Abstract
Hypoplastic left heart syndrome (HLHS) is a severe congenital heart defect (CHD) that necessitates staged, single ventricle surgical palliation. An increased frequency of bicuspid aortic valve (BAV) has been observed among relatives. We postulated number of mutant alleles as a molecular basis for variable CHD expression in an extended family comprised of an HLHS proband and four family members who underwent echocardiography and whole-genome sequencing (WGS). Dermal fibroblast-derived induced pluripotent stem cells (iPSC) were procured from the proband–parent trio and bioengineered into cardiomyocytes. Cardiac phenotyping revealed aortic valve atresia and a slit-like left ventricular cavity in the HLHS proband, isolated bicuspid pulmonary valve in his mother, BAV in a maternal 4° relative, and no CHD in his father or sister. Filtering of WGS for rare, functional variants that segregated with CHD and were compound heterozygous in the HLHS proband identified NOTCH1 as the sole candidate gene. An unreported missense mutation (P1964L) in the cytoplasmic domain, segregating with semilunar valve malformation, was maternally inherited and a rare missense mutation (P1256L) in the extracellular domain, clinically silent in the heterozygous state, was paternally inherited. Patient-specific iPSCs exhibited diminished transcript levels of NOTCH1 signaling pathway components, impaired myocardiogenesis, and a higher prevalence of heterogeneous myofilament organization. Extended, phenotypically characterized families enable WGS-derived variant filtering for plausible Mendelian modes of inheritance, a powerful strategy to discover molecular underpinnings of CHD. Identification of compound heterozygous NOTCH1 mutations and iPSC-based functional modeling implicate mutant allele burden and impaired myogenic potential as mechanisms for HLHS.
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Introduction
The molecular basis of hypoplastic left heart syndrome (HLHS) is poorly understood. Characterized by an underdeveloped left ventricle, aortic and mitral valves, and aorta, children born with this severe congenital heart defect (CHD) require staged, single ventricle surgical palliation or cardiac transplantation for survival. The fundamental principle of blood flow-induced fetal cardiac growth suggests that HLHS could be caused by developmental arrest of myogenesis, valvulogenesis, and/or vasculogenesis. Although HLHS typically occurs as a sporadic, apparently non-Mendelian disorder, genetic underpinnings of HLHS are implicated by recurrence risks of 2–4 % in families with one affected child and 25 % in families with two affected children (Norwood et al. 1983). Furthermore, screening echocardiography in first-degree relatives has identified less severe, often asymptomatic CHD including bicuspid/stenotic aortic valve, hypoplastic aortic arch, and coarctation of the aorta (Loffredo et al. 2004; Wessels et al. 2005; McBride et al. 2005). Heterozygous NOTCH1 mutations have in fact been identified in patients with a spectrum of left-sided cardiac malformations, including HLHS (Garg et al. 2005; Mohamed et al. 2006; McKellar et al. 2007; McBride et al. 2008; Iascone et al. 2012; Foffa et al. 2014). Functional characterization of mutant Notch1 (G661S and A683T) in mouse fibroblasts did not demonstrate altered protein expression, but both mutations reduced ligand-induced signaling (McBride et al. 2008) and ultimately impaired the efficiency of epithelial to mesenchymal cell transition (EMT) (Riley et al. 2011). Incomplete penetrance of NOTCH1 missense mutations with extreme variability of intra- and inter-familial phenotypic expression implicates unknown genetic or environmental modifiers (Garg et al. 2005; McBride et al. 2008).
Here, we utilized whole-genome sequencing (WGS) for disease gene discovery in an extended, phenotypically characterized family comprised of a proband with HLHS and 1° and 4° relatives with semilunar valve malformations. This approach enabled inheritance-based filtering for rare, functional variants and revealed compound heterozygosity as an explanation for CHD severity. Procurement of induced pluripotent stem cells (iPSC) from the proband–parent trio provided for the first time a patient-specific cellular model of genetically defined HLHS, revealing impaired myogenic potential.
Methods
Study subjects
Five family members, including the proband with HLHS, provided written informed consent under a research protocol approved by the Mayo Clinic Institutional Review Board. Cardiac anatomy was assessed by two-dimensional echocardiography in all family members. Genomic deoxyribonucleic acid (DNA) was isolated from peripheral-blood white cells or saliva for all five family members and dermal fibroblasts were procured from the proband–parent trio.
