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Title: Ligand-induced dynamics of heterotrimeric G protein-coupled receptor-like kinase complexes

Journal Article · · PLoS ONE
 [1];  [2]
  1. Univ. of North Carolina, Chapel Hill, NC (United States). Dept. of Biology
  2. Univ. of North Carolina, Chapel Hill, NC (United States). Dept. of Biology; Univ. of North Carolina, Chapel Hill, NC (United States). Dept. of Pharmacology

Background Arabidopsis, 7-transmembrane Regulator of G signaling protein 1 (AtRGS1) modulates canonical G protein signaling by promoting the inactive state of heterotrimeric G protein complex on the plasma membrane. It is known that plant leucine-rich repeat receptor-like kinases (LRR RLKs) phosphorylate AtRGS1 in vitro but little is known about the in vivo interaction, molecular dynamics, or the cellular consequences of this interaction. Methods Therefore, a subset of the known RLKs that phosphorylate AtRGS1 were selected for elucidation, namely, BAK1, BIR1, FLS2. Several microscopies for both static and dynamic protein-protein interactions were used to follow in vivo interactions between the RLKs and AtRGS1 after the presentation of the Pathogen-associated Molecular Pattern, Flagellin 22 (Flg22). These microscopies included FoÈrster Resonance Energy Transfer, Bimolecular Fluoresence Complementation, and Cross Number and Brightness fluorescence Correlation Spectroscopy. In addition, reactive oxygen species and calcium changes in living cells were quantitated using luminometry and R-GECO1 microscopy. Results The LRR RLKs BAK1 and BIR1, interact with AtRGS1 at the plasma membrane. The RLK ligand flg22 sets BAK1 in motion toward AtRGS1 and BIR1 away, both returning to the baseline orientations by 10 minutes. The C-terminal tail of AtRGS1 is important for the interaction with BAK1 and for the tempo of the AtRGS1/BIR1 dynamics. This window of time corresponds to the flg22-induced transient production of reactive oxygen species and calcium release which are both attenuated in the rgs1 and the bak1 null mutants. Conclusions A temporal model of these interactions is proposed. flg22 binding induces nearly instantaneous dimerization between FLS2 and BAK1. Phosphorylated BAK1 interacts with and enables AtRGS1 to move away from BIR1 and AtRGS1 becomes phosphorylated leading to its endocytosis thus leading to de-repression by permitting AtGPA1 to exchange GDP for GTP. Finally, the G protein complex becomes dissociated thus AGB1 interacts with its effector proteins leading to changes in reactive oxygen species and calcium.

Research Organization:
University of North Carolina, Chapel Hill, NC (United States)
Sponsoring Organization:
USDOE Office of Science (SC), Basic Energy Sciences (BES)
Grant/Contract Number:
FG02-05ER15671; R01GM065989; MCB-0718202
OSTI ID:
1362033
Journal Information:
PLoS ONE, Vol. 12, Issue 2; ISSN 1932-6203
Publisher:
Public Library of ScienceCopyright Statement
Country of Publication:
United States
Language:
English
Citation Metrics:
Cited by: 32 works
Citation information provided by
Web of Science

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Cited By (7)

Ligand-triggered de-repression of Arabidopsis heterotrimeric G proteins coupled to immune receptor kinases journal March 2018
Plant G-protein activation: connecting to plant receptor kinases journal May 2018
A receptor-like kinase mediated phosphorylation of Gα protein affects signaling during nodulation posted_content December 2019
Nucleotide exchange–dependent and nucleotide exchange–independent functions of plant heterotrimeric GTP-binding proteins journal November 2019
JA-Induced Endocytosis of AtRGS1 Is Involved in G-Protein Mediated JA Responses journal August 2019
Plant G-protein activation: connecting to plant receptor kinases text January 2018
Predicted Functional Implications of Phosphorylation of Regulator of G Protein Signaling Protein in Plants journal August 2017

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