Calibration of intracellular Ca transients of isolated adult heart cells labelled with fura-2 by acetoxymethyl ester loading

A procedure for calibration of fluorescence signals from adult rat heart cells loaded with the -AM ester of fura-2 is described. Calibration is complicated by dye compartmentation and potentially incomplete dye hydrolysis. These problems were overcome by subtracting from fluorescence transients the...

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Bibliographic Details
Published in:Cell calcium (Edinburgh) 1998-10, Vol.24 (4), p.263-273
Main Authors: Haworth, R.A., Redon, D.
Format: Article
Language:English
Subjects:
Adenosine Triphosphate
Animals
Biochemistry - methods
Calcium - analysis
Calcium - metabolism
Calibration
Cytosol - metabolism
Dogs
Egtazic Acid - analogs & derivatives
Female
Fluorescent Dyes - chemistry
Fura-2 - analogs & derivatives
Fura-2 - analysis
Fura-2 - chemistry
Ionomycin
Manganese - analysis
Mitochondria - metabolism
Myocardium - cytology
Myocardium - metabolism
Rats
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Description
Summary:A procedure for calibration of fluorescence signals from adult rat heart cells loaded with the -AM ester of fura-2 is described. Calibration is complicated by dye compartmentation and potentially incomplete dye hydrolysis. These problems were overcome by subtracting from fluorescence transients the non-cytosolic (mitochondrial) component of fura-2 fluorescence plus any Ca-insensitive component of dye fluorescence, after selectively and sequentially quenching cytosolic and non-cytosolic dye with Mn. The Kd of fura-2 in cells loaded by the -AM ester, in cells depleted of ATP and equilibrated with Ca buffers, was found to be 371 +/− 39 nM at 37°C. We found that calibration values for R MAX and R MIN derived from previously measured cells were of general validity, removing the need to measure R MAX and R MIN on every cell. Once these calibration values are determined, the calibration procedure to measure cytosolic Ca on any cell is a five minute procedure to determine compartmentation, using just one non-toxic and inexpensive solution. Finally, we have calculated how the errors intrinsic to the measurements translate into errors of the calculated Ca concentration and transient peak heights. These calculations allow reasonable parameters for data acquisition to be set.
ISSN:0143-4160
1532-1991
DOI:10.1016/S0143-4160(98)90050-1