Quantification and Localization of Intracellular Free Mg2+ in Bovine Chromaffin Cells

Magnesium is an essential element for all living systems. The quantification of free intracellular Mg2+ concentration ([Mg2+]i) is of utmost importance since changes in its basal value may be an indication of different pathologies due to abnormalities of Mg2+ metabolism. In this work we used 31P NMR and fluorescence spectroscopy to determine the resting [Mg2+]i in bovine chromaffin cells, a neuron-like cellular model, as well as confocal laser scanning microscopy to study the free Mg2+ spatial distribution in these cells. 31P NMR spectroscopy did not prove to be effective for the determination of [Mg2+]i in this particular case due to some special morphological and physiological properties of this cell type. A basal [Mg2+]i value of 0.551 ± 0.008 mM was found for these cells using fluorescence spectroscopy and the Mg2+-sensitive probe furaptra; this value falls in the concentration range reported in the literature for neurons from different sources. This technique proved to be an accurate and sensitive tool to determine the [Mg2+]i

Li+ Influx and Binding, and Li+/Mg2+ Competition in Bovine Chromaffin Cell Suspensions as Studied by 7Li NMR and Fluorescence Spectroscopy

Li+ influx by bovine chromaffin cells, obtained from bovine adrenal medulla, was studied in intact cell suspensions using 7Li NMR spectroscopy with the shift reagent [Tm(HDOTP)]4-. The influx rate constants, ki, were determined in the absence and in the presence of two Na+ membrane transport inhibitors. The values obtained indicate that both voltage sensitive Na+ channels and (Na+/K+)-ATPase play an important role in Li+ uptake by these cells. 7Li NMR T1 and T2 relaxation times for intracellular Li+ in bovine chromaffin cells provided a T1/T2 ratio of 305, showing that Li+ is highly, immobilized due to strong binding to intracellular structures. Using fluorescence spectroscopy and the Mg2+ fluorescent probe, furaptra, the free intracellular Mg2+ concentration in the bovine chromaffin cells incubated with 15 mM LiCl was found to increase by about mM after the intracellular Li+ concentration reached a steady state. Therefore, once inside the cell, Li+ is able to displace Mg2+ from its binding sites