A possible role of the non-GAT1 GABA transporters in transfer of GABA from GABAergic to glutamatergic neurons in mouse cerebellar neuronal cultures
| Autor: | Cristina Suñol, Rosa Cristòfol, Arne Schousboe, Zoila Babot, Helle S. Waagepetersen, Ursula Sonnewald |
|---|---|
| Jazyk: | angličtina |
| Rok vydání: | 2010 |
| Předmět: |
Cerebellum
GABA Plasma Membrane Transport Proteins Tiagabine GABA Agents Population Nipecotic Acids Glutamic Acid Biology Inhibitory postsynaptic potential Biochemistry Cellular and Molecular Neuroscience chemistry.chemical_compound Glutamatergic Mice medicine Nipecotic acid Animals education GABA Agonists Cells Cultured gamma-Aminobutyric Acid Neurons education.field_of_study Lipotropic Agents Glutamate Decarboxylase General Medicine Cell biology Betaine Guvacine medicine.anatomical_structure chemistry nervous system Vesicular Glutamate Transport Protein 1 GABAergic medicine.drug |
| Zdroj: | Digital.CSIC. Repositorio Institucional del CSIC instname |
| ISSN: | 1573-6903 0364-3190 |
| Popis: | Cultures of dissociated cerebellum from 7-day-old mice were used to investigate the mechanism involved in synthesis and cellular redistribution of GABA in these cultures consisting primarily of glutamatergic granule neurons and a smaller population of GABAergic Golgi and stellate neurons. The distribution of GAD, GABA and the vesicular glutamate transporter VGlut-1 was assessed using specific antibodies combined with immunofluorescence microscopy. Additionally, tiagabine, SKF 89976-A, betaine, beta-alanine, nipecotic acid and guvacine were used to inhibit the GAT1, betaine/GABA (BGT1), GAT2 and GAT3 transporters. Only a small population of cells were immuno-stained for GAD while many cells exhibited VGlut-1 like immuno-reactivity which, however, never co-localized with GAD positive neurons. This likely reflects the small number of GABAergic neurons compared to the glutamatergic granule neurons constituting the majority of the cells. GABA uptake exhibited the kinetics of high affinity transport and could be partly (20%) inhibited by betaine (IC(50) 142 microM), beta-alanine (30%) and almost fully (90%) inhibited by SKF 89976-A (IC(50) 0.8 microM) or nipecotic acid and guvacine at 1 mM concentrations (95%). Essentially all neurons showed GABA like immunostaining albeit with differences in intensity. The results indicate that GABA which is synthesized in a small population of GAD-positive neurons is redistributed to essentially all neurons including the glutamatergic granule cells. GAT1 is not likely involved in this redistribution since addition of 15 microM tiagabine (GAT1 inhibitor) to the culture medium had no effect on the overall GABA content of the cells. Likewise the BGT1 transporter cannot alone account for the redistribution since inclusion of 3 mM betaine in the culture medium had no effect on the overall GABA content. The inhibitory action of beta-alanine and high concentrations of nipecotic acid and guvacine on GABA transport strongly suggests that also GAT2 or GAT3 (HUGO nomenclature) could play a role. This work was supported by grants from FIS 061212 (Ministry of Health, Spain), 2009/SGR/214 (CIRIT, Generalitat de Catalunya, Spain) and The Danish Medical Research Council (22-03-250; 22-04-0314). Z. B. was recipient of a predoctoral fellowship from the Spanish Ministry of Education. |
| Databáze: | OpenAIRE |
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