Differential Involvement of ACKR3 C-Tail in β-Arrestin Recruitment, Trafficking and Internalization

Aurélien Zarca; Claudia Perez; Jelle van den Bor; Jan Paul Bebelman; Joyce Heuninck; Rianna J.F. de Jonker; Thierry Durroux; Henry F. Vischer; Marco Siderius; Martine J. Smit

doi:10.3390/cells10030618

Differential Involvement of ACKR3 C-Tail in β-Arrestin Recruitment, Trafficking and Internalization

Aurélien Zarca
, Claudia Perez
, Jelle van den Bor
, Jan Paul Bebelman
, Joyce Heuninck
, Rianna J.F. de Jonker
, Thierry Durroux
, Henry F. Vischer
, Marco Siderius
, Martine J. Smit

AIMMS

Research output: Contribution to Journal › Article › Academic › peer-review

Abstract

Background: The atypical chemokine receptor 3 (ACKR3) belongs to the superfamily of G protein-coupled receptors (GPCRs). Unlike classical GPCRs, this receptor does not activate G proteins in most cell types but recruits β-arrestins upon activation. ACKR3 plays an important role in cancer and vascular diseases. As recruitment of β-arrestins is triggered by phosphorylation of the C-terminal tail of GPCRs, we studied the role of different potential phosphorylation sites within the ACKR3 C-tail to further delineate the molecular mechanism of internalization and trafficking of this GPCR. Methods: We used various bioluminescence and fluorescence resonance energy transfer-based sensors and techniques in Human Embryonic Kidney (HEK) 293T cells expressing WT or phosphorylation site mutants of ACKR3 to measure CXCL12-induced recruitment of β-arrestins and G-protein-coupled receptor kinases (GRKs), receptor internalization and trafficking. Results: Upon CXCL12 stimulation, ACKR3 recruits both β-arrestin 1 and 2 with equivalent kinetic profiles. We identified interactions with GRK2, 3 and 5, with GRK2 and 3 being important for β-arrestin recruitment. Upon activation, ACKR3 internalizes and recycles back to the cell membrane. We demonstrate that β-arrestin recruitment to the receptor is mainly determined by a single cluster of phosphorylated residues on the C-tail of ACKR3, and that residue T352 and in part S355 are important residues for β-arrestin1 recruitment. Phosphorylation of the C-tail appears essential for ligand-induced internalization and important for differential β-arrestin recruitment. GRK2 and 3 play a key role in receptor internalization. Moreover, ACKR3 can still internalize when β-arrestin recruitment is impaired or in the absence of β-arrestins, using alternative internalization pathways. Our data indicate that distinct residues within the C-tail of ACKR3 differentially regulate CXCL12-induced β-arrestin recruitment, ACKR3 trafficking and internalization.

Original language	English
Article number	618
Pages (from-to)	1-16
Number of pages	16
Journal	Cells
Volume	10
Issue number	3
Early online date	11 Mar 2021
DOIs	https://doi.org/10.3390/cells10030618
Publication status	Published - Mar 2021

Bibliographical note

This article belongs to the Special Issue: Novel Insights on G Protein-Coupled Receptor Kinases: From Cell Biology to Pathology.

Copyright:
This record is sourced from MEDLINE/PubMed, a database of the U.S. National Library of Medicine.

Funding

Funders	Funder number
Horizon 2020 Framework Programme	860229, 641833

UN SDGs

This output contributes to the following UN Sustainable Development Goals (SDGs)

SDG 3 Good Health and Well-being

Keywords

ACKR3
bioluminescence energy transfer (BRET)
chemokine receptor
GPCR
GRKs
homogeneous time resolved fluorescence (HTRF)
internalization
protein phosphorylation
protein recruitment
β-arrestins

