Introduction

Molecular Medicine Reports

1791-2997 1791-3004

D.A. Spandidos

10.3892/mmr.2017.6592

mmr-16-01-0410

Articles

Whole-exome sequencing identifies a novel mutation (R367G) in SCN5A to be associated with familial cardiac conduction disease

Rong

1 Fan

Xue-Feng

2 Chen

Chan

1 Liu

Zheng-Hua

1Department of Anesthesiology, The Second Xiangya Hospital of Central South University, Changsha, Hunan 410011, P.R. China 2Department of Orthopaedics, Xiangya Hospital, Central South University, Changsha, Hunan 410010, P.R. China 3Department of Thoracic Surgery, The Second Xiangya Hospital of Central South University, Changsha, Hunan 410011, P.R. China

Correspondence to: Dr Zheng-Hua Liu, Department of Thoracic Surgery, The Second Xiangya Hospital of Central South University, 139 Ren Ming Road, Changsha, Hunan 410011, P.R. China, E-mail: 911fanfan@sina.com

072017

17052017

16 1 410 414 16042016 16032017

2017

Cardiac conduction disease is a primary cause of sudden cardiac death. Sodium voltage-gated channel-α subunit 5 (SCN5A) mutations have been reported to underlie a variety of inherited arrhythmias. Numerous disease-causing mutations of SCN5A have been identified in patients with ≥10 different conditions, including type 3 long-QT syndrome and Brugada syndrome. The present study investigated a family with a history of arrhythmia, with the proband having a history of arrhythmia and syncope. Whole-exome sequencing was applied in order to detect the disease-causing mutation in this family, and Sanger sequencing was used to confirm the co-segregation among the family members. A missense mutation (c.1099C>G/p.R367G) of SCN5A was identified in the family and was observed to be co-segregated in all affected members of the family. The missense mutation results in a substitution of glycine for arginine, which may affect sodium transmembrane transport. The present study provides an accurate genetic test which may be used in individuals who exhibit no clinical symptoms.

sodium voltage-gated channel-α subunit 5 arrhythmia whole-exome sequencing arrhythmia-associated gene filtering

Introduction

Cardiac conduction disease is the major risk factor for sudden cardiac death (SCD), and therefore is the primary cause of mortality from SCD worldwide (1,2). The principal characteristics of the disease are sudden arrhythmia and syncope (3). The human voltage-gated cardiac sodium channel serves a role in cardiac conduction, and mutations in sodium channel genes have been demonstrated to be associated with cardiac conduction disease (4), including sodium voltage-gated channel-α subunit 5 (SCN5A) (5), sodium voltage-gated channel-β subunit 4 (6) and sodium voltage-gated channel-β subunit 1 (7).

The gene SCN5A encodes the pore-forming subunit of the human cardiac sodium channel NaV1.5 (8) and mutations in this gene have been reported to be associated with a variety of arrhythmogenic disorders, including type 3 long-QT syndrome (9), atrial fibrillation (10), dilated cardiomyopathy (11), Brugada syndrome (8) and certain complex overlapping disorders (12).

The present study investigated a clinically-characterized family with a history of syncope and arrhythmia. A clear autosomal-dominant inheritance of arrhythmia had been identified in the family. Using whole-exome sequencing (WES), in combination with arrhythmia-associated gene filtering, a novel missense mutation (c.1099C>G/p.R367G) was identified in SCN5A, which may underlie the pathogenesis of this type of familial arrhythmia.

Materials and methods <sec> <title>Patients and subjects

The protocol of the present study was approved by the Review Board of the Second Xiangya Hospital of Central South University (Changsha, China) and the study participants gave informed consent. A total of 14 members of the family (5 affected, 7 unaffected and 2 unknown) were enrolled in the present study. Blood was obtained from the affected probands and family members. Subjects underwent medical tests, including 12-lead electrocardiogram (ECG; Fig. 1) and ultrasonic cardiogram (UCG), and their hospital records were analyzed. A further 200 healthy people were also enrolled to exclude the single nucleotide polymorphism (13).

Whole-exome sequencing

Genomic DNA was extracted using the DNeasy Blood & Tissue kit (Qiagen, Inc., Valencia, CA, USA). The Novogene Bioinformatics Institute (Beijing, China) performed the exome capture, high-throughput sequencing and common filtering. All of the exomes were captured using SureSelect Human All ExonV5 kits (Agilent Technologies, Inc., Santa Clara, CA, USA) and were sequenced using the HiSeq2000 platform (Illumina, Inc., San Diego, CA, USA). Filtering strategies were as described in a previous study (13). The effect of variants were predicted by polyphen2 (http://genetics.bwh.harvard.edu/pph2/index.shtml), SIFT (http://sift.jcvi.org/) and MutationTaster (http://www.mutationtaster.org/).

Co-segregation analysis

Segregation analysis was applied in all family members according to the results of the WES. Primer pairs were designed using DNASTAR version 6.0 (Madison, WI, USA) and the sequences of primers are forward: CTA CAC CAG CTT CGA TTC CTT; reverse: TGA TCC CTT CTC CCT CAG AA.

