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Ca2+ is the most common signal transduction element in cells and plays critical rolls in neuronal development and plasticity. Ca2+ signals encode information in their oscillation frequency or amplitude and response time to regular cellular function. In this study, in order to reveal the spatio-temporal characterization of Ca2+ oscillations in rat hippocampal neurons, two kinds of Ca2+ fluorescent probes, yellow cameleons 2.1 (YC2.1) and Fluo-3, were used to monitor the change of the intracellular free Ca2+ concentration (]Ca2+[i). Spontaneous Ca2+ oscillations and glutamate elicited Ca2+ oscillations were observed with multi-photon excitation laser scan microscope (MPELSM) and confocal laser scan microscope (CLSM). The observation showed that the spatio- temporal characterization of either spontaneous or glutamate provoked Ca2+ oscillations had difference between the neurites and somata in individual nerons, especially in some distal end of neurites. The result indicated that Ca2+ oscillations were most important signal transduction pattern in neuronal development and activation. The spatio-temporal characterization of difference of Ca2+ signals between the distal endo of neurites and the somata might be associated with the distribution of ionotropic receptor and metabotropic glutamate receptors, and Ca2+ response mechanism mediated by two kinds of glutamate receptor. Ca2+ signal elicited by glutamate in the distal end of neurites appeared more complex and generated faster than that in the somata. It was suggested that Ca2+ signal in glutamate stimulated hippacamal neurons first generated from the distal end of neurites and then transduted to the somata. The complicated Ca2+ signal characterization in the distal end of neurites might be associated with neuronal activitation, neurotransmitter releasing, and other functions of neurons.
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