Correlation Between Myofilament Response to Ca2+ and Altered Dynamics of Contraction and Relaxation in Transgenic Cardiac Cells That Express beta-Tropomyosin

We compared the dynamics of the contraction and relaxation of single myocytes isolated from nontransgenic (NTG) mouse hearts and from transgenic (TG-beta-Tm) mouse hearts that overexpress the skeletal isoform of tropomyosin (Tm). Compared with NTG controls, TG-beta-Tm myocytes showed significantly r...

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Published in:	Circulation research Vol. 84; no. 7; pp. 745 - 751
Main Authors:	Wolska, Beata M, Keller, Rebecca S, Evans, Christian C, Palmiter, Kimberly A, Phillips, Ronald M, Muthuchamy, Mariappan, Oehlenschlager, James, Wieczorek, David F, de Tombe, Pieter P, Solaro, R. John
Format:	Journal Article
Language:	English
Published:	Hagerstown, MD American Heart Association, Inc 16-04-1999 Lippincott
Subjects:	Actin Cytoskeleton - drug effects Actin Cytoskeleton - physiology Adenosine Triphosphatases - metabolism Animals Biological and medical sciences Calcium - pharmacology Fundamental and applied biological sciences. Psychology Gene Expression - physiology Heart In Vitro Techniques Mice Mice, Inbred Strains Mice, Transgenic Muscle Contraction - drug effects Muscle Contraction - physiology Muscle Fibers, Skeletal - cytology Muscle Fibers, Skeletal - drug effects Muscle Fibers, Skeletal - enzymology Myocardium - cytology Myocardium - enzymology Sarcomeres - chemistry Sarcomeres - enzymology Tropomyosin - genetics Tropomyosin - metabolism Vertebrates: cardiovascular system Heart Molecular form Myofibril Tropomyosin Rodentia Transgenic animal Gene overexpression Muscle contraction Myocyte Muscular relaxation Vertebrata Mammalia Mouse Circulatory system Sarcomere
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Summary:	We compared the dynamics of the contraction and relaxation of single myocytes isolated from nontransgenic (NTG) mouse hearts and from transgenic (TG-beta-Tm) mouse hearts that overexpress the skeletal isoform of tropomyosin (Tm). Compared with NTG controls, TG-beta-Tm myocytes showed significantly reduced maximal rates of contraction and relaxation with no change in the extent of shortening. This result indicated that the depression in contraction dynamics determined in TG-beta-Tm isolated hearts is intrinsic to the cells. To further investigate the effect of Tm isoform switching on myofilament activity and regulation, we measured myofilament force and ATPase rate as functions of pCa (-log of [Ca]). Compared with controls, force generated by myofilaments from TG-beta-Tm hearts and myofibrillar ATPase activity were both more sensitive to Ca. However, the shift in pCa50 (half-maximally activating pCa) caused by changing sarcomere length from 1.8 to 2.4 [micro sign]m was not significantly different between NTG and TG-beta-Tm fiber preparations. To test directly whether isoform switching affected the economy of contraction, force versus ATPase rate relationships were measured in detergent-extracted fiber bundles. In both NTG and TG-beta-Tm preparations, force and ATPase rate were linear and identically correlated, which indicated that crossbridge turnover was unaffected by Tm isoform switching. However, detergent extracted fibers from TG-beta-Tm demonstrated significantly less maximum tension and ATPase activity than NTG controls. Our results provide the first evidence that the Tm isoform population modulates the dynamics of contraction and relaxation of single myocytes by a mechanism that does not alter the rate-limiting step of crossbridge detachment. Our results also indicate that differences in sarcomere-length dependence of activation between cardiac and skeletal muscle are not likely due to differences in the isoform population of Tm. (Circ Res. 1999;84:745-751.)
Bibliography:	ObjectType-Article-1 SourceType-Scholarly Journals-1 ObjectType-Feature-2 content type line 23
ISSN:	0009-7330 1524-4571