.Stove@UGent.be.

PMID: 29309765
DOI: 10.1016/j.bcp.2018.01.008

Abstract

Besides classical G protein coupling, G protein-coupled receptors (GPCRs) are nowadays well known to show significant signalling via other adaptor proteins, such as β-arrestin2 (βarr2). The elucidation of the molecular mechanism of the GPCR-βarr2 interaction is a prerequisite for the structure-activity based design of biased ligands, which introduces a new chapter in drug discovery. The general mechanism of the interaction is believed to rely on phosphorylation sites, exposed upon agonist binding. However, it is not known whether this mechanism is universal throughout the GPCR family or if GPCR-specific patterns are involved. In recent years, promising orally active agonists for the human A₃ adenosine receptor (A₃AR), a GPCR highly expressed in inflammatory and cancer cells, have been evaluated in clinical trials for the treatment of rheumatoid arthritis, psoriasis, and hepatocellular carcinoma. In this study, the effect of cytoplasmic modifications of the A₃AR on βarr2 recruitment was evaluated in transiently transfected HEK293T cells, using a live-cell split-reporter system (NanoBit®, Promega), based on the structural complementation of NanoLuc luciferase, allowing real-time βarr2 monitoring. The A₃AR-selective reference agonist 2-Cl-IB-MECA yielded a robust, concentration dependent (5 nM-1 µM) recruitment of βarr2 (logEC50: -7.798 ± 0.076). The role of putative phosphorylation sites, located in the C-terminal part and cytoplasmic loops, and the role of the 'DRY' motif was evaluated. It was shown that the A₃AR C-terminus was dispensable for βarr2 recruitment. This contrasts with studies in the past for the rat A₃AR, which pointed at crucial C-terminal phosphorylation sites. When combining truncation of the A₃AR with modification of the 'DRY' motif to 'AAY', the βarr2 recruitment was drastically reduced. Recruitment could be partly rescued by back-mutation to 'NQY', or by extending the C-terminus again. In conclusion, other parts of the human A₃AR, either cytosolic or exposed upon receptor activation, rather than the C-terminus alone, are responsible for βarr2 recruitment in a complementary or synergistic way.

Keywords: A(3) adenosine receptor; Functional complementation; Live-cell reporter assay; Nanoluciferase; β-Arrestin2.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Adenosine / analogs & derivatives
Adenosine / pharmacology
Adenosine A3 Receptor Agonists / pharmacology
Gene Expression Regulation / drug effects
Genetic Complementation Test
HEK293 Cells
Humans
Mutation
Receptor, Adenosine A3 / metabolism*
beta-Arrestin 2 / metabolism*

Substances

Adenosine A3 Receptor Agonists
Receptor, Adenosine A3
beta-Arrestin 2
Adenosine
2-chloro-N(6)-(3-iodobenzyl)adenosine-5'-N-methyluronamide