Genomic and bioinformatics analyses
Array comparative genomic hybridization using a custom 180 K oligonucleotide microarray (Agilent, Santa Clara, CA) was performed on DNA from the proband with a genome-wide functional resolution of approximately 100 kilobases. Deletions larger than 200 kilobases and duplications larger than 500 kilobases were considered clinically relevant. WGS of DNA and variant call annotation were performed utilizing the Mayo Clinic Medical Genome Facility and Bioinformatics Core. Paired-end libraries were prepared using the TruSeq DNA v2 sample prep kit following the manufacturer’s protocol (Illumina, San Diego, CA). Each whole-genome library was loaded into four lanes of a flow cell and 101 base pair paired-end sequencing was carried out on Illumina’s HiSeq 2000 platform using TruSeq SBS sequencing kit version 3 and HiSeq data collection version 1.4.8 software. Reads were aligned to the hg19 reference genome using Novoalign version 2.08 (http://novocraft.com) and duplicate reads were marked using Picard (http://picard.sourceforge.net). Local realignment of insertion/deletions (INDELs) and base quality score recalibration were then performed using the Genome Analysis Toolkit version 1.6-9 (GATK) (McKenna et al. 2010). Single-nucleotide variants (SNV) and INDELs were called across all samples simultaneously using GATK’s Unified Genotyper with variant quality score recalibration (DePristo et al. 2011).
Variant call format files with SNV and INDEL calls from each individual were uploaded and analyzed using Ingenuity® Variant Analysis™ software (QIAGEN, Redwood City, CA, USA) where variants were functionally annotated and filtered by an iterative process. First, a filter was put into place to select for rare, high-quality heterozygous variants that (a) had a read depth of at least 10; (b) were not adjacent to a homopolymer exceeding 5 base pairs; (c) were present in <5 whole-exome sequencing (WES) datasets collected from 147 individuals not affected with HLHS; (d) were not identified within the top 1 % most exonically variable genes; and (e) were present at a frequency <1 % in the Exome Variant Server (WES data from 6503 individuals) (Exome Variant Server 2014) and/or 1000 Genomes (WGS data from 1092 individuals) (The 1000 Genomes Consortium 2012). Functional variants were defined as those that impacted a protein sequence, canonical splice site, microRNA coding sequence/binding site, enhancer region, or transcription factor binding site within a promoter validated by ENCODE chromatin immunoprecipitation experiments (Raney et al. 2014). Using WGS data from five family members, rare functional variants were then filtered for (a) segregation with CHD and (b) compound heterozygosity in the HLHS proband.
Linkage analysis
All five family members underwent genotyping and locus mapping using the Omni1 (I.1, I.2, II.1 and II.2) or Omni 2.5 (I.3) SNV chip. The average call rate for SNVs and individuals was greater than 98 %. A total of 593,743 SNVs overlapped between genotyping chips and had a call rate over 95 % with a minor allele frequency (MAF) among the genotyped individuals above 5 %. Genomic positions from Rutgers were incorporated into the data for linkage analysis (Matise et al. 2007). The number of SNVs was reduced to 13,991 when imposing the following criteria: MAF greater than 20 %, Hardy–Weinberg P > 10−5, and pairwise r 2 < 0.05. Population allele frequencies for linkage analysis were retrieved from the CEU population in the November 23, 2010 release of the 1000 genomes data (The 1000 Genomes Consortium 2012). Data were prepared using SAS (version 9.3, SAS Institute, Cary, NC), R (vesion 3.0.2, R Foundation for Statistical Computing, Vienna, Austria), PLINK (version 1.07) and VCFTools (version 0.1.7) (Purcell et al. 2007; Danacek et al. 2011). Parametric linkage analyses were performed with Merlin (Version 1.1.2) (Abecasis et al. 2002), modeling dominant inheritance and specifying the following variables: phenocopy rate 0.005, dichotomous liability classes (‘affected’ and ‘unaffected’) and a 100 % penetrance model.
