Eclipse te

Hippocampal cells were loaded with Fluo-3 AM (1 μM in pluronic acid/DMSO, Molecular Probes, Eugene, OR, USA) for 30 min at 37°C and then washed twice with external solution, as described above, and incubated under control or experimental conditions for a maximal time of 30 min at 37°C. Neurons were mounted in a perfusion chamber that was placed on the stage of an inverted fluorescent microscope (Eclipse TE, Nikon), equipped with a CCD camera (SensiCam camera, PCO, Germany) and xenon excitation lamp. Cells were subsequently excited for 200 ms each 2 s intervals and recorded during 5 min, using a Lambda 10-2 filter wheel (Sutter Instruments) and regions of interest (ROI) were simultaneously selected on several neuronal somata on each plate (Ex:Em; 480:510 nm) recording more than 10 cells in each experiment. Finally, calcium transients, as defined by their TTX sensitivity (Gu et al., 1994 (link)), were acquired and analyzed off line with Axon Instruments Workbench 2.2 software.