Abstract

The overall aim of the proposed research is to quantify the spatio-temporal variation of cytoplasmic [Ca2+] during excitation-contration coupling in mammalian heart cells, in order to understand the cellular processes that produce the cytoplasmic [Ca2+] transient, and to quantify the influence of Ca2+ on cellular functions. To be tested in the present research is an hypothesis which comprises a specific aspect of the overall aim. Hypothesis: Ca2+ entering the cell via surface membrane Ca2+ channels enters rapidly into junctional regions of the sarcoplasmic reticulum (SR), rather than accumulatilng in the cytoplasm. In Purkinje fibers, release of Ca2+ into the cytoplasm from junctional SR underlies a rapid initial rise in cytoplasmic [Ca2+] (L1 component of the aequorin signal). Ca2+ diffuses to regions of SR deep in the cell, triggering Ca2+ release (component L2). In ventricular cells, separate components of Ca2+ indicator signals are not evident because the diffusion delays are small, compared to Purkinje fibers. Predictions and tests of this hypothesis are: 1) In Purkinje fibers, L1 is highly spatially localized. To test this prediction, the spatial variation of the cytoplasmic [Ca2+] transient will be assessed by the extensive use of different intracellular Ca2+ indicators which give different estimates of [Ca2+] when spatial gradients of [Ca2+] are present. 2) L1 should depend on Ca2+ loading of junctional SR. A signal arising directly from entering Ca2+, and not from Ca2+ released from SR, will be sought by pulsing high [Ca2+] solution onto single, isolated, Ca2+ depleted heart cells which contain a Ca2+ indicator. 3) The release of Ca2+ from deep SR, signalled by L2, should depend on L1 and not directly on membrane depolarization. To test this prediction, [Ca2+] transients will be studied in voltage-clamped, aequorin containing Purkinje fibers, and in fibers containing a Ca2+ buffer, quin2. (Quin2 will bind Ca2+ released from junctional SR; no other Ca2+ release should then occur). This research will reveal the extent of spatial gradients of [Ca2+] during E-C coupling and it will elucidate differences in E-C coupling between Purkinje fibers and ventricular tissue. It will permit determination of the roles of entering Ca2+ and Ca2+ induced Ca2+ release from the SR in intact tissue.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL029473-11
Application #
3340600
Study Section
Physiology Study Section (PHY)
Project Start
1982-01-01
Project End
1992-06-30
Budget Start
1991-07-01
Budget End
1992-06-30
Support Year
11
Fiscal Year
1991
Total Cost
Indirect Cost

  Institution

Name
University of Maryland Baltimore
Department
Type
Schools of Medicine
DUNS #
003255213
City
Baltimore
State
MD
Country
United States
Zip Code
21201

  Publications

Shorofsky, S R; Aggarwal, R; Corretti, M et al. (1999) Cellular mechanisms of altered contractility in the hypertrophied heart: big hearts, big sparks. Circ Res 84:424-34
Parker, I; Callamaras, N; Wier, W G (1997) A high-resolution, confocal laser-scanning microscope and flash photolysis system for physiological studies. Cell Calcium 21:441-52
Parker, I; Wier, W G (1997) Variability in frequency and characteristics of Ca2+ sparks at different release sites in rat ventricular myocytes. J Physiol 505 ( Pt 2):337-44
Wier, W G; ter Keurs, H E; Marban, E et al. (1997) Ca2+ 'sparks' and waves in intact ventricular muscle resolved by confocal imaging. Circ Res 81:462-9
Parker, I; Zang, W J; Wier, W G (1996) Ca2+ sparks involving multiple Ca2+ release sites along Z-lines in rat heart cells. J Physiol 497 ( Pt 1):31-8
Pratusevich, V R; Balke, C W (1996) Factors shaping the confocal image of the calcium spark in cardiac muscle cells. Biophys J 71:2942-57
Blatter, L A (1995) Depletion and filling of intracellular calcium stores in vascular smooth muscle. Am J Physiol 268:C503-12
Wier, W G (1995) Confocal microscopy reveals local SR calcium release in voltage-clamped cardiac cells. Adv Exp Med Biol 382:81-8
Shacklock, P S; Wier, W G; Balke, C W (1995) Local Ca2+ transients (Ca2+ sparks) originate at transverse tubules in rat heart cells. J Physiol 487 ( Pt 3):601-8
Lopez-Lopez, J R; Shacklock, P S; Balke, C W et al. (1995) Local calcium transients triggered by single L-type calcium channel currents in cardiac cells. Science 268:1042-5

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