iPSC and patient-specific cardiomyocyte analysis
Cell culture Reprogrammed iPSCs (ReGen Theranostics, Rochester, MN) from the proband–parent trio were maintained on mouse embryonic fibroblasts in DMEM/F12 supplemented with 20 % KOSR, recombinant human FGF basic (20 ng/ml; R&D Systems, Minneapolis, MN), non-essential amino acids (EMD Millipore, Billerica, MA), L-glutamax, and 2-mercaptoethanol (Sigma, St. Louis, MO). Unless specified otherwise, cell culture reagents were purchased from Invitrogen (Carlsbad, CA). For comparison of mRNA transcript levels in iPSCs, all clones were adapted to mTeSR (StemCell Technologies, Vancouver, British Columbia) prior to sample collection. To differentiate iPSCs into the cardiac lineage, cells were cultured for one passage on Geltrex (LDEV-Free, hESC-qualified, reduced growth factor) in MEF-conditioned medium (iPSC maintenance medium conditioned for 24 h by MEFs) for depletion of feeder cells, then dissociated using TrypLE Select and plated as a monolayer. At confluence, the medium was changed to RPMI supplemented with B27 (minus insulin), which served as the maintenance medium for differentiating cells. For days 0–4 of cardiac differentiation, Activin A (10 ng/ml; R&D Systems) and BMP4 (20 ng/ml; R&D Systems) were included in the medium. To obtain cardiomyocytes from the proband’s iPSCs for myofilament analysis, medium was supplemented with Activin A (100 ng/ml) for the first 24 h, and for days 1–5 the differentiation medium included BMP4 (10 ng/ml) and FGF basic (5 ng/ml). The differentiating cells were maintained in 5 % oxygen for days 0–14. All iPSC-derived cardiomyocytes were transferred to coverslips at day 30 and harvested at day 50.
Gene expression Total RNA was extracted with TRIzol Reagent (Invitrogen) and purified using a Qiagen RNeasy Mini Kit. cDNA synthesis was completed using reagents supplied in the iScript cDNA Synthesis Kit (Bio-Rad Laboratories, Hercules, CA).
qPCR reactions consisted of cDNA, TaqMan Universal PCR Master Mix (Life Technologies, Carlsbad, CA), and PrimeTime predesigned assay primers (Integrated DNA Technologies, Inc., Coralville, IA), and were completed using an Applied Biosystems 7500 Real-Time PCR System. Primer sets included HES1 (Hs.PT.56a.4181121), HEY1 (Hs.PT.56a.4299267.g), NOTCH1-intracellular domain (Hs.PT.58.39600723), and GAPDH (Hs.PT.39a.22214836).
Immunofluorescent staining iPSCs and iPSC cardiomyocytes were fixed with 4 % paraformaldehyde (Sigma), permeabilized with 0.5 % Tween20 (Sigma) and blocked overnight with SuperBlock Blocking Buffer. Primary antibodies included Sox2 (EMD Millipore), SSEA3 (Stemgent, Cambridge, MA), and Tra-1-60 (EMD Millipore) for iPSCs, and α-actinin (clone EA-53; Sigma) and sarcomeric myosin heavy chain (MF20) (Developmental Studies Hybridoma Bank, Iowa City, IA) for iPSC cardiomyocytes. Secondary antibodies were conjugated with an Alexa Fluor® 488, 568, or 633 dye. Samples were mounted with ProLong® antifade reagent with DAPI. Images were acquired on a Zeiss LSM 510 Meta confocal microscope.
Flow cytometry Differentiating iPSCs were dissociated into a single cell suspension by treatment with Worthington Biochemical Type 2 Collagenase II followed by 0.05 % Gibco® Trypsin–EDTA, and then exposed to the LIVE/DEAD® Fixable Near-IR Dead Cell Stain. Cells were fixed and permeabilized using IntraPrep (Beckman Coulter, Indianapolis, IN) and stained with MF20 Alexa Fluor® 488 (eBioscience, San Diego, CA). Data were collected with a Gallios flow cytometer (Beckman Coulter) and analyzed with Kaluza 1.2.
Statistics Data are presented as the mean ± SEM. Significant differences were calculated with a two-tailed Student’s t test with Welch’s correction when appropriate using Prism5 (Graphpad Software, La Jolla, CA). A P < 0.05 was considered significant.
Results
Family phenotype
We identified and phenotypically characterized a family of White European ancestry, comprised of three individuals with CHD of varying severity (Fig. 1). On the first day of life, the proband (II.2) was diagnosed with HLHS with severe mitral stenosis, aortic valve atresia, slit-like left ventricular cavity, and hypoplastic ascending aorta (4 mm diameter). He had no apparent extra-cardiac abnormalities. His 1° family members underwent screening echocardiography for our research study. His mother (I.2) was asymptomatic with a bicuspid pulmonary valve (BPV) and his father (I.1) and sister (II.1) had no CHD. Family history and medical records review revealed a 4° maternal relative (I.3) previously diagnosed with BAV at age 32, who underwent aortic valve replacement at age 41 for progressive calcific aortic valve stenosis. Maternal history was notable for two prior miscarriages at 8 and 11 weeks gestation.
