lucifer-yellow and cesium-chloride

Ethanol (EtOH) is known to alter neuronal physiology, but much less is known about the actions of this drug on glial function. To this end, we examined acute effects of ethanol on resting and voltage-activated membrane currents in striatal astrocytes using rat brain slices. Ten minutes exposure to 50mM EtOH reduced slope conductance by 20%, increased input resistance by 25% and decreased capacitance by 38% but did not affect resting membrane potential. Current generated by a hyperpolarizing pulse was inhibited in a concentration dependent manner in passive astrocytes, while no significant EtOH effect was observed in complex astrocytes or neurons. The EtOH effect was blocked when intracellular KCl was replaced with CsCl, but not during chelation of intracellular calcium with BAPTA. During blockage of gap junction coupling with high intracellular CaCl(2) or extracellular carbenoxolone the EtOH effect persisted but was reduced. Interestingly, EtOH effects were largely irreversible when gap junctions were open, but were fully reversible when gap junctions were closed. Ethanol also reduced the spread to other cells of Lucifer Yellow dye from individual glia filled via the patch pipette. These data suggest that EtOH inhibits a calcium-insensitive potassium channel, most likely a passive potassium channel, but also affects gap junction coupling in a way that is sustained after ethanol withdrawal. Astrocytes play a critical role in brain potassium homeostasis, and therefore EtOH effects on astrocytic function could influence neuronal activity.

Topics: 1-Octanol; Animals; Astrocytes; Calcium; Carbenoxolone; Cell Communication; Cell Membrane Permeability; Cesium; Chelating Agents; Chlorides; Corpus Striatum; Egtazic Acid; Ethanol; Fluorescent Dyes; Gap Junctions; Ion Transport; Isoquinolines; Membrane Potentials; Microscopy, Fluorescence; Patch-Clamp Techniques; Potassium; Potassium Channels; Potassium Chloride; Rats; Rats, Sprague-Dawley

Cells, identified as supporting cells by Lucifer Yellow injection, were recorded from slices of frog olfactory epithelium using patch-clamp recordings. Cell-attached single-channel recordings indicated that the intracellular potential (IP) was -68 +/- 7 mV (n = 22) with 4 mM K+ in the bath ([K+]o). IP was -67 +/- 4 mV (n = 32) in whole-cell conditions with 100 mM KCl inside the cell, suggesting a low membrane permeability for Cl-. IP depended on [K+]o in a manner described by the Goldman-Hodgkin-Katz equation with a permeability ratio pk+:PNa+ of 40. The input resistance was 32 +/- 14 M omega (n = 15), indicating a high membrane conductance at rest. Odorant stimulations evoked passive membrane depolarizations, probably reflecting an increase in [K+]o due to the neuronal activation. Whole-cell recordings with 100 mM CsCl instead of KCl in the pipette, together with the block of gap-junctions with octanol, indicated the existence of an electrical coupling between supporting cells. The electrical coupling between these glial-like cells could facilitate the clearance of K+ ions released by olfactory receptor neurons during odorant stimulation.

Topics: Animals; Cell Membrane Permeability; Cesium; Chlorides; Electric Conductivity; Electrophysiology; Epithelium; Fluorescent Dyes; Gap Junctions; Isoquinolines; Octanols; Odorants; Olfactory Mucosa; Patch-Clamp Techniques; Potassium Chloride; Rana esculenta; Solutions