Detail of Fig2B_C220S_SFN_60min

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Project
Title
Live imaging of HEK293 cells coexpressing P2Y6R C220S-YFP and Lifeact at time point of 60min.
Description
Live imaging of HEK293 cells coexpressing P2Y6R C220S-YFP and Lifeact at time point of 60min.
Release, Updated
2022-11-23
License
CC BY
Kind
Image data
File Formats
NA
Data size
25.3 KB

Organism
Homo sapiens ( NCBI:txid9606 )
Strain(s)
-
Cell Line
HEK293 ( CLO_0001230 )
Protein names
P2Y6R
Protein tags
YFP

Datatype
-
Molecular Function (MF)
G protein-coupled receptor kinase activity ( GO:0004703 )
Biological Process (BP)
regulation of G protein-coupled receptor internalization ( GO:1904020 )
Cellular Component (CC)
Biological Imaging Method
confocal microscopy ( Fbbi:00000251 )
X scale
84.6582 micrometer/pixel
Y scale
84.6582 micrometer/pixel
Z scale
-
T scale
-

Image Acquisition
Experiment type
-
Microscope type
-
Acquisition mode
-
Contrast method
-
Microscope model
-
Detector model
-
Objective model
-
Filter set
-

Summary of Methods
See details in Nishiyama K, et. al. (2022) Sci Signal, Jan 11;15(716):eabj0644.
Related paper(s)

Kazuhiro Nishiyama, Akiyuki Nishimura, Kakeru Shimoda, Tomohiro Tanaka, Yuri Kato, Takahiro Shibata, Hiroshi Tanaka, Hitoshi Kurose, Yasu-Taka Azuma, Hideshi Ihara, Yoshito Kumagai, Takaaki Akaike, Philip Eaton, Koji Uchida, Motohiro Nishida (2022) Redox-dependent internalization of the purinergic P2Y6 receptor limits colitis progression., Science signaling, Volume 15, Number 716, pp. eabj0644

Published in 2022 Jan 11 (Electronic publication in Jan. 11, 2022, midnight )

(Abstract) After ligand stimulation, many G protein-coupled receptors (GPCRs) undergo beta-arrestin-dependent desensitization, during which they are internalized and either degraded or recycled to the plasma membrane. Some GPCRs are not subject to this type of desensitization because they lack the residues required to interact with beta-arrestins. We identified a mechanism of redox-dependent alternative internalization (REDAI) that promotes the internalization and degradation of the purinergic P2Y6 receptor (P2Y6R). Synthetic and natural compounds containing electrophilic isothiocyanate groups covalently modified P2Y6R at Cys(220), which promoted the ubiquitylation of Lys(137) and receptor internalization and degradation in various mouse and human cultured cell lines. Endogenous electrophiles also promoted ligand-dependent P2Y6R internalization and degradation. P2Y6R is highly abundant in inflammatory cells and promotes the pathogenesis of colitis. Deficiency in P2Y6R protected mice against experimentally induced colitis, and mice expressing a form of P2Y6R in which Cys(220) was mutated to nonmodifiable serine were more sensitive to the induction of colitis. Several other GPCRs, including A2BAR, contain cysteine and lysine residues at the appropriate positions to mediate REDAI, and isothiocyanate stimulated the internalization of A2BAR and of a form of P2Y2R with insertions of the appropriate residues. Thus, endogenous and exogenous electrophiles may limit colitis progression through cysteine modification of P2Y6R and may also mediate internalization of other GPCRs.
(MeSH Terms)

Contact
Motohiro Nishida , Kyushu University , Graduate School of Pharmaceutical Sciences
Contributors

OMERO Dataset
OMERO Project
Source