Silencing of CCR4-NOT complex subunits affects heart structure and function

Lisa Elmén; Claudia B. Volpato; Anaïs Kervadec; Santiago Pineda; Sreehari Kalvakuri; Nakissa N. Alayari; Luisa Foco; Peter P. Pramstaller; Karen Ocorr; Alessandra Rossini; Anthony Cammarato; Alexandre R. Colas; Andrew A. Hicks; Rolf Bodmer

doi:10.1242/dmm.044727

Silencing of CCR4-NOT complex subunits affects heart structure and function

Lisa Elmén, Claudia B. Volpato, Anaïs Kervadec, Santiago Pineda, Sreehari Kalvakuri, Nakissa N. Alayari, Luisa Foco, Peter P. Pramstaller, Karen Ocorr, Alessandra Rossini, Anthony Cammarato, Alexandre R. Colas, Andrew A. Hicks, Rolf Bodmer

School of Medicine

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

5 Scopus citations

Abstract

The identification of genetic variants that predispose individuals to cardiovascular disease and a better understanding of their targets would be highly advantageous. Genome-wide association studies have identified variants that associate with QT-interval length (a measure of myocardial repolarization). Three of the strongest associating variants (single-nucleotide polymorphisms) are located in the putative promotor region of CNOT1, a gene encoding the central CNOT1 subunit of CCR4-NOT: a multifunctional, conserved complex regulating gene expression and mRNA stability and turnover. We isolated the minimum fragment of the CNOT1 promoter containing all three variants from individuals homozygous for the QT risk alleles and demonstrated that the haplotype associating with longer QT interval caused reduced reporter expression in a cardiac cell line, suggesting that reduced CNOT1 expression might contribute to abnormal QT intervals. Systematic siRNA-mediated knockdown of CCR4-NOT components in human induced pluripotent stem cell-derived cardiomyocytes (hiPSC-CMs) revealed that silencing CNOT1 and other CCR4-NOT genes reduced their proliferative capacity. Silencing CNOT7 also shortened action potential duration. Furthermore, the cardiac-specific knockdown of Drosophila orthologs of CCR4-NOT genes in vivo (CNOT1/Not1 and CNOT7/8/Pop2) was either lethal or resulted in dilated cardiomyopathy, reduced contractility or a propensity for arrhythmia. Silencing CNOT2/Not2, CNOT4/Not4 and CNOT6/6L/twin also affected cardiac chamber size and contractility. Developmental studies suggested that CNOT1/Not1 and CNOT7/8/Pop2 are required during cardiac remodeling from larval to adult stages. To summarize, we have demonstrated how disease-associated genes identified by GWAS can be investigated by combining human cardiomyocyte cell-based and whole-organism in vivo heart models. Our results also suggest a potential link of CNOT1 and CNOT7/8 to QT alterations and further establish a crucial role of the CCR4-NOT complex in heart development and function.

Original language	English (US)
Article number	dmm044727
Journal	DMM Disease Models and Mechanisms
Volume	13
Issue number	7
DOIs	https://doi.org/10.1242/dmm.044727
State	Published - Jul 2020

Keywords

Arrhythmia
CNOT1
Cardiomyocytes
Drosophila heart
GWAS
HiPSC
Long-QT syndrome

ASJC Scopus subject areas

Neuroscience (miscellaneous)
Medicine (miscellaneous)
Immunology and Microbiology (miscellaneous)
General Biochemistry, Genetics and Molecular Biology

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10.1242/dmm.044727

Cite this

Elmén, L., Volpato, C. B., Kervadec, A., Pineda, S., Kalvakuri, S., Alayari, N. N., Foco, L., Pramstaller, P. P., Ocorr, K., Rossini, A., Cammarato, A., Colas, A. R., Hicks, A. A., & Bodmer, R. (2020). Silencing of CCR4-NOT complex subunits affects heart structure and function. DMM Disease Models and Mechanisms, 13(7), Article dmm044727. https://doi.org/10.1242/dmm.044727

