Measuring local gradients of intramitochondrial [Ca(2+)] in cardiac myocytes during sarcoplasmic reticulum Ca(2+) release

Xiyuan Lu; Kenneth S Ginsburg; Sarah Kettlewell; Julie Bossuyt; Godfrey L Smith; Donald M Bers

doi:10.1161/CIRCRESAHA.111.300501

Measuring local gradients of intramitochondrial [Ca(2+)] in cardiac myocytes during sarcoplasmic reticulum Ca(2+) release

Circ Res. 2013 Feb 1;112(3):424-31. doi: 10.1161/CIRCRESAHA.111.300501. Epub 2012 Dec 14.

Authors

Xiyuan Lu¹, Kenneth S Ginsburg, Sarah Kettlewell, Julie Bossuyt, Godfrey L Smith, Donald M Bers

Affiliation

¹ Department of Pharmacology, University of California, Davis, CA 95616, USA.

Abstract

Rationale: Mitochondrial [Ca(2+)] ([Ca(2+)](mito)) regulates mitochondrial energy production, provides transient Ca(2+) buffering under stress, and can be involved in cell death. Mitochondria are near the sarcoplasmic reticulum (SR) in cardiac myocytes, and evidence for crosstalk exists. However, quantitative measurements of [Ca(2+)](mito) are limited, and spatial [Ca(2+)](mito) gradients have not been directly measured.

Objective: To directly measure local [Ca(2+)](mito) during normal SR Ca release in intact myocytes, and evaluate potential subsarcomeric spatial [Ca(2+)](mito) gradients.

Methods and results: Using the mitochondrially targeted inverse pericam indicator Mitycam, calibrated in situ, we directly measured [Ca(2+)](mito) during SR Ca(2+) release in intact rabbit ventricular myocytes by confocal microscopy. During steady state pacing, Δ[Ca(2+)](mito) amplitude was 29±3 nmol/L, rising rapidly (similar to cytosolic free [Ca(2+)]) but declining much more slowly. Taking advantage of the structural periodicity of cardiac sarcomeres, we found that [Ca(2+)](mito) near SR Ca(2+) release sites (Z-line) versus mid-sarcomere (M-line) reached a high peak amplitude (37±4 versus 26±4 nmol/L, respectively P<0.05) which occurred earlier in time. This difference was attributed to ends of mitochondria being physically closer to SR Ca(2+) release sites, because the mitochondrial Ca(2+) uniporter was homogeneously distributed, and elevated [Ca(2+)] applied laterally did not produce longitudinal [Ca(2+)](mito) gradients.

Conclusions: We developed methods to measure spatiotemporal [Ca(2+)](mito) gradients quantitatively during excitation-contraction coupling. The amplitude and kinetics of [Ca(2+)](mito) transients differ significantly from those in the cytosol and are respectively higher and faster near the Z-line versus M-line. This approach will help clarify SR-mitochondrial Ca(2+) signaling.

Publication types

Research Support, N.I.H., Extramural

MeSH terms

Animals
Biosensing Techniques / standards
Calcium / metabolism*
Calcium Signaling*
Calibration
Cardiac Pacing, Artificial
Cells, Cultured
Cytosol / metabolism
Excitation Contraction Coupling
Fluorescent Dyes / metabolism
Kinetics
Microscopy, Confocal / standards
Microscopy, Fluorescence / standards
Mitochondria, Heart / metabolism*
Myocardial Contraction
Myocytes, Cardiac / metabolism*
Rabbits
Sarcoplasmic Reticulum / metabolism*
Transfection

Substances

Fluorescent Dyes
Calcium

Abstract

Publication types

MeSH terms

Substances

Grants and funding