Calcium ions (Ca(2+)) play central roles in cellular physiology. Fluorescent indicators for Ca(2+) ions revolutionized our ability to make rapid, accurate, and highly parallel measurement of Ca(2+) concentrations in living cells. The use of ratio-based imaging with one particular indicator, fura-2, allowed practitioners to correct for a number of experimental confounds, including dye bleaching, variations in sample thickness, and fluctuations in illumination intensity. Ratio-based imaging with fura-2 was the most accurate and reliable method for measuring Ca(2+) concentrations. Two drawbacks to fura-2 exist. First, it requires ultraviolet (UV) excitation, which is more toxic to living cells than visible light. Second, our ability to use fura-2 for accurate, stable, ratio-based determinations of Ca(2+) concentration in living cells is fast becoming a method of the past. This is due, in part, because modern microscopes are phasing out the use of mercury arc lamps that provide the UV excitation needed for fura-2 imaging. To address this problem, we describe the design, synthesis, and cellular application of benzo[b]phosphole-based fluorescent Ca(2+) indicators for ratio-based imaging of Ca(2+) in living cells that can be used with modern light emitting diode (LED)-equipped fluorescence microscopes. We report isoCaRed-1Me, a Ca(2+) indicator that enables ratio-based imaging in immortalized cell lines, primary mammalian hippocampal neurons, and human-induced pluripotent stem cell-derived cardiomyocytes. These data show that isoCaRed-1Me will be useful for ratio-based Ca(2+) imaging using modern microscopes.
Ratio-based indicators for cytosolic Ca(2+) with visible light excitation.
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作者:Zhou Xinqi, Belavek Kayla J, Navarro Marisol X, Martinez Kayli N, Hinojosa Abigail, Miller Evan W
| 期刊: | Proceedings of the National Academy of Sciences of the United States of America | 影响因子: | 9.100 |
| 时间: | 2025 | 起止号: | 2025 Feb 18; 122(7):e2410436122 |
| doi: | 10.1073/pnas.2410436122 | ||
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