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Measuring Fast Calcium Fluxes in Cardiomyocytes
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Measuring Fast Calcium Fluxes in Cardiomyocytes

Measuring Fast Calcium Fluxes in Cardiomyocytes

DOI:
10.3791/3505-v

12:10 min

November 29, 2011

,
1Department of Biological Sciences and Geology,Queensborough Community College, 2Department of Physiology & Biophysics,Stony Brook University

Chapters

  • 00:05Title
  • 01:15Loading Cells with Calcium Indicators
  • 02:23Microinjecting Cells
  • 03:42Co-immunofluorescence Studies
  • 04:49Fast Calcium Imaging and Data Analysis
  • 06:28Dissecting the Timing of Ca++ Fluxes Facilitates Evaluation of Their Impact on Cellular Events
  • 11:22Conclusion

Summary

자동 번역

자동 번역

We present a method to isolate rapid (microsecond) calcium events from slower fluxes in living cells using laser scanning confocal microscopy. The method measures fluorescence intensity fluctuations of calcium indicators by recording line scans of several hundred pixels in a cell. Histogram analysis allows us to isolate the time scales of different calcium fluxes.

Tags

Calcium FluxesCardiomyocytesMeasuringFastCa2+ ActivityPhospholipase Cβ- Gαq PathwayAcetylcholineCaveolaeEntrapmentGαqProlonged Ca2+ SignalsDynamic Calcium ResponsesFluorescent Ca2+ IndicatorCa2+ GreenFluorescence Emission IntensityLine-scan ModeLaser Scanning Confocal MicroscopeTime CourseMicrosecond Time ScaleExcel AnalysisSigmaplot AnalysisFlux Rate

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