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title = "Silencing of CCR4-NOT complex subunits affects heart structure and function",

abstract = "The identification of genetic variants that predispose individuals to cardiovascular disease and a better understanding of their targets would be highly advantageous. Genome-wide association studies have identified variants that associate with QT-interval length (a measure of myocardial repolarization). Three of the strongest associating variants (single-nucleotide polymorphisms) are located in the putative promotor region of CNOT1, a gene encoding the central CNOT1 subunit of CCR4-NOT: a multifunctional, conserved complex regulating gene expression and mRNA stability and turnover. We isolated the minimum fragment of the CNOT1 promoter containing all three variants from individuals homozygous for the QT risk alleles and demonstrated that the haplotype associating with longer QT interval caused reduced reporter expression in a cardiac cell line, suggesting that reduced CNOT1 expression might contribute to abnormal QT intervals. Systematic siRNA-mediated knockdown of CCR4-NOT components in human induced pluripotent stem cell-derived cardiomyocytes (hiPSC-CMs) revealed that silencing CNOT1 and other CCR4-NOT genes reduced their proliferative capacity. Silencing CNOT7 also shortened action potential duration. Furthermore, the cardiac-specific knockdown of Drosophila orthologs of CCR4-NOT genes in vivo (CNOT1/Not1 and CNOT7/8/Pop2) was either lethal or resulted in dilated cardiomyopathy, reduced contractility or a propensity for arrhythmia. Silencing CNOT2/Not2, CNOT4/Not4 and CNOT6/6L/twin also affected cardiac chamber size and contractility. Developmental studies suggested that CNOT1/Not1 and CNOT7/8/Pop2 are required during cardiac remodeling from larval to adult stages. To summarize, we have demonstrated how disease-associated genes identified by GWAS can be investigated by combining human cardiomyocyte cell-based and whole-organism in vivo heart models. Our results also suggest a potential link of CNOT1 and CNOT7/8 to QT alterations and further establish a crucial role of the CCR4-NOT complex in heart development and function.",

keywords = "Arrhythmia, CNOT1, Cardiomyocytes, Drosophila heart, GWAS, HiPSC, Long-QT syndrome",

author = "Lisa Elm{\'e}n and Volpato, {Claudia B.} and Ana{\"i}s Kervadec and Santiago Pineda and Sreehari Kalvakuri and Alayari, {Nakissa N.} and Luisa Foco and Pramstaller, {Peter P.} and Karen Ocorr and Alessandra Rossini and Anthony Cammarato and Colas, {Alexandre R.} and Hicks, {Andrew A.} and Rolf Bodmer",

note = "Funding Information: This study was supported by the National Institutes of Health (R01-HL054732 to R.B.; R01-HL124091 to A.C.; R01-HL132241 to K.O.), the Wanek Foundation (R.B. and A.C.) and the Department of Innovation, Research and Universities of the Autonomous Province of Bolzano-South Tyrol (Italy) (C.B.V., L.F., A.R. and A.A.H.). Funding Information: This study was supported by the National Institutes of Health (R01-HL054732 to R.B.; R01-HL124091 to A.C.; R01-HL132241 to K.O.), the Wanek Foundation (R.B. and A.C.) and the Department of Innovation, Research and Universities of the Autonomous Province of Bolzano-South Tyrol (Italy) (C.B.V., L.F., A.R. and A.A.H.). The authors thank the Department of Innovation, Research and University of the Autonomous Province of Bozen/Bolzano for covering the Open Access publication costs. Publisher Copyright: {\textcopyright} 2020. Published by The Company of Biologists Ltd",

year = "2020",

month = jul,

doi = "10.1242/dmm.044727",

language = "English (US)",

volume = "13",

journal = "DMM Disease Models and Mechanisms",

issn = "1754-8403",

publisher = "Company of Biologists Ltd",

number = "7",

}

TY - JOUR

T1 - Silencing of CCR4-NOT complex subunits affects heart structure and function

AU - Elmén, Lisa

AU - Volpato, Claudia B.

AU - Kervadec, Anaïs

AU - Pineda, Santiago

AU - Kalvakuri, Sreehari

AU - Alayari, Nakissa N.

AU - Foco, Luisa

AU - Pramstaller, Peter P.

AU - Ocorr, Karen

AU - Rossini, Alessandra

AU - Cammarato, Anthony

AU - Colas, Alexandre R.

AU - Hicks, Andrew A.