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10.3390/cells10030618

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Cite this

@article{de4c778b08d94369949a1e4d34e8a1a8,

title = "Differential Involvement of ACKR3 C-Tail in β-Arrestin Recruitment, Trafficking and Internalization",

abstract = "Background: The atypical chemokine receptor 3 (ACKR3) belongs to the superfamily of G protein-coupled receptors (GPCRs). Unlike classical GPCRs, this receptor does not activate G proteins in most cell types but recruits β-arrestins upon activation. ACKR3 plays an important role in cancer and vascular diseases. As recruitment of β-arrestins is triggered by phosphorylation of the C-terminal tail of GPCRs, we studied the role of different potential phosphorylation sites within the ACKR3 C-tail to further delineate the molecular mechanism of internalization and trafficking of this GPCR. Methods: We used various bioluminescence and fluorescence resonance energy transfer-based sensors and techniques in Human Embryonic Kidney (HEK) 293T cells expressing WT or phosphorylation site mutants of ACKR3 to measure CXCL12-induced recruitment of β-arrestins and G-protein-coupled receptor kinases (GRKs), receptor internalization and trafficking. Results: Upon CXCL12 stimulation, ACKR3 recruits both β-arrestin 1 and 2 with equivalent kinetic profiles. We identified interactions with GRK2, 3 and 5, with GRK2 and 3 being important for β-arrestin recruitment. Upon activation, ACKR3 internalizes and recycles back to the cell membrane. We demonstrate that β-arrestin recruitment to the receptor is mainly determined by a single cluster of phosphorylated residues on the C-tail of ACKR3, and that residue T352 and in part S355 are important residues for β-arrestin1 recruitment. Phosphorylation of the C-tail appears essential for ligand-induced internalization and important for differential β-arrestin recruitment. GRK2 and 3 play a key role in receptor internalization. Moreover, ACKR3 can still internalize when β-arrestin recruitment is impaired or in the absence of β-arrestins, using alternative internalization pathways. Our data indicate that distinct residues within the C-tail of ACKR3 differentially regulate CXCL12-induced β-arrestin recruitment, ACKR3 trafficking and internalization.",

keywords = "ACKR3, bioluminescence energy transfer (BRET), chemokine receptor, GPCR, GRKs, homogeneous time resolved fluorescence (HTRF), internalization, protein phosphorylation, protein recruitment, β-arrestins",

author = "Aur{\'e}lien Zarca and Claudia Perez and \{van den Bor\}, Jelle and Bebelman, \{Jan Paul\} and Joyce Heuninck and \{de Jonker\}, \{Rianna J.F.\} and Thierry Durroux and Vischer, \{Henry F.\} and Marco Siderius and Smit, \{Martine J.\}",

note = "This article belongs to the Special Issue: Novel Insights on G Protein-Coupled Receptor Kinases: From Cell Biology to Pathology. Copyright: This record is sourced from MEDLINE/PubMed, a database of the U.S. National Library of Medicine.",

year = "2021",

month = mar,

doi = "10.3390/cells10030618",

language = "English",

volume = "10",

pages = "1--16",

journal = "Cells",

issn = "2073-4409",

publisher = "Multidisciplinary Digital Publishing Institute (MDPI)",

number = "3",

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TY - JOUR

T1 - Differential Involvement of ACKR3 C-Tail in β-Arrestin Recruitment, Trafficking and Internalization

AU - Zarca, Aurélien

AU - Perez, Claudia

AU - van den Bor, Jelle

AU - Bebelman, Jan Paul

AU - Heuninck, Joyce

AU - de Jonker, Rianna J.F.

AU - Durroux, Thierry

AU - Vischer, Henry F.

AU - Siderius, Marco

AU - Smit, Martine J.

N1 - This article belongs to the Special Issue: Novel Insights on G Protein-Coupled Receptor Kinases: From Cell Biology to Pathology. Copyright: This record is sourced from MEDLINE/PubMed, a database of the U.S. National Library of Medicine.

