Effects of irbesartan on gene expression revealed by transcriptome analysis of left atrial tissue in a porcine model of acute rapid pacing in vivo

Ravi Kumar Chilukoti; Jörg Mostertz; Alicja Bukowska; Christoph Aderkast; Stephan B Felix; Matthias Busch; Uwe Völker; Andreas Goette; Carmen Wolke; Georg Homuth; Uwe Lendeckel

doi:10.1016/j.ijcard.2013.01.007

Effects of irbesartan on gene expression revealed by transcriptome analysis of left atrial tissue in a porcine model of acute rapid pacing in vivo

Int J Cardiol. 2013 Oct 3;168(3):2100-8. doi: 10.1016/j.ijcard.2013.01.007. Epub 2013 Feb 12.

Authors

Ravi Kumar Chilukoti¹, Jörg Mostertz, Alicja Bukowska, Christoph Aderkast, Stephan B Felix, Matthias Busch, Uwe Völker, Andreas Goette, Carmen Wolke, Georg Homuth, Uwe Lendeckel

Affiliation

¹ University Medicine, Ernst-Moritz-Arndt-University Greifswald, Interfaculty Institute for Genetics and Functional Genomics, Greifswald, Germany.

PMID: 23414741
DOI: 10.1016/j.ijcard.2013.01.007

Abstract

Background: Atrial fibrillation (AF) is characterized by electrical and structural remodeling of the atria with atrial fibrosis being one hallmark. Angiotensin II (AngII) is a major contributing factor and blockage of its type I receptor (AT1R) prevents remodeling to some extent. Here we explored the effects of the AT1R antagonist irbesartan on global gene expression and profibrotic signaling pathways after induction of rapid atrial pacing (RAP) in vivo in pigs.

Methods and results: Microarray-based RNA profiling was used to screen left atrial (LA) tissue specimens for differences in atrial gene expression in a model of acute RAP. RAP caused an overall expression profile that reflected AngII-induced ROS production, tissue remodeling, and energy depletion. Of special note, the mRNA levels of EDN1, SGK1, and CTGF encoding pro-endothelin, stress- and glucocorticoid activated kinase-1, and of connective tissue growth factor were identified to be significantly increased after 7h of rapid pacing. These specific expression changes were additionally validated by RT-qPCR or immunoblot analyses in LA, RA, and partly in LV samples. All RAP-induced differential gene expression patterns were partially attenuated in the presence of irbesartan. Similar results were obtained after RAP of HL-1 cardiomyocytes in vitro. Furthermore, exogenously added endothelin-1 (ET1) induced CTGF expression concomitant to the transcriptional activation of SGK1 in HL-1 cells.

Conclusions: RAP provokes substantial changes in atrial and ventricular myocardial gene expression that could be partly reversed by irbesartan. ET1 contributes to AF-dependent atrial fibrosis by synergistic activity with AngII to stimulate SGK1 expression and enhance phosphorylation of the SGK1 protein which, in turn, induces CTGF. The latter has been consistently associated with tissue fibrosis. These findings suggest ETR antagonists as being beneficial in AF treatment.

Keywords: Acute atrial tachyarrhythmia; Angiotensin; Atrial fibrillation; CTGF; Endothelin; SGK1.

MeSH terms

Angiotensin II
Angiotensin II Type 1 Receptor Blockers / pharmacology
Animals
Atrial Fibrillation / drug therapy
Atrial Fibrillation / genetics*
Atrial Fibrillation / physiopathology
Biphenyl Compounds / pharmacology*
Blotting, Western
Cell Line
Connective Tissue Growth Factor / biosynthesis
Connective Tissue Growth Factor / genetics*
Disease Models, Animal
Gene Expression Profiling / methods*
Gene Expression Regulation / drug effects*
Heart Atria / drug effects
Heart Atria / metabolism*
Heart Atria / pathology
Heart Rate
Irbesartan
Mice
Microarray Analysis
Myocytes, Cardiac / metabolism
Myocytes, Cardiac / pathology
RNA, Messenger / genetics*
Reverse Transcriptase Polymerase Chain Reaction
Swine
Tetrazoles / pharmacology*

Substances

Angiotensin II Type 1 Receptor Blockers
Biphenyl Compounds
RNA, Messenger
Tetrazoles
Angiotensin II
Connective Tissue Growth Factor
Irbesartan