Patient-independent human induced pluripotent stem cell model: A new tool for rapid determination of genetic variant pathogenicity in long QT syndrome

Nikhil V Chavali; Dmytro O Kryshtal; Shan S Parikh; Lili Wang; Andrew M Glazer; Daniel J Blackwell; Brett M Kroncke; Moore Benjamin Shoemaker; Bjorn C Knollmann

doi:10.1016/j.hrthm.2019.04.031

Patient-independent human induced pluripotent stem cell model: A new tool for rapid determination of genetic variant pathogenicity in long QT syndrome

Heart Rhythm. 2019 Nov;16(11):1686-1695. doi: 10.1016/j.hrthm.2019.04.031. Epub 2019 Apr 18.

Authors

Nikhil V Chavali¹, Dmytro O Kryshtal², Shan S Parikh¹, Lili Wang², Andrew M Glazer², Daniel J Blackwell², Brett M Kroncke², Moore Benjamin Shoemaker², Bjorn C Knollmann³

Affiliations

¹ Vanderbilt University School of Medicine, Nashville, Tennessee; Vanderbilt Center for Arrhythmia Research and Therapeutics, Department of Medicine, Nashville, Tennessee.
² Vanderbilt Center for Arrhythmia Research and Therapeutics, Department of Medicine, Nashville, Tennessee.
³ Vanderbilt University School of Medicine, Nashville, Tennessee; Vanderbilt Center for Arrhythmia Research and Therapeutics, Department of Medicine, Nashville, Tennessee. Electronic address: bjorn.knollmann@vanderbilt.edu.

Abstract

Background: Commercial genetic testing for long QT syndrome (LQTS) has rapidly expanded, but the inability to accurately predict whether a rare variant is pathogenic has limited its clinical benefit. Novel missense variants are routinely reported as variant of unknown significance (VUS) and cannot be used to screen family members at risk for sudden cardiac death. Better approaches to determine the pathogenicity of VUS are needed.

Objective: The purpose of this study was to rapidly determine the pathogenicity of a CACNA1C variant reported by commercial genetic testing as a VUS using a patient-independent human induced pluripotent stem cell (hiPSC) model.

Methods: Using CRISPR/Cas9 genome editing, CACNA1C-p.N639T was introduced into a previously established hiPSC from an unrelated healthy volunteer, thereby generating a patient-independent hiPSC model. Three independent heterozygous N639T hiPSC lines were generated and differentiated into cardiomyocytes (CM). Electrophysiological properties of N639T hiPSC-CM were compared to those of isogenic and population control hiPSC-CM by measuring the extracellular field potential (EFP) of 96-well hiPSC-CM monolayers and by patch clamp.

Results: Significant EFP prolongation was observed only in optically stimulated but not in spontaneously beating N639T hiPSC-CM. Patch-clamp studies revealed that N639T prolonged the ventricular action potential by slowing voltage-dependent inactivation of Ca_V1.2 currents. Heterologous expression studies confirmed the effect of N639T on Ca_V1.2 inactivation.

Conclusion: The patient-independent hiPSC model enabled rapid generation of functional data to support reclassification of a CACNA1C VUS to likely pathogenic, thereby establishing a novel LQTS type 8 mutation. Furthermore, our results indicate the importance of controlling beating rates to evaluate the functional significance of LQTS VUS in high-throughput hiPSC-CM assays.

Keywords: Action potential; Extracellular field potential; Human induced pluripotent stem cells; L-type Ca current; Long QT syndrome type 8.

Publication types

Case Reports
Research Support, N.I.H., Extramural
Research Support, Non-U.S. Gov't

MeSH terms

Action Potentials
Calcium Channels, L-Type / genetics*
Child
Clustered Regularly Interspaced Short Palindromic Repeats
Female
Gene Editing
Genetic Testing
Genetic Variation*
Humans
Induced Pluripotent Stem Cells*
Long QT Syndrome / genetics*
Long QT Syndrome / pathology*
Pedigree
Phenotype

Substances

CACNA1C protein, human
Calcium Channels, L-Type

Abstract

Publication types

MeSH terms

Substances

Grants and funding