A Variant Noncoding Region Regulates Prrx1 and Predisposes to Atrial Arrhythmias

Fernanda M. Bosada; Mathilde R. Rivaud; Jae-Sun Uhm; Sander Verheule; Karel van Duijvenboden; Arie O. Verkerk; Vincent M. Christoffels; Bastiaan J. Boukens

doi:10.1161/circresaha.121.319146

A Variant Noncoding Region Regulates Prrx1 and Predisposes to Atrial Arrhythmias

Fernanda M. Bosada, Mathilde R. Rivaud, Jae-Sun Uhm, Sander Verheule, Karel van Duijvenboden, Arie O. Verkerk, Vincent M. Christoffels^*, Bastiaan J. Boukens^*

^*Corresponding author for this work

Research output: Contribution to journal › Article › Academic › peer-review

Abstract

RATIONALE: Atrial fibrillation (AF) is the most common cardiac arrhythmia diagnosed in clinical practice. Genome-wide association studies have identified AF-associated common variants across 100+ genomic loci, but the mechanism underlying the impact of these variant loci on AF susceptibility in vivo has remained largely undefined. One such variant region, highly associated with AF, is found at 1q24, close to PRRX1, encoding the paired-related homeobox 1 transcription factor.

OBJECTIVE: To identify the mechanistic link between the variant region at 1q24 and AF predisposition.

METHODS AND RESULTS: The mouse orthologue of the noncoding variant genomic region (R1A) at 1q24 was deleted using CRISPR genome editing. Among the genes sharing the topologically associated domain with the deleted R1A region (Kifap3, Prrx1, Fmo2, and Prrc2c), only the broadly expressed gene Prrx1 was downregulated in mutants, and only in cardiomyocytes. Expression and epigenetic profiling revealed that a cardiomyocyte lineage-specific gene program (Mhrt, Myh6, Rbm20, Tnnt2, Ttn, and Ckm) was upregulated in R1A(-/-) atrial cardiomyocytes and that Mef2 (myocyte enhancer factor)-binding motifs were significantly enriched at differentially accessible chromatin sites. Consistently, Prrx1 suppressed Mef2-activated enhancer activity in HL-1 cells. Mice heterozygous or homozygous for the R1A deletion were susceptible to atrial arrhythmia induction, had atrial conduction slowing and more irregular RR intervals. Isolated R1A(-/-) mouse left atrial cardiomyocytes showed lower action potential upstroke velocities and sodium current, as well as increased systolic and diastolic calcium concentrations compared with controls.

CONCLUSIONS: The noncoding AF variant region at 1q24 modulates Prrx1 expression in cardiomyocytes. Cardiomyocyte-specific reduction of Prrx1 expression upon deletion of the noncoding region leads to a profound induction of a cardiac lineage-specific gene program and to propensity for AF. These data indicate that AF-associated variants in humans may exert AF predisposition through reduced PRRX1 expression in cardiomyocytes.

Original language	English
Pages (from-to)	420-434
Number of pages	15
Journal	Circulation Research
Volume	129
Issue number	3
DOIs	https://doi.org/10.1161/circresaha.121.319146
Publication status	Published - 23 Jul 2021

Keywords

atrial fibrillation
chromatin
electrophysiology
gene expression
transcription factors
HOMEOBOX GENE
HOMEODOMAIN PROTEIN
MESSENGER-RNA
FIBRILLATION
COMMON
LOCI
MHOX
RISK
SKELETOGENESIS
EPIDEMIOLOGY

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10.1161/circresaha.121.319146

Cite this

@article{0e98fd1d66834ec5a9116d5ec41e7251,

title = "A Variant Noncoding Region Regulates Prrx1 and Predisposes to Atrial Arrhythmias",

