SNAP-tag-enabled super-resolution imaging reveals constitutive and agonist-dependent trafficking of GPR56 in pancreatic β-cells

OBJECTIVE: Members of the adhesion G protein-coupled receptor (aGPCR) subfamily are important actors in metabolic processes, with GPR56 (ADGRG1) emerging as a possible target for type 2 diabetes therapy. GPR56 can be activated by collagen III, its endogenous ligand, and by a synthetic seven amino-ac...

Descripción completa

Detalles Bibliográficos
Autores principales: Olaniru, Oladapo E., Cheng, Jordan, Ast, Julia, Arvaniti, Anastasia, Atanes, Patricio, Huang, Guo C., King, Aileen J.F., Jones, Peter M., Broichhagen, Johannes, Hodson, David J., Persaud, Shanta J.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Elsevier 2021
Materias:
Original Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8326393/
https://www.ncbi.nlm.nih.gov/pubmed/34224919
http://dx.doi.org/10.1016/j.molmet.2021.101285
_version_ 1783731807107153920
author Olaniru, Oladapo E.
Cheng, Jordan
Ast, Julia
Arvaniti, Anastasia
Atanes, Patricio
Huang, Guo C.
King, Aileen J.F.
Jones, Peter M.
Broichhagen, Johannes
Hodson, David J.
Persaud, Shanta J.
author_facet Olaniru, Oladapo E.
Cheng, Jordan
Ast, Julia
Arvaniti, Anastasia
Atanes, Patricio
Huang, Guo C.
King, Aileen J.F.
Jones, Peter M.
Broichhagen, Johannes
Hodson, David J.
Persaud, Shanta J.
author_sort Olaniru, Oladapo E.
collection PubMed
description OBJECTIVE: Members of the adhesion G protein-coupled receptor (aGPCR) subfamily are important actors in metabolic processes, with GPR56 (ADGRG1) emerging as a possible target for type 2 diabetes therapy. GPR56 can be activated by collagen III, its endogenous ligand, and by a synthetic seven amino-acid peptide (TYFAVLM; P7) contained within the GPR56 Stachel sequence. However, the mechanisms regulating GPR56 trafficking dynamics and agonist activities are not yet clear. METHODS: Here, we introduced SNAPf-tag into the N-terminal segment of GPR56 to monitor GPR56 cellular activity in situ. Confocal and super-resolution microscopy were used to investigate the trafficking pattern of GPR56 in native MIN6 β-cells and in MIN6 β-cells where GPR56 had been deleted by CRISPR-Cas9 gene editing. Insulin secretion, changes in intracellular calcium, and β-cell apoptosis were determined by radioimmunoassay, single-cell calcium microfluorimetry, and measuring caspase 3/7 activities, respectively, in MIN6 β-cells and human islets. RESULTS: SNAP-tag labelling indicated that GPR56 predominantly underwent constitutive internalisation in the absence of an exogenous agonist, unlike GLP-1R. Collagen III further stimulated GPR56 internalisation, whereas P7 was without significant effect. The overexpression of GPR56 in MIN6 β-cells did not affect insulin secretion. However, it was associated with reduced β-cell apoptosis, while the deletion of GPR56 made MIN6 β-cells more susceptible to cytokine-induced apoptosis. P7 induced a rapid increase in the intracellular calcium in MIN6 β-cells (in a GPR56-dependent manner) and human islets, and it also caused a sustained and reversible increase in insulin secretion from human islets. Collagen III protected human islets from cytokine-induced apoptosis, while P7 was without significant effect. CONCLUSIONS: These data indicate that GPR56 exhibits both agonist-dependent and -independent trafficking in β-cells and suggest that while GPR56 undergoes constitutive signalling, it can also respond to its ligands when required. We have also identified that constitutive and agonist-dependent GPR56 activation is coupled to protect β-cells against apoptosis, offering a potential therapeutic target to maintain β-cell mass in type 2 diabetes.
format Online
Article
Text
id pubmed-8326393
institution National Center for Biotechnology Information
language English
publishDate 2021
publisher Elsevier
record_format MEDLINE/PubMed
spelling pubmed-83263932021-08-06 SNAP-tag-enabled super-resolution imaging reveals constitutive and agonist-dependent trafficking of GPR56 in pancreatic β-cells Olaniru, Oladapo E. Cheng, Jordan Ast, Julia Arvaniti, Anastasia Atanes, Patricio Huang, Guo C. King, Aileen J.F. Jones, Peter M. Broichhagen, Johannes Hodson, David J. Persaud, Shanta J. Mol Metab Original Article OBJECTIVE: Members of the adhesion G protein-coupled receptor (aGPCR) subfamily are important actors in metabolic processes, with GPR56 (ADGRG1) emerging as a possible target for type 2 diabetes therapy. GPR56 can be activated by collagen III, its endogenous ligand, and by a synthetic seven amino-acid peptide (TYFAVLM; P7) contained within the GPR56 Stachel sequence. However, the mechanisms regulating GPR56 trafficking dynamics and agonist activities are not yet clear. METHODS: Here, we introduced SNAPf-tag into the N-terminal segment of GPR56 to monitor