AU - Bodmer, Rolf

N1 - Funding Information: This study was supported by the National Institutes of Health (R01-HL054732 to R.B.; R01-HL124091 to A.C.; R01-HL132241 to K.O.), the Wanek Foundation (R.B. and A.C.) and the Department of Innovation, Research and Universities of the Autonomous Province of Bolzano-South Tyrol (Italy) (C.B.V., L.F., A.R. and A.A.H.). Funding Information: This study was supported by the National Institutes of Health (R01-HL054732 to R.B.; R01-HL124091 to A.C.; R01-HL132241 to K.O.), the Wanek Foundation (R.B. and A.C.) and the Department of Innovation, Research and Universities of the Autonomous Province of Bolzano-South Tyrol (Italy) (C.B.V., L.F., A.R. and A.A.H.). The authors thank the Department of Innovation, Research and University of the Autonomous Province of Bozen/Bolzano for covering the Open Access publication costs. Publisher Copyright: © 2020. Published by The Company of Biologists Ltd

PY - 2020/7

Y1 - 2020/7

N2 - The identification of genetic variants that predispose individuals to cardiovascular disease and a better understanding of their targets would be highly advantageous. Genome-wide association studies have identified variants that associate with QT-interval length (a measure of myocardial repolarization). Three of the strongest associating variants (single-nucleotide polymorphisms) are located in the putative promotor region of CNOT1, a gene encoding the central CNOT1 subunit of CCR4-NOT: a multifunctional, conserved complex regulating gene expression and mRNA stability and turnover. We isolated the minimum fragment of the CNOT1 promoter containing all three variants from individuals homozygous for the QT risk alleles and demonstrated that the haplotype associating with longer QT interval caused reduced reporter expression in a cardiac cell line, suggesting that reduced CNOT1 expression might contribute to abnormal QT intervals. Systematic siRNA-mediated knockdown of CCR4-NOT components in human induced pluripotent stem cell-derived cardiomyocytes (hiPSC-CMs) revealed that silencing CNOT1 and other CCR4-NOT genes reduced their proliferative capacity. Silencing CNOT7 also shortened action potential duration. Furthermore, the cardiac-specific knockdown of Drosophila orthologs of CCR4-NOT genes in vivo (CNOT1/Not1 and CNOT7/8/Pop2) was either lethal or resulted in dilated cardiomyopathy, reduced contractility or a propensity for arrhythmia. Silencing CNOT2/Not2, CNOT4/Not4 and CNOT6/6L/twin also affected cardiac chamber size and contractility. Developmental studies suggested that CNOT1/Not1 and CNOT7/8/Pop2 are required during cardiac remodeling from larval to adult stages. To summarize, we have demonstrated how disease-associated genes identified by GWAS can be investigated by combining human cardiomyocyte cell-based and whole-organism in vivo heart models. Our results also suggest a potential link of CNOT1 and CNOT7/8 to QT alterations and further establish a crucial role of the CCR4-NOT complex in heart development and function.

AB - The identification of genetic variants that predispose individuals to cardiovascular disease and a better understanding of their targets would be highly advantageous. Genome-wide association studies have identified variants that associate with QT-interval length (a measure of myocardial repolarization). Three of the strongest associating variants (single-nucleotide polymorphisms) are located in the putative promotor region of CNOT1, a gene encoding the central CNOT1 subunit of CCR4-NOT: a multifunctional, conserved complex regulating gene expression and mRNA stability and turnover. We isolated the minimum fragment of the CNOT1 promoter containing all three variants from individuals homozygous for the QT risk alleles and demonstrated that the haplotype associating with longer QT interval caused reduced reporter expression in a cardiac cell line, suggesting that reduced CNOT1 expression might contribute to abnormal QT intervals. Systematic siRNA-mediated knockdown of CCR4-NOT components in human induced pluripotent stem cell-derived cardiomyocytes (hiPSC-CMs) revealed that silencing CNOT1 and other CCR4-NOT genes reduced their proliferative capacity. Silencing CNOT7 also shortened action potential duration. Furthermore, the cardiac-specific knockdown of Drosophila orthologs of CCR4-NOT genes in vivo (CNOT1/Not1 and CNOT7/8/Pop2) was either lethal or resulted in dilated cardiomyopathy, reduced contractility or a propensity for arrhythmia. Silencing CNOT2/Not2, CNOT4/Not4 and CNOT6/6L/twin also affected cardiac chamber size and contractility. Developmental studies suggested that CNOT1/Not1 and CNOT7/8/Pop2 are required during cardiac remodeling from larval to adult stages. To summarize, we have demonstrated how disease-associated genes identified by GWAS can be investigated by combining human cardiomyocyte cell-based and whole-organism in vivo heart models. Our results also suggest a potential link of CNOT1 and CNOT7/8 to QT alterations and further establish a crucial role of the CCR4-NOT complex in heart development and function.

KW - Arrhythmia

KW - CNOT1

KW - Cardiomyocytes

KW - Drosophila heart

KW - GWAS

KW - HiPSC

KW - Long-QT syndrome

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Silencing of CCR4-NOT complex subunits affects heart structure and function

Abstract

Keywords

ASJC Scopus subject areas

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