To make direct measurements of Ca2+ uptake and release by the sarcoplasmic reticulum (SR) of isolated smooth muscle cells, a fluorometric method for monitoring Ca2+ uptake by striated muscle SR vesicles (Kargacin, M.E., C.R. Scheid, and T.W. Honeyman. 1988. American Journal of Physiology. 245:C694-C698) was modified. With the method, it was possible to make continuous measurements of SR function in saponin-skinned smooth muscle cells in suspension. Calcium uptake by the SR was inhibited by thapsigargin and sequestered Ca2+ could be released by Br-A23187 and thapsigargin. From the rate of Ca2+ uptake by the skinned cells and the density of cells in suspension, it was possible to calculate the Ca2+ uptake rate for the SR of a single cell. Our results indicate that the SR Ca2+ pump in smooth muscle cells can remove Ca2+ at a rate that is 45-75% of the rate at which Ca2+ is removed from the cytoplasm of intact cells during transient Ca2+ signals. From estimates of SR volume reported by others and our measurements of the amount of Ca2+ taken up by the skinned cells, we conclude that the SR of a single cell can store greater than 10 times the amount of Ca2+ needed to elicit a single transient contractile response.
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1 September 1995
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September 01 1995
Direct measurement of Ca2+ uptake and release by the sarcoplasmic reticulum of saponin permeabilized isolated smooth muscle cells.
M E Kargacin,
M E Kargacin
Department of Medical Physiology, University of Calgary, Alberta, Canada.
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G J Kargacin
G J Kargacin
Department of Medical Physiology, University of Calgary, Alberta, Canada.
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M E Kargacin
,
G J Kargacin
Department of Medical Physiology, University of Calgary, Alberta, Canada.
Online ISSN: 1540-7748
Print ISSN: 0022-1295
J Gen Physiol (1995) 106 (3): 467–484.
Citation
M E Kargacin, G J Kargacin; Direct measurement of Ca2+ uptake and release by the sarcoplasmic reticulum of saponin permeabilized isolated smooth muscle cells.. J Gen Physiol 1 September 1995; 106 (3): 467–484. doi: https://doi.org/10.1085/jgp.106.3.467
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