Intramolecular feedback regulation of the LRRK2 Roc G domain by a LRRK2 kinase dependent mechanism

Bernd K. Gilsbach
Franz Y. Ho
Benjamin Riebenbauer
Xiaojuan Zhang
Giambattista Guaitoli
Arjan Kortholt author has email address
Christian Johannes Gloeckner author has email address

German Center for Neurodegenerative diseases (DZNE), Tübingen, Germany
Department of Cell Biochemistry, University of Groningen, Groningen, The Netherlands
YETEM-Innovative Technologies Application and Research Centre Suleyman Demirel University West Campus, Isparta, Turkey
Core Facility for Medical Bioanalytics, Institute for Ophthalmic Research, Center for Ophthalmology, University of Tübingen, Tübingen, Germany

https://doi.org/10.7554/eLife.91083.2

Open access
Copyright information

Figures and data

Determination of kinetical parameters for LRRK2 GTP hydrolysis of PD variants by the Charcoal Assay. (A) Michaelis-Menten kinetics for pathogenic variant within the RocCOR module. (B) comparison of K_M values. (C) Comparison of k_cat values. (D) catalytic efficiency (k_cat/K_M). (E)-(G) Determination of k_obs values for full-length LRRK2 at 100µM (E) and 2000µM (F) GTP. (H) Domain structure of LRRK2 and the position of PD variants analyzed in this study.

HPLC-based full-length LRRK2 Michaelis-Menten kinetics

Comparison of PD mutants in the HPLC-based GTPase assay for the LRRK2 full-length protein. (A) Michaelis-Menten kinetics for the R1441G Roc-domain variant compared to LRRK2 wt. (B) Michaelis-Menten kinetics for the G2019S kinase-domain variant compared to LRRK2 wt. (C) Michaelis-Menten kinetics for a kinase-dead variant compared to LRRK2 wt.

Identification of T1343 as relevant autophosphorylation site for a negative feedback loop. (A) Michaelis-Menten kinetics for LRRK2 wt +/- ATP, (B) Phospho-site screen: Position of the LRRK2 phosho-sites within the Roc domain which were included in the screen mapped on PDB:7LHW (Myasnikov et al., 2021). Individual domains are highlighted in color as follows: Armadillo (gray), Ankyrin (green), LRR (yellow), Roc (magenta), COR (wheat), Kinase (blue), WD40 (dark green). (C) Michaelis-Menten kinetics for T1343A LRRK2 +/- ATP.

Overview of the kinetical parameters for fl. LRRK2 GTPase determined by the HPLC assay. (A) K_M values. (B) k_cat values and (C) catalytic efficiency (k_cat/K_M). Significant differences have been determined by an ANOVA followed by a post hoc test (p=0.05: *).

Autophosphorylation-induced LRRK2 monomerization as shown in Guaitoli et al., 2023 (Guaitoli et al., 2023) is abolished by the T1343A variant. (A) Mass photometry assays for LRRK2 wt and (B) T1343A LRRK2. Significance has been determined by a student’s T-test (p=0.05: *; p=0.01: **).

Effect of Roc T1343A on LRRK2 kinase activity and comparison to PD variants (A) In vitro LRRKtide HPLC-based kinase assay. (B) Western blot for LRRK2 pS935, total LRRK2, Rab10 pT73 and total Rab10. (C) Relative Rab phosphorylation levels. (D) Relative LRRK2 pS935 levels. Significant differences have been determined by an ANOVA followed by a post hoc test (p=0.05: *).

MBP-RocCOR Michaelis-Menten kinetics as measured by charcoal based GTPase assay

GTPase activity (k_obs) as measured by charcoal based GTPase assay

Cell-based phospho-Rab assays. Quantification of Western Blots

Michaelis-Menten kinetics for MLi-2 treated LRRK2 wt

Initial Phosphosite-screen (alanine screen). Michaelis-Menten parameters were determined in dependence of ATP pre-incubation. (A) K_M values. (B) k_cat values. The number of replicates is indicated.

Raw data for the In vitro LRRKtide HPLC Assay (determination of k_obs values). (A) LRRK2 G2019S, (B) LRRK2 wt, (C) LRRK2 T1343A, (D) kinase-dead (KD) LRRK2 K1906M

Cell-based phosphor-Rab assays, blot raw images used for quantification. (A-C) biological replicates

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