PY - 2021/3

Y1 - 2021/3

N2 - Background: The atypical chemokine receptor 3 (ACKR3) belongs to the superfamily of G protein-coupled receptors (GPCRs). Unlike classical GPCRs, this receptor does not activate G proteins in most cell types but recruits β-arrestins upon activation. ACKR3 plays an important role in cancer and vascular diseases. As recruitment of β-arrestins is triggered by phosphorylation of the C-terminal tail of GPCRs, we studied the role of different potential phosphorylation sites within the ACKR3 C-tail to further delineate the molecular mechanism of internalization and trafficking of this GPCR. Methods: We used various bioluminescence and fluorescence resonance energy transfer-based sensors and techniques in Human Embryonic Kidney (HEK) 293T cells expressing WT or phosphorylation site mutants of ACKR3 to measure CXCL12-induced recruitment of β-arrestins and G-protein-coupled receptor kinases (GRKs), receptor internalization and trafficking. Results: Upon CXCL12 stimulation, ACKR3 recruits both β-arrestin 1 and 2 with equivalent kinetic profiles. We identified interactions with GRK2, 3 and 5, with GRK2 and 3 being important for β-arrestin recruitment. Upon activation, ACKR3 internalizes and recycles back to the cell membrane. We demonstrate that β-arrestin recruitment to the receptor is mainly determined by a single cluster of phosphorylated residues on the C-tail of ACKR3, and that residue T352 and in part S355 are important residues for β-arrestin1 recruitment. Phosphorylation of the C-tail appears essential for ligand-induced internalization and important for differential β-arrestin recruitment. GRK2 and 3 play a key role in receptor internalization. Moreover, ACKR3 can still internalize when β-arrestin recruitment is impaired or in the absence of β-arrestins, using alternative internalization pathways. Our data indicate that distinct residues within the C-tail of ACKR3 differentially regulate CXCL12-induced β-arrestin recruitment, ACKR3 trafficking and internalization.

AB - Background: The atypical chemokine receptor 3 (ACKR3) belongs to the superfamily of G protein-coupled receptors (GPCRs). Unlike classical GPCRs, this receptor does not activate G proteins in most cell types but recruits β-arrestins upon activation. ACKR3 plays an important role in cancer and vascular diseases. As recruitment of β-arrestins is triggered by phosphorylation of the C-terminal tail of GPCRs, we studied the role of different potential phosphorylation sites within the ACKR3 C-tail to further delineate the molecular mechanism of internalization and trafficking of this GPCR. Methods: We used various bioluminescence and fluorescence resonance energy transfer-based sensors and techniques in Human Embryonic Kidney (HEK) 293T cells expressing WT or phosphorylation site mutants of ACKR3 to measure CXCL12-induced recruitment of β-arrestins and G-protein-coupled receptor kinases (GRKs), receptor internalization and trafficking. Results: Upon CXCL12 stimulation, ACKR3 recruits both β-arrestin 1 and 2 with equivalent kinetic profiles. We identified interactions with GRK2, 3 and 5, with GRK2 and 3 being important for β-arrestin recruitment. Upon activation, ACKR3 internalizes and recycles back to the cell membrane. We demonstrate that β-arrestin recruitment to the receptor is mainly determined by a single cluster of phosphorylated residues on the C-tail of ACKR3, and that residue T352 and in part S355 are important residues for β-arrestin1 recruitment. Phosphorylation of the C-tail appears essential for ligand-induced internalization and important for differential β-arrestin recruitment. GRK2 and 3 play a key role in receptor internalization. Moreover, ACKR3 can still internalize when β-arrestin recruitment is impaired or in the absence of β-arrestins, using alternative internalization pathways. Our data indicate that distinct residues within the C-tail of ACKR3 differentially regulate CXCL12-induced β-arrestin recruitment, ACKR3 trafficking and internalization.

KW - ACKR3

KW - bioluminescence energy transfer (BRET)

KW - chemokine receptor

KW - GPCR

KW - GRKs

KW - homogeneous time resolved fluorescence (HTRF)

KW - internalization

KW - protein phosphorylation

KW - protein recruitment

KW - β-arrestins

UR - https://www.scopus.com/pages/publications/85103919725

UR - https://www.scopus.com/pages/publications/85103919725#tab=citedBy

U2 - 10.3390/cells10030618

DO - 10.3390/cells10030618

M3 - Article

C2 - 33799570

AN - SCOPUS:85103919725

SN - 2073-4409

VL - 10

SP - 1

EP - 16

JO - Cells

JF - Cells

IS - 3

M1 - 618

ER -

Differential Involvement of ACKR3 C-Tail in β-Arrestin Recruitment, Trafficking and Internalization

Abstract

Bibliographical note

Funding

UN SDGs

Keywords

Access to Document

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