Whole-genome sequencing and bioinformatics analysis
Array comparative genomic hybridization analysis excluded aneuploidy in the HLHS proband. To identify pathogenic coding or regulatory SNVs or INDELs, WGS was carried out on all five family members. Each sample yielded approximately 1.5 billion 101 base paired-end reads which passed quality control standards with 95 % of the reads mapping to the genome. After marking and filtering out duplicate reads, over 99 % of the hg19 human reference genome had coverage. The average depth across the genome was 42X and an average of 95 % of the gene body regions (exons, introns, and 5′ and 3′ untranslated regions) demonstrated a minimal read depth of 20 reads. Each family member had approximately 5 million variants which, upon filtering for rarity, function and mode of inheritance, were reduced to two missense mutations in the HLHS proband (Fig. 2). Both mutations were identified in NOTCH1, encoding neurogenic locus notch homolog protein 1. The mutation on the paternal allele localized to extracellular EGF-like domain 32 (exon 23: c.3767 C > T, p.P1256L), while the mutation on the maternal allele localized to the intracellular ankyrin 2 domain (exon 31: c.5891 C > T, p.P1964L) (Fig. 3a). NOTCH1 has a residual variant intolerance score of 0.33 %, indicating its tolerance of genetic variation is less than 99 % of other genes (Petrovski et al. 2013), and the altered amino acid residues are highly conserved across species (Fig. 3b). NOTCH1-P1964L, an unreported mutation that segregated with variably expressed CHD, was predicted to be damaging by both SIFT (Ng and Henikoff 2001) and Polyphen2 (Adzhubei et al. 2010). NOTCH1-P1256L was also identified in the unaffected father and sibling and, while predicted to be benign by SIFT (Ng and Henikoff 2001) and Polyphen2 (Adzhubei et al. 2010) is extremely rare in 28,800 ethnically matched, unrelated European (Non-Finnish) individuals who comprise the Exome Aggregation Consortium (ExAC) database (allele frequency = 0.000048) (Fig. 3c) (Exome Aggregation Consortium 2015).
Linkage analysis
To validate our findings and ensure that mutations in equally plausible candidate genes were not missed by poor WGS coverage, we performed linkage analysis recognizing that the family was underpowered for conclusive locus mapping. We identified seven equally plausible loci (peak LOD scores of 1.1) based on haplotypes shared by the three family members with CHD but not the proband’s unaffected sibling. The five loci spanned 1421 genes, one of which was NOTCH1. The candidacy of all 1421 genes was assessed based on an established association with CHD, utilizing the Ingenuity® Variant Analysis™ software Knowledge Base, a manually curated resource that integrates data from top-tier scientific literature. In addition to NOTCH1, there were 25 other genes associated with CHD. However, none of these genes harbored a rare functional mutation. Visual inspection of the raw data utilizing the Integrated Genomics Viewer (Robinson et al. 2011) revealed ample coverage of each gene, verifying that the segregating NOTCH1 mutation was the sole candidate.
