Literature DB >> 17473172

Tbx3 controls the sinoatrial node gene program and imposes pacemaker function on the atria.

Willem M H Hoogaars1, Angela Engel, Janynke F Brons, Arie O Verkerk, Frederik J de Lange, L Y Elaine Wong, Martijn L Bakker, Danielle E Clout, Vincent Wakker, Phil Barnett, Jan Hindrik Ravesloot, Antoon F M Moorman, E Etienne Verheijck, Vincent M Christoffels.   

Abstract

The sinoatrial node initiates the heartbeat and controls the rate and rhythm of contraction, thus serving as the pacemaker of the heart. Despite the crucial role of the sinoatrial node in heart function, the mechanisms that underlie its specification and formation are not known. Tbx3, a transcriptional repressor required for development of vertebrates, is expressed in the developing conduction system. Here we show that Tbx3 expression delineates the sinoatrial node region, which runs a gene expression program that is distinct from that of the bordering atrial cells. We found lineage segregation of Tbx3-negative atrial and Tbx3-positive sinoatrial node precursor cells as soon as cardiac cells turn on the atrial gene expression program. Tbx3 deficiency resulted in expansion of expression of the atrial gene program into the sinoatrial node domain, and partial loss of sinoatrial node-specific gene expression. Ectopic expression of Tbx3 in mice revealed that Tbx3 represses the atrial phenotype and imposes the pacemaker phenotype on the atria. The mice displayed arrhythmias and developed functional ectopic pacemakers. These data identify a Tbx3-dependent pathway for the specification and formation of the sinoatrial node, and show that Tbx3 regulates the pacemaker gene expression program and phenotype.

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Year:  2007        PMID: 17473172      PMCID: PMC1855235          DOI: 10.1101/gad.416007

Source DB:  PubMed          Journal:  Genes Dev        ISSN: 0890-9369            Impact factor:   11.361


  59 in total

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Journal:  Cardiovasc Res       Date:  2004-06-01       Impact factor: 10.787

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  140 in total

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7.  Inducible gene deletion in the entire cardiac conduction system using Hcn4-CreERT2 BAC transgenic mice.

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