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THERAPEUTIC POTENTIAL OF MPI INHIBITION TO REVERT PATHOGENIC CA<SUB>V</SUB>2.1 GAIN-OF-FUNCTION IN <EM>CACNA1A</EM>-RELATED NEUROLOGICAL DISORDERS
Gorane Rodríguez-Urquirizarand 2 co-authors
University Pompeu Fabra
FENS Forum 2026 (2026)
Barcelona, Spain
Board PS01-07AM-152
Presentation
Date TBA
Board: PS01-07AM-152
Event Information
Poster Board
PS01-07AM-152
Poster
View posterAbstract
The CACNA1A gene encodes the α1A subunit of the CaV2.1 (P/Q-type) voltage-gated calcium channel. Gain-of-function mutations in CACNA1A cause neurological disorders such as Familial Hemiplegic Migraine type 1 (FHM1) and Congenital Ataxia (CA) by increasing calcium influx and favouring neuronal excitability, which in turn promote cortical spreading depression (migraine pathophysiology) and Purkinje cell hyperexcitability (ataxia). Hypoglycosylation of CaV2.1, observed in Phosphomannomutase 2 deficiency (PMM2-CDG), mimics this effect. Since Phosphomannose Isomerase (MPI) competes with PMM2 for mannose-6-phosphate, we hypothesized that MPI inhibition combined with mannose supplementation could enhance N-glycosylation and counteract channel gain-of-function.
Using HEK293 cells expressing wild-type or mutant (Y1245C, Δ1502) CaV2.1, we tested the effect of MPI inhibitor MLS0315771 with mannose on N-glycosylation (Western Blot) and channel function (whole-cell patch-clamp electrophysiology). Treatment increased N-glycosylation of the α2δ subunit (p<0.01, n=4). The Δ1502 mutation caused a ~26 mV leftward shift in activation voltage (p<0.01, n=3-13) and slowed inactivation (p<0.05, n=5-11), both hallmarks of pathological gain-of-function. MPI inhibition with mannose partially normalized activation (by 6.5 mV, p<0.05, n=4) and inactivation kinetics (p<0.05, n=4-5). The Y1245C mutation reduced activation voltage (by ~6 mV, p<0.05, n=7-13), but treatment did not alter this effect. PMM2 silencing by siRNA decreased α2δ subunit N-glycosylation and membrane trafficking (p<0.05, n=3) and slowed inactivation (p<0.05, n=16-18), mimicking gain-of-function, which was reversed by MPI inhibition plus mannose (p<0.05, n=9-16).
These findings show that enhancing N-glycosylation via MPI inhibition mitigates pathogenicgain-of-function in specific CACNA1A mutations and PMM2 deficiency, proposing a targeted therapeutic approach for CaV2.1-related channelopathies.
Funding: MCIN/AEI/10.13039/501100011033; FEDER (PID2022-136546OB-I00).
Using HEK293 cells expressing wild-type or mutant (Y1245C, Δ1502) CaV2.1, we tested the effect of MPI inhibitor MLS0315771 with mannose on N-glycosylation (Western Blot) and channel function (whole-cell patch-clamp electrophysiology). Treatment increased N-glycosylation of the α2δ subunit (p<0.01, n=4). The Δ1502 mutation caused a ~26 mV leftward shift in activation voltage (p<0.01, n=3-13) and slowed inactivation (p<0.05, n=5-11), both hallmarks of pathological gain-of-function. MPI inhibition with mannose partially normalized activation (by 6.5 mV, p<0.05, n=4) and inactivation kinetics (p<0.05, n=4-5). The Y1245C mutation reduced activation voltage (by ~6 mV, p<0.05, n=7-13), but treatment did not alter this effect. PMM2 silencing by siRNA decreased α2δ subunit N-glycosylation and membrane trafficking (p<0.05, n=3) and slowed inactivation (p<0.05, n=16-18), mimicking gain-of-function, which was reversed by MPI inhibition plus mannose (p<0.05, n=9-16).
These findings show that enhancing N-glycosylation via MPI inhibition mitigates pathogenicgain-of-function in specific CACNA1A mutations and PMM2 deficiency, proposing a targeted therapeutic approach for CaV2.1-related channelopathies.
Funding: MCIN/AEI/10.13039/501100011033; FEDER (PID2022-136546OB-I00).
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