Abstract

Receptors for many cardiac hormones and neurotransmitters are coupled to their effector enzymes and ion channels by a family of heterotrimeric GDP-binding proteins (G proteins made up of alpha and betagamma subunits. These proteins act as critical control points for directing signals initiated at the cell surface to specific intracellular second messenger pathways. They are essential for normal cardiac function, and their derangement in pathological states may contribute to abnormal responses of the heart to some agonists. In the past project period, we have created strains of transgenic mice carrying mutated G protein subunits targeted to the heart. One set of animals expressing a constitutively activated, HA epitope-tagged Galpha subunit (HAalpha/q*) develops cardiac hypertrophy, dilation and failure. Surprisingly, we found that expression of HAalpha/q* was transient, being present at 2 weeks in atria and ventricles, and becoming undetectable by 10 weeks of age. At 2 weeks of age when the product of the transgene is expressed, the hearts are essentially normal morphologically, but not functionally. This early transient expression of HAALPHA/q* causes pathological changes that continue and that worsen despite the fact that the level of HAalpha/q* drops. These mice provide a powerful, novel system in which to dissect primary from secondary changes leading to cardiac hypertrophy and eventually to failure. A major challenge is to define how changes that begin in the cardiomyocyte lead to changes in non-myocyte cells to produce the full-blown global cardiac pathology. Ultimately, the persistent pathology must be the result of persistent changes in the activity of sets of genes. A major long-term goal will be to use the system that we have developed to identify novel genes involved in the initiation and continuation of cardiac dilatation hypertrophy and the transition to failure, and to understand how changes in their function determine the pathology. Ultimately, the persistent pathology must be the result of persistent changes in the activity of sets of genes. A major long-term goal will be to use the system that we have developed to identify novel genes involved in the initiation and continuation of cardiac dilatation hypertrophy and the transition to failure, and to understand how changes in their function determine the pathology.
The Specific Aims are: 1) To define the mechanisms that link transient expression of constitutively activated alpha/1 in cardiac myocytes to persistent, fatal cardiac pathology. 2) To define the change in gene expression profile in cardiomyocytes from transgenic animals expressing HAalpha1* at an age when pathology is minimal and when it is severe. Transgenic animals will also be compared to age- and sex-matched wild-type animals. 3) To define the effect of increased alpha/1 signaling on development of hypertrophy through an independent pathway.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Specialized Center (P50)
Project #
2P50HL052320-06
Application #
6302290
Study Section
Project Start
2000-02-07
Project End
2001-01-31
Budget Start
Budget End
Support Year
6
Fiscal Year
2000
Total Cost
$214,676
Indirect Cost

  Institution

Name
Brigham and Women's Hospital
Department
Type
DUNS #
071723621
City
Boston
State
MA
Country
United States
Zip Code
02115

  Publications

Herman, Daniel S; Lam, Lien; Taylor, Matthew R G et al. (2012) Truncations of titin causing dilated cardiomyopathy. N Engl J Med 366:619-28
Alcalai, Ronny; Wakimoto, Hiroko; Arad, Michael et al. (2011) Prevention of ventricular arrhythmia and calcium dysregulation in a catecholaminergic polymorphic ventricular tachycardia mouse model carrying calsequestrin-2 mutation. J Cardiovasc Electrophysiol 22:316-24
Pinz, Ilka; Zhu, Ming; Mende, Ulrike et al. (2011) An improved isolation procedure for adult mouse cardiomyocytes. Cell Biochem Biophys 61:93-101
Shen, Weiqun; Vatner, Dorothy E; Vatner, Stephen F et al. (2010) Progressive loss of creatine maintains a near normal DeltaG approximately (ATP) in transgenic mouse hearts with cardiomyopathy caused by overexpressing Gsalpha. J Mol Cell Cardiol 48:591-9
Saltzman, Adam J; Mancini-DiNardo, Debora; Li, Chumei et al. (2010) Short communication: the cardiac myosin binding protein C Arg502Trp mutation: a common cause of hypertrophic cardiomyopathy. Circ Res 106:1549-52
Gnecchi, Massimiliano; He, Huamei; Melo, Luis G et al. (2009) Early beneficial effects of bone marrow-derived mesenchymal stem cells overexpressing Akt on cardiac metabolism after myocardial infarction. Stem Cells 27:971-9
Pinz, Ilka; Ostroy, Sanford E; Hoyer, Kirsten et al. (2008) Calcineurin-induced energy wasting in a transgenic mouse model of heart failure. Am J Physiol Heart Circ Physiol 294:H1459-66
Pinz, Ilka; Robbins, Jeffrey; Rajasekaran, Namakkal S et al. (2008) Unmasking different mechanical and energetic roles for the small heat shock proteins CryAB and HSPB2 using genetically modified mouse hearts. FASEB J 22:84-92
Pinz, Ilka; Wax, Stephen D; Anderson, Paul et al. (2008) Low over-expression of TNFalpha in the mouse heart increases contractile performance via TNFR1. J Cell Biochem 105:99-107
Hoyer, Kirsten; Krenz, Maike; Robbins, Jeffrey et al. (2007) Shifts in the myosin heavy chain isozymes in the mouse heart result in increased energy efficiency. J Mol Cell Cardiol 42:214-21

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