In vitro modeling
Dermal samples were collected from the father, mother, and proband and fibroblast outgrowths were expanded in culture for a brief period prior to reprogramming with a cocktail of lentiviruses carrying POU5F/OCT4, SOX2, KLF4, or c-MYC. After a period of approximately 3 weeks, colonies with morphology similar to human embryonic stem cells (hESCs) were selected and expanded. Each established clone was characterized by immunofluorescent staining for standard pluripotency markers including SSEA-3, Tra-1-60, and Sox2 (Fig. 4a), as well as Oct4 and Nanog (data not shown), yielding three clones for the proband, three clones for the mother and two clones for the father which underwent further experimentation. Because it has been reported that several Notch signaling pathway components are expressed in hESCs (Yu et al. 2008), the mRNA transcript levels for NOTCH1 and its downstream targets HES1 and HEY1 were measured by RT-qPCR. The expression levels of these components were similar among the clones established for both parents. In contrast, the levels of these components were approximately twofold lower in the proband compared to parents (NOTCH1 P = 0.005, HES1 P = 0.008, and HEY1, P = 0.007) (Fig. 4b). These data indicate that the Notch signaling pathway is dysregulated in the proband’s iPSCs. Next, all iPSC clones were differentiated into the cardiovascular lineages starting from a monolayer of cells and using an adaptive protocol that combines Activin A and BMP4 in RPMI-based differentiation medium for the first 4 days, followed by maintenance in unmodified differentiation medium (Fig. 4c). By day 16, robust areas of beating were observed in the iPSC clones from the parents, and small beating clusters were observed with the iPSC clones from the proband. At day 20, the differentiated cells were dissociated into a single cell suspension and analyzed by flow cytometry to determine the percentage of cardiomyocytes within the cell population based on the expression of MF20. On average, 65 % of the cells were MF20+ in the iPSC clones for the parents, whereas only 17 % of the cells were MF20+ with the iPSC clones from the proband (P < 0.0001) (Fig. 4d). For a final assessment, the myofibril organization of d50 iPSC cardiomyocytes was examined by immunocytochemistry for the sarcomeric protein α-actinin. In comparison to the iPSC-derived cardiomyocytes obtained from the parents (n = 195), those obtained from the proband’s iPSCs (n = 208) had a higher percentage of cells (42 vs. 11 %) in which sarcomeric α-actinin exhibited either a punctate staining pattern or short fragmented myofibrils in greater than one-fourth of the total cellular area (P = 0.03) (Fig. 4e). However, no differences were observed in the size of the iPSC cardiomyocytes, which is similar to what has been reported for iPSCs from patients with dilated cardiomyopathy (Sun et al. 2012).
Discussion
Role of NOTCH1 in cardiac development
NOTCH1, encoding neurogeneic locus notch homolog protein 1, is a single-pass transmembrane receptor in the evolutionarily conserved Notch signaling pathway that has been shown to play a vital role in murine cardiac development (High and Epstein 2008). Activation results in its cleavage and nuclear translocation of the intracellular domain to guide transcription of downstream targets, which are required during multiple phases of cardiogenesis. During ventricular morphogenesis, elevated expression of Notch1 in the developing trabeculae is critical for differentiation of cardiomyocytes and proper development of the ventricular chambers (Grego-Bessa et al. 2007). Notch1 is also necessary for cardiac valvulogenesis due to its role in EMT, a transformation of cells required for proper development of cardiac valves (Timmerman et al. 2004). Mice lacking functional protein due to a targeted homozygous Notch1 mutation die at embryonic day 10.5 (Swiatek et al. 1994) with a collapsed endocardium and paucity of mesenchymal cushion cells due to severe impairment of EMT (Timmerman et al. 2004). The association of NOTCH1 with valvulogenesis was also observed in zebrafish where its constitutive activation lead to hypercellular cardiac valves (Timmerman et al. 2004).
Heterozygous NOTCH1 mutations in CHD
NOTCH1 mutations associated with abnormal cardiac development were first identified by genome-wide locus mapping and mutation scanning in two families with a spectrum of autosomal dominant CHDs including BAV, ventricular septal defect, tetralogy of Fallot, mitral stenosis, and mitral atresia with left ventricular hypoplasia and double outlet right ventricle (Garg et al. 2005). Within each family, identification of a heterozygous nonsense or frameshift mutation resulted in a truncated NOTCH1 transcript. Subsequent candidate gene studies identified thirteen heterozygous mutations in NOTCH1 in individuals with BAV (Mohamed et al. 2006; McKellar et al. 2007; McBride et al. 2008; Foffa et al. 2014), aortic valve stenosis (McBride et al. 2008), coarctation of the aorta (McBride et al. 2008), or HLHS (McBride et al. 2008; Iascone et al. 2012). Ten were missense mutations (eight extracellular, two cytoplasmic), all reported at low frequencies in ~60,000 individuals who make up the ExAC database (allele frequencies = 0.000008–0.013), supporting their role as CHD susceptibility alleles with variable expressivity. In contrast, three were unreported loss of function mutations, including an inherited nonsense mutation in two family members with BAV (Foffa et al. 2014) and de novo frameshift and splice site mutations in two unrelated probands with HLHS (Iascone et al. 2012). Functional characterization of two of the missense mutations, each linked to diverse CHDs and reported in ExAC (A683T = 0.0028 and G661S = 0.038), demonstrated impaired EMT due to perturbed downstream Notch1 signaling (Riley et al. 2011). To our knowledge, genetic or environmental factors that modify phenotypic expression of NOTCH1 mutations and account for the severe HLHS phenotype have not been identified previously.
