Glutamate release from microglia via glutamate transporter is enhanced by amyloid-beta peptide

Abstract

In the present study, we found that amyloid-β peptide enhanced glutamate release from primary cultured rat microglia via the Na +-dependent glutamate transporter, which was activated by extracellular K +. Glutamate transport current was measured by a conventional whole-cell patch recording mode under voltage-clamp conditions. With the pipette solution containing 10 mM glutamate and 100 mM Na +, an increase of the external K + concentration from 0 to 10 mM evoked an outward current, resulting from co-extrusion of glutamate and Na +. The inward current, reflecting forward glutamate transport, was also activated by external glutamate. Both these reverse and forward glutamate transport currents were three-fold greater in microglia incubated with a relatively low concentration of amyloid-β peptide (25–35) (5 μM) for four days. The glutamate-activated inward current was blocked by d, l- threo-β-hydroxyaspartate in a dose-dependent manner (ranging from 0.001 to 1 mM), but not by a high concentration of kainate (1 mM). The glutamate concentration released from microglia upon high-K + stimulation was also significantly increased (up to 170 μM) after treatment with amyloid-β peptide (25–35). These results suggest that, at the pathological sites where extracellular K + concentration may increase, the activation of microglia by amyloid-β peptide causes an increase in extracellular glutamate concentration via reverse glutamate transporter, and therefore this mechanism may contribute to the pathogenesis of neuronal dysfunction and death in Alzheimer's disease.