Abstract

The overall aim of the proposed research is to investigate the cellular mechanisms responsible for the systolic and diastolic abnormalities of contraction sen in myocardial hypertrophy and failure. Abnormalities in calcium homeostasis have previously been demonstrated in animal models of hypertrophy and failure and in cells isolated from failing human hearts. However, these studies fail to identify the individual cellular processes that underlie these abnormalities. The important question is what step(s) in the coupling of membrane excitation with subsequent contraction and relaxation is (are) altered in hypertrophy and failure. Within the theoretical framework of a quantitative scheme of calcium homeostasis, the various steps of excitation-contraction-relaxation coupling will be individually probed by current methods in voltage clamping (whole-cell & single-channel), intracellular fluorescent calcium (Ca2+) indicators, and the flash photolysis of caged compounds.
The specific aims of the proposed research include: 1.) Test the hypothesis that the influx of Ca2+ through the L-type Ca2+-channel required to """"""""trigger"""""""" the release of Ca2+ from the sarcoplasmic reticulum (SR) is altered in hypertrophy and failure. This will involve measurement of both hole-cell and unitary Ca2+-currents. 2.) Test the hypothesis that the grading of the SR calcium release b the L-type Ca2+-current is altered in hypertrophy and failure. This will involve the measurement of single-channel Ca2+-currents and the simultaneous measurement of whole-cell calcium currents, intracellular calcium transients, and cell shortening. 3) Test the general hypothesis that the handling of Ca2+ by the SR is altered in hypertrophy and failure. Specifically, 3.1) test the hypothesis that the systolic abnormalities of contraction result from abnormalities of Ca2=-efflux from the SR Ca2+- release channel, and 3.2) test the hypothesis that the diastolic or relaxation abnormalities seen in hypertrophy and failure are the result of impaired sequestration of Ca2+ by athe SR Ca2+=ATP-ase pump. 4.) Test the hypothesis that the Ca2+-binding ligands (including the contractile regulatory proteins troponin C and calmodulin) are altered in hypertrophy and failure.
These specific aims will be investigated in single isolated myocytes from animal models of cardiac hypertrophy and failure and from failing human heart. This research addresses the fundamental question regarding the precise cellular mechanism(s) responsible for the altered contractility characteristic of hypertrophy and failure in a quantitative way.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
1R01HL050435-01A1
Application #
2226622
Study Section
Cardiovascular and Pulmonary Research A Study Section (CVA)
Project Start
1994-04-01
Project End
1998-03-31
Budget Start
1994-04-01
Budget End
1995-03-31
Support Year
1
Fiscal Year
1994
Total Cost
Indirect Cost

  Institution

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

  Publications

Armoundas, Antonis A; Rose, Jochen; Aggarwal, Rajesh et al. (2007) Cellular and molecular determinants of altered Ca2+ handling in the failing rabbit heart: primary defects in SR Ca2+ uptake and release mechanisms. Am J Physiol Heart Circ Physiol 292:H1607-18
Izu, Leighton T; Means, Shawn A; Shadid, John N et al. (2006) Interplay of ryanodine receptor distribution and calcium dynamics. Biophys J 91:95-112
Chen-Izu, Ye; McCulle, Stacey L; Ward, Chris W et al. (2006) Three-dimensional distribution of ryanodine receptor clusters in cardiac myocytes. Biophys J 91:1-13
Kirk, Malcolm M; Izu, Leighton T; Chen-Izu, Ye et al. (2003) Role of the transverse-axial tubule system in generating calcium sparks and calcium transients in rat atrial myocytes. J Physiol 547:441-51
Sha, Qun; Robinson, Shawn W; McCulle, Stacey L et al. (2003) An antisense oligonucleotide against H1 inhibits the classical sodium current but not ICa(TTX) in rat ventricular cells. J Physiol 547:435-40
Goldman, L; Balke, C W (2002) Do defects in the late sodium current in human ventricular cells cause heart failure? J Mol Cell Cardiol 34:1473-6
Chen-Izu, Y; Sha, Q; Shorofsky, S R et al. (2001) I(Ca(TTX)) channels are distinct from those generating the classical cardiac Na(+) current. Biophys J 81:2647-59
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
Aggarwal, R; Shorofsky, S R; Goldman, L et al. (1997) Tetrodotoxin-blockable calcium currents in rat ventricular myocytes; a third type of cardiac cell sodium current. J Physiol 505 ( Pt 2):353-69
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

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