Drosophila melanogaster as a model for unraveling unique molecular features of epilepsy elicited by human GABA transporter 1 variants

Ameya S Kasture; Florian P Fischer; Lisa Kunert; Melanie L Burger; Alexander C Burgstaller; Ali El-Kasaby; Thomas Hummel; Sonja Sucic

doi:10.3389/fnins.2022.1074427

Drosophila melanogaster as a model for unraveling unique molecular features of epilepsy elicited by human GABA transporter 1 variants

Front Neurosci. 2023 Jan 19:16:1074427. doi: 10.3389/fnins.2022.1074427. eCollection 2022.

Authors

Ameya S Kasture^{1

2}, Florian P Fischer^{1

3}, Lisa Kunert², Melanie L Burger¹, Alexander C Burgstaller¹, Ali El-Kasaby¹, Thomas Hummel², Sonja Sucic¹

Affiliations

¹ Institute of Pharmacology, Medical University of Vienna, Vienna, Austria.
² Department of Neuroscience and Developmental Biology, University of Vienna, Vienna, Austria.
³ Department of Epileptology and Neurology, University of Aachen, Aachen, Germany.

Abstract

Mutations in the human γ-aminobutyric acid (GABA) transporter 1 (hGAT-1) can instigate myoclonic-atonic and other generalized epilepsies in the afflicted individuals. We systematically examined fifteen hGAT-1 disease variants, all of which dramatically reduced or completely abolished GABA uptake activity. Many of these loss-of-function variants were absent from their regular site of action at the cell surface, due to protein misfolding and/or impaired trafficking machinery (as verified by confocal microscopy and de-glycosylation experiments). A modest fraction of the mutants displayed correct targeting to the plasma membrane, but nonetheless rendered the mutated proteins devoid of GABA transport, possibly due to structural alterations in the GABA binding site/translocation pathway. We here focused on a folding-deficient A288V variant. In flies, A288V reiterated its impeded expression pattern, closely mimicking the ER-retention demonstrated in transfected HEK293 cells. Functionally, A288V presented a temperature-sensitive seizure phenotype in fruit flies. We employed diverse small molecules to restore the expression and activity of folding-deficient hGAT-1 epilepsy variants, in vitro (in HEK293 cells) and in vivo (in flies). We identified three compounds (chemical and pharmacological chaperones) conferring moderate rescue capacity for several variants. Our data grant crucial new insights into: (i) the molecular basis of epilepsy in patients harboring hGAT-1 mutations, and (ii) a proof-of-principle that protein folding deficits in disease-associated hGAT-1 variants can be corrected using the pharmacochaperoning approach. Such innovative pharmaco-therapeutic prospects inspire the rational design of novel drugs for alleviating the clinical symptoms triggered by the numerous emerging pathogenic mutations in hGAT-1.

Keywords: 4-phenylbutyrate; Drosophila melanogaster; GABA transporter 1; epilepsy; protein folding and trafficking; transporter disease variants; uptake; γ -aminobutyric acid (GABA).

Grants and funding

The authors acknowledge financial support from the Austrian Science Fund (FWF projects P36574-B27 and P31255-B27 to SS).