GPR56 cellular activity in situ. Confocal and super-resolution microscopy were used to investigate the trafficking pattern of GPR56 in native MIN6 β-cells and in MIN6 β-cells where GPR56 had been deleted by CRISPR-Cas9 gene editing. Insulin secretion, changes in intracellular calcium, and β-cell apoptosis were determined by radioimmunoassay, single-cell calcium microfluorimetry, and measuring caspase 3/7 activities, respectively, in MIN6 β-cells and human islets. RESULTS: SNAP-tag labelling indicated that GPR56 predominantly underwent constitutive internalisation in the absence of an exogenous agonist, unlike GLP-1R. Collagen III further stimulated GPR56 internalisation, whereas P7 was without significant effect. The overexpression of GPR56 in MIN6 β-cells did not affect insulin secretion. However, it was associated with reduced β-cell apoptosis, while the deletion of GPR56 made MIN6 β-cells more susceptible to cytokine-induced apoptosis. P7 induced a rapid increase in the intracellular calcium in MIN6 β-cells (in a GPR56-dependent manner) and human islets, and it also caused a sustained and reversible increase in insulin secretion from human islets. Collagen III protected human islets from cytokine-induced apoptosis, while P7 was without significant effect. CONCLUSIONS: These data indicate that GPR56 exhibits both agonist-dependent and -independent trafficking in β-cells and suggest that while GPR56 undergoes constitutive signalling, it can also respond to its ligands when required. We have also identified that constitutive and agonist-dependent GPR56 activation is coupled to protect β-cells against apoptosis, offering a potential therapeutic target to maintain β-cell mass in type 2 diabetes. Elsevier 2021-07-02 /pmc/articles/PMC8326393/ /pubmed/34224919 http://dx.doi.org/10.1016/j.molmet.2021.101285 Text en © 2021 The Author(s) https://creativecommons.org/licenses/by-nc-nd/4.0/This is an open access article under the CC BY-NC-ND license (http://creativecommons.org/licenses/by-nc-nd/4.0/).
spellingShingle Original Article
Olaniru, Oladapo E.
Cheng, Jordan
Ast, Julia
Arvaniti, Anastasia
Atanes, Patricio
Huang, Guo C.
King, Aileen J.F.
Jones, Peter M.
Broichhagen, Johannes
Hodson, David J.
Persaud, Shanta J.
SNAP-tag-enabled super-resolution imaging reveals constitutive and agonist-dependent trafficking of GPR56 in pancreatic β-cells
title SNAP-tag-enabled super-resolution imaging reveals constitutive and agonist-dependent trafficking of GPR56 in pancreatic β-cells
title_full SNAP-tag-enabled super-resolution imaging reveals constitutive and agonist-dependent trafficking of GPR56 in pancreatic β-cells
title_fullStr SNAP-tag-enabled super-resolution imaging reveals constitutive and agonist-dependent trafficking of GPR56 in pancreatic β-cells
title_full_unstemmed SNAP-tag-enabled super-resolution imaging reveals constitutive and agonist-dependent trafficking of GPR56 in pancreatic β-cells
title_short SNAP-tag-enabled super-resolution imaging reveals constitutive and agonist-dependent trafficking of GPR56 in pancreatic β-cells
title_sort snap-tag-enabled super-resolution imaging reveals constitutive and agonist-dependent trafficking of gpr56 in pancreatic β-cells
topic Original Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8326393/
https://www.ncbi.nlm.nih.gov/pubmed/34224919
http://dx.doi.org/10.1016/j.molmet.2021.101285
work_keys_str_mv AT olaniruoladapoe snaptagenabledsuperresolutionimagingrevealsconstitutiveandagonistdependenttraffickingofgpr56inpancreaticbcells
AT chengjordan snaptagenabledsuperresolutionimagingrevealsconstitutiveandagonistdependenttraffickingofgpr56inpancreaticbcells
AT astjulia snaptagenabledsuperresolutionimagingrevealsconstitutiveandagonistdependenttraffickingofgpr56inpancreaticbcells
AT arvanitianastasia snaptagenabledsuperresolutionimagingrevealsconstitutiveandagonistdependenttraffickingofgpr56inpancreaticbcells
AT atanespatricio snaptagenabledsuperresolutionimagingrevealsconstitutiveandagonistdependenttraffickingofgpr56inpancreaticbcells
AT huangguoc snaptagenabledsuperresolutionimagingrevealsconstitutiveandagonistdependenttraffickingofgpr56inpancreaticbcells
AT kingaileenjf snaptagenabledsuperresolutionimagingrevealsconstitutiveandagonistdependenttraffickingofgpr56inpancreaticbcells
AT jonespeterm snaptagenabledsuperresolutionimagingrevealsconstitutiveandagonistdependenttraffickingofgpr56inpancreaticbcells
AT broichhagenjohannes snaptagenabledsuperresolutionimagingrevealsconstitutiveandagonistdependenttraffickingofgpr56inpancreaticbcells
AT hodsondavidj snaptagenabledsuperresolutionimagingrevealsconstitutiveandagonistdependenttraffickingofgpr56inpancreaticbcells
AT persaudshantaj snaptagenabledsuperresolutionimagingrevealsconstitutiveandagonistdependenttraffickingofgpr56inpancreaticbcells

Ejemplares similares