Values for ionized [Ca] in squid axons were obtained by measuring the light emission from a 0.1-mul drop of aequorin confined to a plastic dialysis tube of 140-mum diameter located axially. Ionized Ca had a mean value of 20 x 10(-9) M as judged by the subsequent introduction of CaEGTA/EGTA buffer (ratio ca. 0.1) into the axoplasm, and light measurement on a second aequorin drop. Ionized Ca in axoplasma was also measured by introducing arsenazo dye into an axon by injection and measuring the Ca complex of such a dye by multichannel spectrophotometry. Values so obtained were ca. 50 x 10(-9) M as calibrated against CaEGTA/EGTA buffer mixtures. Wth a freshly isolated axon in 10 mM Ca seawater, the aequorin glow invariably increased with time; a seawater [Ca] of 2-3 mM allowed a steady state with respect to [Ca]. Replacement of Na+ in seawater with choline led to a large increase in light emission from aequorin. Li seawater partially reversed this change and the reintroduction of Na+ brought light levels back to their initial value. Stimulation at 60/s for 2-5 min produced an increase in aequorin glow about 0.1% of that represented by the known Ca influx, suggesting operationally the presence of substantial Ca buffering. Treatment of an axon with CN produced a very large increase in aequorin glow and in Ca arsenazo formation only if the external seawater contained Ca.
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1 April 1976
Article|
April 01 1976
Ionized calcium concentrations in squid axons.
R Dipolo,
J Requena,
F J Brinley, Jr,
L J Mullins,
A Scarpa,
T Tiffert
Online ISSN: 1540-7748
Print ISSN: 0022-1295
J Gen Physiol (1976) 67 (4): 433–467.
Citation
R Dipolo, J Requena, F J Brinley, L J Mullins, A Scarpa, T Tiffert; Ionized calcium concentrations in squid axons.. J Gen Physiol 1 April 1976; 67 (4): 433–467. doi: https://doi.org/10.1085/jgp.67.4.433
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