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Physiol. Genomics 26: 109-115, 2006. First published May 2, 2006; doi:10.1152/physiolgenomics.00281.2005
1094-8341/06 $8.00
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Received 12 November 2005; accepted in final form 19 April 2006.
Physiological Genomics 26:109-115 (2006)
1094-8341/06 $8.00 © 2006 American Physiological Society

Differential regional gene expression from cardiac dyssynchrony induced by chronic right ventricular free wall pacing in the mouse

Kenneth C. Bilchick1, Sudip K. Saha1, Ed Mikolajczyk3, Leslie Cope2, Will J. Ferguson4, Wayne Yu2, Steven Girouard3 and David A. Kass1

1 Division of Cardiology, Department of Medicine, School of Medicine, Baltimore, Maryland
2 Sidney Kimmel Comprehensive Cancer Center, Johns Hopkins University, Baltimore, Maryland
3 Guidant Corporation, St. Paul, Minnesota
4 Agilent Technologies, Columbia, Maryland

Routine clinical right ventricular pacing generates left ventricular dyssynchrony manifested by early septal shortening followed by late lateral contraction, which, in turn, reciprocally stretches the septum. Dyssynchrony is disadvantageous to cardiac mechanoenergetics and worsens clinical prognosis, yet little is known about its molecular consequences. Here, we report the influence of cardiac dyssynchrony on regional cardiac gene expression in mice. Mice were implanted with a custom-designed miniature cardiac pacemaker and subjected to 1-wk overdrive right ventricular free wall pacing (720 beats/min, baseline heart rate 520–620 beats/min) to generate dyssynchrony (pacemaker: 3-V lithium battery, rate programmable, 1.5 g, bipolar lead). Electrical capture was confirmed by pulsed-wave Doppler and dyssynchrony by echocardiography. Gene expression from the left ventricular septal and lateral wall myocardium was assessed by microarray (dual-dye method, Agilent) using oligonucleotide probes and dye swap. Identical analysis was applied to four synchronously contracting controls. Of the 22,000 genes surveyed, only 18 genes displayed significant (P < 0.01) differential expression between septal/lateral walls >1.5 times that in synchronous controls. Gene changes were confirmed by quantitative PCR with excellent correlations. Most of the genes (n = 16) showed greater septal expression. Of particular interest were seven genes coding proteins involved with stretch responses, matrix remodeling, stem cell differentiation to myocyte lineage, and Purkinje fiber differentiation. One week of iatrogenic cardiac dyssynchrony triggered regional differential expression in relatively few select genes. Such analysis using a murine implantable pacemaker should facilitate molecular studies of cardiac dyssynchrony and help elucidate novel mechanisms by which stress/stretch stimuli due to dyssynchrony impact the normal and failing heart.

microarray; heart; activation timing




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