Localized, transient elevations in cytosolic Ca2+, known as Ca2+ sparks, caused by Ca2+ release from sarcoplasmic reticulum, are thought to trigger the opening of large conductance Ca2+-activated potassium channels in the plasma membrane resulting in spontaneous transient outward currents (STOCs) in smooth muscle cells. But the precise relationships between Ca2+ concentration within the sarcoplasmic reticulum and a Ca2+ spark and that between a Ca2+ spark and a STOC are not well defined or fully understood. To address these problems, we have employed two approaches using single patch-clamped smooth muscle cells freshly dissociated from toad stomach: a high speed, wide-field imaging system to simultaneously record Ca2+ sparks and STOCs, and a method to simultaneously measure free global Ca2+ concentration in the sarcoplasmic reticulum ([Ca2+]SR) and in the cytosol ([Ca2+]CYTO) along with STOCs. At a holding potential of 0 mV, cells displayed Ca2+ sparks and STOCs. Ca2+ sparks were associated with STOCs; the onset of the sparks coincided with the upstroke of STOCs, and both had approximately the same decay time. The mean increase in [Ca2+]CYTO at the time and location of the spark peak was ∼100 nM above a resting concentration of ∼100 nM. The frequency and amplitude of spontaneous Ca2+ sparks recorded at −80 mV were unchanged for a period of 10 min after removal of extracellular Ca2+ (nominally Ca2+-free solution with 50 μM EGTA), indicating that Ca2+ influx is not necessary for Ca2+sparks. A brief pulse of caffeine (20 mM) elicited a rapid decrease in [Ca2+]SR in association with a surge in [Ca2+]CYTO and a fusion of STOCs, followed by a fast restoration of [Ca2+]CYTO and a gradual recovery of [Ca2+]SR and STOCs. The return of global [Ca2+]CYTO to rest was an order of magnitude faster than the refilling of the sarcoplasmic reticulum with Ca2+. After the global [Ca2+]CYTO was fully restored, recovery of STOC frequency and amplitude were correlated with the level of [Ca2+]SR, even though the time for refilling varied greatly. STOC frequency did not recover substantially until the [Ca2+]SR was restored to 60% or more of resting levels. At [Ca2+]SR levels above 80% of rest, there was a steep relationship between [Ca2+]SR and STOC frequency. In contrast, the relationship between [Ca2+]SR and STOC amplitude was linear. The relationship between [Ca2+]SR and the frequency and amplitude was the same for Ca2+ sparks as it was for STOCs. The results of this study suggest that the regulation of [Ca2+]SR might provide one mechanism whereby agents could govern Ca2+ sparks and STOCs. The relationship between Ca2+ sparks and STOCs also implies a close association between a sarcoplasmic reticulum Ca2+ release site and the Ca2+-activated potassium channels responsible for a STOC.
The Influence of Sarcoplasmic Reticulum Ca2+ Concentration on Ca2+ Sparks and Spontaneous Transient Outward Currents in Single Smooth Muscle Cells
Dr. Fay died on 18 March 1997.
Address correspondence to John V. Walsh, Jr., Department of Physiology, Biomedical Imaging Group, University of Massachusetts Medical Center, Worcester, MA 01605. Fax: 508-856-5997; E-mail: [email protected]
The ability of the ultrafast microscope to resolve and measure highly localized calcium signals was examined using a computer simulation of Ca2+ sparks of known peak [Ca2+] as imaged inside a model cell. Fluorescence ratios (ΔF/F0) were calculated from simulated images of a range of spark [Ca2+] amplitudes, both in and out of focus. From these simulations, we estimated that an observed average spark amplitude of 10% (ΔF/F0) is consistent with a peak spark [Ca2+] of 200 nM, or 100 nM above resting [Ca2+]. This estimate was made in the following way.
First, the fluorescence intensity distribution of a typical Ca2+ spark inside a smooth muscle cell was simulated. Custom software was used to calculate the three-dimensional image of a model smooth muscle cell filled with 50 μM fluo-3 (Kd = 390 nM) in equilibrium with a resting [Ca2+] of 100 nM. The cell was modeled as a cylinder with cross-sectional diameters of 10 μm in the transverse direction and 6 μm in the axial direction, the direction of focus in the microscope, and of infinite length with respect to the imaging. These dimensions were previously derived from three-dimensional reconstructions of toad gastric smooth muscle cells (our unpublished data). The three-dimensional fluorescence intensity distribution was calculated assuming bound fluo-3 was 100× as fluorescent as the free species. At resting [Ca2+], ∼25% of the fluo-3 was bound to Ca2+ and the fluorescence signal at rest was ∼20% of the maximum attainable with saturating Ca2+.
Second, the spatial [Ca2+] profile of a Ca2+ spark was added to the simulated resting cell. A Ca2+ spark was modeled as a stationary, Gaussian spot of calcium with a known peak [Ca2+] and a spatial full width at half-maximum amplitude of 1.7 μm. This simulates the spark at a single point in time, corresponding to the observed images of sparks at the time of peak fluorescence intensity. The Ca2+ spark was added to the resting cell model with the spark peak at the center of the cell, and the corresponding three-dimensional image of fluo-3 distribution was calculated as for the resting cell alone. The center of the cell was used to avoid having to simulate the effect of the cell membrane on diffusion. Since the fluorescence background due to resting [Ca2+] is likely highest at the center, where the cell is thickest, this is probably the worst case, for our purposes, for measuring ΔF/F0.
Next, the image formation and acquisition was simulated. The three-dimensional fluorescence image of the cell and spark was blurred with the three-dimensional image of a theoretical, wide-field, point spread function, for a 1.3 NA objective lens (Nikon Inc.) calculated at 530 nm wavelength (Tella, 1985). The image resolution was decreased to 300-nm pixels, by adding three-by-three groups of pixels, in order to simulate the image formation (point spread function) and acquisition (camera pixelization) process. The resulting three- dimensional image contained images of the spark in and out of focus, as seen against the fluorescence background arising from the global resting [Ca2+].
Lastly, using the blurred images of the cell with and without the spark, the fluorescence ratios (ΔF/F0) were calculated at the pixel corresponding to the spark center, at 200-nm focus steps through the 6-μm depth of the cell. The effect of uncertainty in focus was examined by weighting the ΔF/F0 calculated at each depth through the cell by the probability of a spark occurring at that depth. Although the modeled spark was located in the cell center, the model used for spark spatial distribution assumed that sparks were constrained to occur at the outer edge of the cell, adjacent to the plasma membrane, and were equally likely to occur anywhere along the plasma membrane. A spark with a known peak [Ca2+] of 200 nM (100 nM above resting [Ca2+]) yielded a ΔF/F0 of 18% when in focus (centered in depth) and 5.5% when 3 μm out of focus (top or bottom of cell). After accounting for the effects of spark location on focus, the average ΔF/F0 was 10%, a value equivalent to the average observed spark peak amplitude described in this report.
Ronghua ZhuGe, Richard A. Tuft, Kevin E. Fogarty, Karl Bellve, Fredric S. Fay, John V. Walsh; The Influence of Sarcoplasmic Reticulum Ca2+ Concentration on Ca2+ Sparks and Spontaneous Transient Outward Currents in Single Smooth Muscle Cells . J Gen Physiol 1 February 1999; 113 (2): 215–228. doi: https://doi.org/10.1085/jgp.113.2.215
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