abstract = "RATIONALE: Atrial fibrillation (AF) is the most common cardiac arrhythmia diagnosed in clinical practice. Genome-wide association studies have identified AF-associated common variants across 100+ genomic loci, but the mechanism underlying the impact of these variant loci on AF susceptibility in vivo has remained largely undefined. One such variant region, highly associated with AF, is found at 1q24, close to PRRX1, encoding the paired-related homeobox 1 transcription factor.OBJECTIVE: To identify the mechanistic link between the variant region at 1q24 and AF predisposition.METHODS AND RESULTS: The mouse orthologue of the noncoding variant genomic region (R1A) at 1q24 was deleted using CRISPR genome editing. Among the genes sharing the topologically associated domain with the deleted R1A region (Kifap3, Prrx1, Fmo2, and Prrc2c), only the broadly expressed gene Prrx1 was downregulated in mutants, and only in cardiomyocytes. Expression and epigenetic profiling revealed that a cardiomyocyte lineage-specific gene program (Mhrt, Myh6, Rbm20, Tnnt2, Ttn, and Ckm) was upregulated in R1A(-/-) atrial cardiomyocytes and that Mef2 (myocyte enhancer factor)-binding motifs were significantly enriched at differentially accessible chromatin sites. Consistently, Prrx1 suppressed Mef2-activated enhancer activity in HL-1 cells. Mice heterozygous or homozygous for the R1A deletion were susceptible to atrial arrhythmia induction, had atrial conduction slowing and more irregular RR intervals. Isolated R1A(-/-) mouse left atrial cardiomyocytes showed lower action potential upstroke velocities and sodium current, as well as increased systolic and diastolic calcium concentrations compared with controls.CONCLUSIONS: The noncoding AF variant region at 1q24 modulates Prrx1 expression in cardiomyocytes. Cardiomyocyte-specific reduction of Prrx1 expression upon deletion of the noncoding region leads to a profound induction of a cardiac lineage-specific gene program and to propensity for AF. These data indicate that AF-associated variants in humans may exert AF predisposition through reduced PRRX1 expression in cardiomyocytes.",

keywords = "atrial fibrillation, chromatin, electrophysiology, gene expression, transcription factors, HOMEOBOX GENE, HOMEODOMAIN PROTEIN, MESSENGER-RNA, FIBRILLATION, COMMON, LOCI, MHOX, RISK, SKELETOGENESIS, EPIDEMIOLOGY",

author = "Bosada, {Fernanda M.} and Rivaud, {Mathilde R.} and Jae-Sun Uhm and Sander Verheule and {van Duijvenboden}, Karel and Verkerk, {Arie O.} and Christoffels, {Vincent M.} and Boukens, {Bastiaan J.}",

note = "Funding Information: This work was supported by Foundation Leducq 14CVD01, CONCOR-GENES CVON2014-18, and ZonMW TOP 91217061 (to V.M. Christoffels); Dutch Heart Foundation 2016T047 (to B.J. Boukens); and CVON2014-18 CONCOR-GENES YTP (to F.M. Bosada). Publisher Copyright: {\textcopyright} 2021 Lippincott Williams and Wilkins. All rights reserved.",

year = "2021",

month = jul,

day = "23",

doi = "10.1161/circresaha.121.319146",

language = "English",

volume = "129",

pages = "420--434",

journal = "Circulation Research",

issn = "0009-7330",

publisher = "LIPPINCOTT WILLIAMS & WILKINS",

number = "3",

}

TY - JOUR

T1 - A Variant Noncoding Region Regulates Prrx1 and Predisposes to Atrial Arrhythmias

AU - Bosada, Fernanda M.

AU - Rivaud, Mathilde R.

AU - Uhm, Jae-Sun

AU - Verheule, Sander

AU - van Duijvenboden, Karel

AU - Verkerk, Arie O.

AU - Christoffels, Vincent M.

AU - Boukens, Bastiaan J.

N1 - Funding Information: This work was supported by Foundation Leducq 14CVD01, CONCOR-GENES CVON2014-18, and ZonMW TOP 91217061 (to V.M. Christoffels); Dutch Heart Foundation 2016T047 (to B.J. Boukens); and CVON2014-18 CONCOR-GENES YTP (to F.M. Bosada). Publisher Copyright: © 2021 Lippincott Williams and Wilkins. All rights reserved.

