Detail of Fig7a_SMovie5_timelapse_D208_170927
Project
Title
Time-lapse images of chemotaxis trajectories of gip1Δ cells harbouring mutant Gip1(D208A).
Description
Time-lapse images of chemotaxis trajectories of gip1Δ cells harbouring mutant Gip1(D208A).
Release, Updated
2022-03-31
License
CC-BY
Kind
Image data
File Formats
.nd2
Data size
1004.2 MB
Gene symbols
gip1
Datatype
-
Molecular Function (MF)
-
Biological Process (BP)
chemotaxis
(
GO:0006935
)
Cellular Component (CC)
-
Biological Imaging Method
time lapse microscopy
(
Fbbi:00000249
)
X scale
2.4859 micrometer/pixel
Y scale
2.4859 micrometer/pixel
Z scale
-
T scale
10 second per time interval
Image Acquisition
Experiment type
-
Microscope type
-
Acquisition mode
-
Contrast method
-
Microscope model
-
Detector model
-
Objective model
-
Filter set
-
Summary of Methods
See details in Miyagawa T, et. al. (2018) Nat Commun., 9(1):4635.
Related paper(s)
Takero Miyagawa, Hiroyasu Koteishi, Yoichiro Kamimura, Yukihiro Miyanaga, Kohei Takeshita, Atsushi Nakagawa, Masahiro Ueda (2018) Structural basis of Gip1 for cytosolic sequestration of G protein in wide-range chemotaxis., Nature communications, Volume 9, Number 1, pp. 4635
Published in 2018 Nov 6 (Electronic publication in Nov. 6, 2018, midnight )
- doi: 10.1038/s41467-018-07035-x
-
pmid: 30401901
(Abstract) G protein interacting protein 1 (Gip1) binds and sequesters heterotrimeric G proteins in the cytosolic pool, thus regulating G protein-coupled receptor (GPCR) signalling for eukaryotic chemotaxis. Here, we report the underlying structural basis of Gip1 function. The crystal structure reveals that the region of Gip1 that binds to the G protein has a cylinder-like fold with a central hydrophobic cavity composed of six alpha-helices. Mutagenesis and biochemical analyses indicate that the hydrophobic cavity and the hydrogen bond network at the entrance of the cavity are essential for complex formation with the geranylgeranyl modification on the Ggamma subunit. Mutations of the cavity impair G protein sequestration and translocation to the membrane from the cytosol upon receptor stimulation, leading to defects in chemotaxis at higher chemoattractant concentrations. These results demonstrate that the Gip1-dependent regulation of G protein shuttling ensures wide-range gradient sensing in eukaryotic chemotaxis.(MeSH Terms)
- Chemotactic Factors/chemistry
- Chemotaxis/physiology[major]
- Crystallography, X-Ray
- Cytosol/metabolism[major]
- Dictyostelium
- Eukaryota
- GTP-Binding Proteins/chemistry[major]
- GTP-Binding Proteins/genetics
- Heterotrimeric GTP-Binding Proteins/chemistry[major]
- Hydrogen Bonding
- Models, Molecular
- Mutagenesis
- Mutation
- Protein Binding
- Protein Conformation
- Protein Interaction Domains and Motifs
- Protein Phosphatase 1
- Receptors, G-Protein-Coupled/chemistry[major]
- Saccharomyces cerevisiae Proteins
- Signal Transduction
Contact
Masahiro Ueda
, Osaka University
, Graduate School of Frontier Biosciences
, Laboratory for Cell Signaling Dynamics
Contributors
OMERO Dataset
OMERO Project
Source