Cardiac muscle cells typically express three myosin isoforms, designated as V1 (high ATPase), V2, and V3 (low ATPase). The pattern of this expression is thought to regulate the intrinsic functional properties of the heart in a wide range of species. Although thyroid hormone (T3) is known to be the chief """"""""up"""""""" regulator of V1 expression, recent findings suggest that high carbohydrate provision can also serve as an """"""""up"""""""" regulator independent of T3 under certain conditions. Since the dependency of carbohydrate as a major energy source appears to be greater in rodents exercised by swimming as opposed to running, factors associated with carbohydrate metabolism in the heart may be critical in accounting for the higher degree of """"""""up"""""""" regulation of V1 expression that occurs in response to training by the former as compared to the latter. The goal of this proposal is to test the hypothesis that the pattern of cardiac isoform expression in response to exercise training is regulated in accordance with the relative degree that carbohydrates contribute to the total energy requirement of the heart during exercise. To test this hypothesis, a series of experiments are proposed using animal models with either """"""""up"""""""" or """"""""down"""""""" regulated cardiac myosin expression in which the utilization potential of carbohydrate by the heart during exercise will be either increased or decreased. This will be accomplished by dietary manipulation coupled with pharmacologic blockers impacting on processes associated with either carbohydrate mobilization or metabolism. Measurements on appropriate nontrained and trained groups of the various manipulated models will focus on cardiac myosin ATPase and isoform expression in the context of the animal's thyroid status and steady state resting and exercise cardiac metabolic patterns. These experiments will thus integrate the important variable of substrate energy provision with the exercise stimulus in expanding our understanding of cardiac myosin isoform regulation.

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL038819-05
Application #
3355214
Study Section
Respiratory and Applied Physiology Study Section (RAP)
Project Start
1987-07-01
Project End
1992-06-30
Budget Start
1991-07-01
Budget End
1992-06-30
Support Year
5
Fiscal Year
1991
Total Cost
Indirect Cost
Name
University of California Irvine
Department
Type
Schools of Medicine
DUNS #
161202122
City
Irvine
State
CA
Country
United States
Zip Code
92697
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Baldwin, K M; Haddad, F (2001) Effects of different activity and inactivity paradigms on myosin heavy chain gene expression in striated muscle. J Appl Physiol 90:345-57
Wright, C E; Haddad, F; Qin, A X et al. (1999) In vivo regulation of beta-MHC gene in rodent heart: role of T3 and evidence for an upstream enhancer. Am J Physiol 276:C883-91
Haddad, F; Qin, A X; McCue, S A et al. (1998) Thyroid receptor plasticity in striated muscle types: effects of altered thyroid state. Am J Physiol 274:E1018-26
Haddad, F; Masatsugu, M; Bodell, P W et al. (1997) Role of thyroid hormone and insulin in control of cardiac isomyosin expression. J Mol Cell Cardiol 29:559-69
Haddad, F; Bodell, P W; McCue, S A et al. (1997) Effects of diabetes on rodent cardiac thyroid hormone receptor and isomyosin expression. Am J Physiol 272:E856-63
Baldwin, K M (1996) Effects of altered loading states on muscle plasticity: what have we learned from rodents? Med Sci Sports Exerc 28:S101-6
Swoap, S J; Boddell, P; Baldwin, K M (1995) Interaction of hypertension and caloric restriction on cardiac mass and isomyosin expression. Am J Physiol 268:R33-9
Swoap, S J; Haddad, F; Bodell, P et al. (1995) Control of beta-myosin heavy chain expression in systemic hypertension and caloric restriction in the rat heart. Am J Physiol 269:C1025-33
Haddad, F; Bodell, P W; Baldwin, K M (1995) Pressure-induced regulation of myosin expression in rodent heart. J Appl Physiol 78:1489-95

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