PY - 2021/7/23

Y1 - 2021/7/23

N2 - RATIONALE: Atrial fibrillation (AF) is the most common cardiac arrhythmia diagnosed in clinical practice. Genome-wide association studies have identified AF-associated common variants across 100+ genomic loci, but the mechanism underlying the impact of these variant loci on AF susceptibility in vivo has remained largely undefined. One such variant region, highly associated with AF, is found at 1q24, close to PRRX1, encoding the paired-related homeobox 1 transcription factor.OBJECTIVE: To identify the mechanistic link between the variant region at 1q24 and AF predisposition.METHODS AND RESULTS: The mouse orthologue of the noncoding variant genomic region (R1A) at 1q24 was deleted using CRISPR genome editing. Among the genes sharing the topologically associated domain with the deleted R1A region (Kifap3, Prrx1, Fmo2, and Prrc2c), only the broadly expressed gene Prrx1 was downregulated in mutants, and only in cardiomyocytes. Expression and epigenetic profiling revealed that a cardiomyocyte lineage-specific gene program (Mhrt, Myh6, Rbm20, Tnnt2, Ttn, and Ckm) was upregulated in R1A(-/-) atrial cardiomyocytes and that Mef2 (myocyte enhancer factor)-binding motifs were significantly enriched at differentially accessible chromatin sites. Consistently, Prrx1 suppressed Mef2-activated enhancer activity in HL-1 cells. Mice heterozygous or homozygous for the R1A deletion were susceptible to atrial arrhythmia induction, had atrial conduction slowing and more irregular RR intervals. Isolated R1A(-/-) mouse left atrial cardiomyocytes showed lower action potential upstroke velocities and sodium current, as well as increased systolic and diastolic calcium concentrations compared with controls.CONCLUSIONS: The noncoding AF variant region at 1q24 modulates Prrx1 expression in cardiomyocytes. Cardiomyocyte-specific reduction of Prrx1 expression upon deletion of the noncoding region leads to a profound induction of a cardiac lineage-specific gene program and to propensity for AF. These data indicate that AF-associated variants in humans may exert AF predisposition through reduced PRRX1 expression in cardiomyocytes.

AB - RATIONALE: Atrial fibrillation (AF) is the most common cardiac arrhythmia diagnosed in clinical practice. Genome-wide association studies have identified AF-associated common variants across 100+ genomic loci, but the mechanism underlying the impact of these variant loci on AF susceptibility in vivo has remained largely undefined. One such variant region, highly associated with AF, is found at 1q24, close to PRRX1, encoding the paired-related homeobox 1 transcription factor.OBJECTIVE: To identify the mechanistic link between the variant region at 1q24 and AF predisposition.METHODS AND RESULTS: The mouse orthologue of the noncoding variant genomic region (R1A) at 1q24 was deleted using CRISPR genome editing. Among the genes sharing the topologically associated domain with the deleted R1A region (Kifap3, Prrx1, Fmo2, and Prrc2c), only the broadly expressed gene Prrx1 was downregulated in mutants, and only in cardiomyocytes. Expression and epigenetic profiling revealed that a cardiomyocyte lineage-specific gene program (Mhrt, Myh6, Rbm20, Tnnt2, Ttn, and Ckm) was upregulated in R1A(-/-) atrial cardiomyocytes and that Mef2 (myocyte enhancer factor)-binding motifs were significantly enriched at differentially accessible chromatin sites. Consistently, Prrx1 suppressed Mef2-activated enhancer activity in HL-1 cells. Mice heterozygous or homozygous for the R1A deletion were susceptible to atrial arrhythmia induction, had atrial conduction slowing and more irregular RR intervals. Isolated R1A(-/-) mouse left atrial cardiomyocytes showed lower action potential upstroke velocities and sodium current, as well as increased systolic and diastolic calcium concentrations compared with controls.CONCLUSIONS: The noncoding AF variant region at 1q24 modulates Prrx1 expression in cardiomyocytes. Cardiomyocyte-specific reduction of Prrx1 expression upon deletion of the noncoding region leads to a profound induction of a cardiac lineage-specific gene program and to propensity for AF. These data indicate that AF-associated variants in humans may exert AF predisposition through reduced PRRX1 expression in cardiomyocytes.

KW - atrial fibrillation

KW - chromatin

KW - electrophysiology

KW - gene expression

KW - transcription factors

KW - HOMEOBOX GENE

KW - HOMEODOMAIN PROTEIN

KW - MESSENGER-RNA

KW - FIBRILLATION

KW - COMMON

KW - LOCI

KW - MHOX

KW - RISK

KW - SKELETOGENESIS

KW - EPIDEMIOLOGY

U2 - 10.1161/circresaha.121.319146

DO - 10.1161/circresaha.121.319146

M3 - Article

C2 - 34092116

SN - 0009-7330

VL - 129

SP - 420

EP - 434

JO - Circulation Research

JF - Circulation Research

IS - 3

ER -