The quantitative measurement of cytosolic calcium concentration is central to the study of excitation-contraction coupling in cardiac cells. Significant problems, however, complicate the valid calibration of cardiac cells loaded with the membrane-permanent acetoxymethyl ester (AM) forms of the Ca 2+ probes, Indo-1 and Fura-2, notable mitochondrial dye compartmentation and incomplete AM-ester hydrolysis. We have developed a novel, simple and practical method to selectively load Indo-1 """"""""free acid"""""""" into the cytosol of adult cardiac myocytes presumable by diffusion through momentarily-permeable gap junctions during mechanical dissociation after low Ca 2+, collagenase treatment. A range of Indo-1 loading has been defined to select cells that produce suitable fluorescence signals, without significant alteration of their functional properties compared to non-Indo loaded cells; in particular, maximal twitch shortening velocity and extend of shortening in this range of Indo-1 is unchanged, with only minimal (less than or equal to 10%) prolongation of twitch duration (i.e., due to Ca 2+ buffering). Calibration of Indo-1 fluorescence in these cells has been accomplished after subtracting average autofluorescence derived from time- matched non-Indo loaded cells. Since there is wide variation in the degree of uncertainty of individual [Ca 2+] i determinations among cells (related principally to differences in cellular Indo-1 content, to nonlinear aspects of the [Ca 2+] vs. fluorescence ratio relationship, and to the uncertainty in the autoflourescence subtraction), a quantitative estimate of uncertainty may also be employed in formulating weighted, valid estimates of cytosolic [Ca 2+]i. The following [Ca 2+] i values in rat ventricular cells (nM; in 1 mM bathing [Ca 2+] o, 25 degrees C) are given as weighted means plus/minus 95% confidence intervals (unweighted values in parenthesis): 138 plus/minus 5 (136 plus/minus 6, n=44) in quiescent cells, 435 plus/minus 74 (482 plus/minus 76, n=43) at the [Ca 2+] i- transient peak during 0.5 Hz steady state stimulation, and 760 plus/minus 124 (1,027 plus/minus 250, n=42) at the [Ca 2+] i-transient peak, post- rest. Thus, the technique affords a practical way to accurately assess [Ca 2+] i in large numbers of isolated cardiac cells from a single batch-loaded preparation, avoiding many of the inherent limitations of micropipette impalement methods (i.e., cytosol dialysis, brief cell survival).

Agency
National Institute of Health (NIH)
Institute
National Institute on Aging (NIA)
Type
Intramural Research (Z01)
Project #
1Z01AG000261-04
Application #
3802231
Study Section
Project Start
Project End
Budget Start
Budget End
Support Year
4
Fiscal Year
1991
Total Cost
Indirect Cost
Name
National Institute on Aging
Department
Type
DUNS #
City
State
Country
United States
Zip Code
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