Compound heterozygous NOTCH1 mutations and impaired myogenic potential in HLHS
Using WGS and a family-based variant filtering approach, we demonstrate for the first time compound heterozygous NOTCH1 mutations in a patient with HLHS. Our strategy enabled a comprehensive survey of essentially all genes with no a priori assumptions of gene candidates or disease mechanisms. While advances are being made in elucidating the complex genetics of CHD, complete understanding of its genetic underpinnings remains a challenge due, in part, to modifier genes/mutations. WGS is now able to provide all of the unique variants in a personal genome, but pinpointing those which are involved in the pathogenesis of CHD is not a simple task (Gelb and Chung. 2014). Here, we capitalized on maternal segregation of variably expressed CHD, using the unaffected sibling as a subtractive filter, and specified compound heterozygosity in the HLHS proband as a plausible inheritance model. This provided robust evidence for NOTCH1 as the top candidate, without imposing filters based on imprecise in silico predictions of a variant’s biological significance. The unreported P1964L mutation on the maternal allele segregated with BPV and BAV in other family members and is the first identified CHD-associated NOTCH1 mutation to reside within the intracellular ankyrin repeat domain, disrupting a highly conserved consensus motif in the first helix of ankyrin repeat 2 (Ehebauer et al. 2005). To our knowledge, it is also the first NOTCH1 mutation associated with pulmonary valve malformation, implicating a role of NOTCH1 signaling in right heart development. The P1256L mutation on the paternal allele is rare but clinically silent in the father and sibling. This is consistent with other CHD-associated NOTCH1 missense mutations that are present in control databases and variably penetrant (Mohamed et al. 2006; McKellar et al. 2007; McBride et al. 2008; Foffa et al. 2014). Our genetic data suggested a genotype–phenotype relationship whereby mutant allele burden may determine the degree of NOTCH1 signaling impairment and corresponding severity of phenotypic expression. We speculate that synergistic heterozygosity for mutations in different NOTCH1 signaling protein genes could underlie other cases of HLHS.
To validate that the identified compound heterozygous NOTCH1 mutations could significantly contribute to HLHS, an in vitro platform was created to screen the cardiogenicity of patient-specific iPSCs and examine the myofilament organization of the iPSC-derived cardiomyocytes for disease-susceptibility characteristics. Comparison of NOTCH1 transcript levels and two of its primary effectors in iPSCs bioengineered from the proband and parents indicated that the Notch signaling pathway was dysregulated in the proband. As a consequence, the iPSC-derived cardiomyocyte yield was diminished in conditions that supported cardiomyogenesis. Moreover, in vitro culture of the iPSC cardiomyocytes from the HLHS proband led to increased sarcomeric disorganization and myofibril disarray. While these data did not achieve statistical significance when comparing the mother and father, it is plausible that a single heterozygous mutation in NOTCH1 confers subtle changes in its expression and activity that require more sensitive assays and/or additional clones. Our findings are consistent with two previous studies that have reported reduced cardiomyocyte yields and a higher prevalence of myofibril disorganization in iPSCs derived from patients with HLHS compared to unrelated controls (Jiang et al. 2014; Kobayashi et al. 2014). Uniquely, our study is the first to model genetically defined HLHS with iPSC-derived cardiomyocytes using parental cells as controls, providing further evidence for impaired myogenic potential as a mechanism for HLHS.
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The authors gratefully acknowledge the patients and family members who participated in this study.
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Informed consent was obtained from all individual participants included in the study.
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Todd and Karen Wanek Family Program for Hypoplastic Left Heart Syndrome, Mayo Clinic Foundation.
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Mayo Clinic and Timothy J. Nelson have a Financial Conflict of Interest managed according to established policies in the context of licensed technology to ReGen Theranostics, Inc.
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Theis, J.L., Hrstka, S.C.L., Evans, J.M. et al. Compound heterozygous NOTCH1 mutations underlie impaired cardiogenesis in a patient with hypoplastic left heart syndrome. Hum Genet 134, 1003–1011 (2015). https://doi.org/10.1007/s00439-015-1582-1
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DOI: https://doi.org/10.1007/s00439-015-1582-1