ITA
ENG

LOCALIZATION OF CALCIUM-ENTRY THROUGH CALCIUM CHANNELS IN OLFACTORY RECEPTOR NEURONS USING A LASER-SCANNING MICROSCOPE AND THE CALCIUM INDICATOR DYES FLUO-3 AND FURA-RED

Authors

SCHILD D JUNG A SCHULTENS HA

Citation

D. Schild et al., LOCALIZATION OF CALCIUM-ENTRY THROUGH CALCIUM CHANNELS IN OLFACTORY RECEPTOR NEURONS USING A LASER-SCANNING MICROSCOPE AND THE CALCIUM INDICATOR DYES FLUO-3 AND FURA-RED, Cell calcium, 15(5), 1994, pp. 341-348

Citations number

Categorie Soggetti

Cytology & Histology

Journal title

Cell calcium → ACNP

ISSN journal

01434160

Volume

Issue

Year of publication

1994

Pages

341 - 348

Database

ISI

SICI code

0143-4160(1994)15:5<341:LOCTCC>2.0.ZU;2-X

Abstract

The intracellular calcium concentration [Ca2+](i) in olfactory recepto r neurones of Xenopus laevis was imaged with high spatial and temporal resolution. A new method using a mixture of the calcium indicator dye s Fluo-3 and Fura-Red was employed. The fluorescence patterns in two w avelength bands were measured on the emission side of a confocal laser scanning microscope, and the ratio R of the fluorescence Intensities was taken as an estimate of [Ca2+](i). When the neurones were depolari zed by elevating the extracellular potassium concentration [K+]o they showed one of three types of responses: a fast increase In [Ca2+](i), a stow increase in [Ca2+](i), or no change in [Ca2+](i). The fast incr ease in [Ca2+](i) took place in the soma compartment. For at least 4 s after the onset of depolarization the calcium distribution in the den drite remained essentially unchanged. To study the fast increase with high time resolution, line scan images were taken. The neurones were d epolarized for brief periods applying a solution containing high [K+] onto the soma from an application pipette. The fast increase in [Ca2+] (i) began with a delay of about 200 ms and went from the resting conce ntration to about 110 nM above resting concentration. Following the de polarization, recovery from elevated [Ca2+](i) to resting levels had a time constant of about 15 s. The slow response seemed to depend on th e removal of [Na+] from the bath rather than on the elevated [K+] In t he bath. The response was also observed with Cd2+, Ni2+, and Co2+ (1.5 mM each) in the bath. The fast increase in [Ca2+](i) upon depolarizat ion was never seen if R > 0.8 ([Ca2+](i) > 300 nM). For R < 0.8, 45% o f the cells showed a fast response. Cells that responded with a fast i ncrease in [Ca2+](i) at low resting [Ca2+](i) did not do so for R > 0. 8. We suggest that the physiological role of calcium entry through cal cium channels on the soma of olfactory cells Is to decrease the membra ne impedance in an activity dependent way by activating a calcium depe ndent potassium conductance.