Results <sec> <title>Clinical features

A Chinese family with a history of arrhythmia and syncope was identified (Fig. 2A). The proband, a 21-year-old college student from the Hunan province of central-southern China, had experienced syncope during strenuous physical exercise 6 months previously. A family history analysis demonstrated that the maternal uncle of the proband had experienced syncope 8 years previously and that the maternal grandmother of the proband had succumbed to an unknown cause during sleep. ECG and UCG analysis demonstrated that the maternal uncle of the proband exhibited sinus bradycardia. The proband and the mother of the proband exhibited ventricular premature beats (Fig. 1). The ECG of the sister of the proband was not obtained.

Genetic analysis

Data filtering excluded shared common variants present in the 1000 Genomes Project (http://www.internationalgenome.org/), dbSNP132 (https://www.ncbi.nlm.nih.gov/projects/SNP/) and ESP databases (http://evs.gs.washington.edu/EVS/). A total of 711 unique single-nucleotide polymorphisms were identified in the proband. Through screening of the variants of arrhythmia-associated genes, a novel missense mutation (p.R367G) of SCN5A was identified and Sanger DNA sequencing demonstrated that this mutation was co-segregated with affected members (Fig. 2B). The newly identified c.1099C>G mutation in SCN5A was not observed in the 200 control individuals. The mutation was not present in the dbSNP and Exome Variant Server databases (evs.gs.washington.edu/EVS). Alignment of SCN5A amino acid sequences from human, Pan troglodytes, Mus musculus, Gallus gallus and other genomes (Fig. 2C) demonstrated that the affected amino acid was evolutionarily conserved. A total of three programs used for analyzing protein functions, polyphen2, SIFT and MutationTaster, predicted that the p.R367G variants of SCN5A may be damaging, deleterious and disease-causing, respectively.

Discussion

In the present study, a novel heterozygous mutation, c.1099C>G, was identified in the SCN5A gene, causing arrhythmia and syncope. Cosegregation analysis demonstrated the involvement of the mutation in the pathogenesis of the arrhythmic phenotype exhibited by the family in the present study. The diagnosis of arrhythmia in the proband was based on the ECG and UCG, which demonstrated a ventricular premature beat, as was additionally observed in the mother of the proband. The maternal uncle of the proband exhibited sinus bradycardia with a history of syncope and arrhythmia. In order to identify the disease-causing gene in the proband, WES analysis was used, in combination with arrhythmia-associated gene filtering, to explore the possible causative genes. A novel missense mutation (c.1099C>G) in exon 9 of the SCN5A gene was identified, which resulted in an amino acid change from arginine to glycine at position 367 in the DI-S6 subunit of the NaV1.5 channel (14,15). Bioinformatics analysis predicted that this mutation was disease-causing, and the site (R367) of SCN5A is evolutionarily conserved. The mutation was further investigated using co-segregation analysis, which demonstrated that all affected individuals in the present study carried the mutation, while the wild-type allele individuals did not. The results of the present study suggested that the SCN5A mutation led to the dysfunction of the NaV1.5 channel, which has been demonstrated to cause syncope during strenuous physical exercise (16).

The NaV1.5 channel α subunit consists of four homologous domains, and each domain contains six α-helical transmembrane repeats (14). In the present study, the substituted amino acid p.R367G was located at the six α-helical transmembrane segment of domain I-S6. The substitution of basic amino acid Arg by neutral amino acid Gly in position 367 of the SCN5A may affect transmembrane sodium transport (17). Numerous mutations in this site and region have been reported. For example, p.R367L and p.R367C were demonstrated to be associated with Brugada syndrome (18,19). The mutation p.R367H was previously demonstrated to be involved in sudden unexplained nocturnal death syndrome (20). In addition, p.M369L, p.T370M and p.W374G were observed in Brugada syndrome and other arrhythmogenic disorders (18,19,21). These previous results demonstrated that the site (R367) exerts an important function in the I-S6 domain of the NaV1.5 channel α subunit, and that this domain serves a role in the regulation of the gating properties of the channel.

Multiple lines of evidence support the notion that the mutation identified in the present study is associated with arrhythmia and syncope: i) This base was not identified in 200 control subjects, suggesting that it is not a common polymorphism; ii) no other meaningful mutations were identified in SCN5A or other genes; iii) this base change was not identified in other siblings who were not diagnosed with arrhythmia and syncope; iv) the mutation is evolutionally conserved in multiple animal species, suggesting that any substitution at this codon is not tolerated; and v) the same site mutations (p.R367H, p.R367L and p.R367C) have been previously identified to cause arrhythmia and SCD (18–20).

In conclusion, using whole-exome sequencing in combination with an arrhythmia-associated gene filtering method, a novel missense mutation (c.1099G>C/p.R367G) in SCN5A was identified to be a possible cause of a case of familial arrhythmia. The present study increases the understanding of SCN5A mutations, and contributes to potential genetic diagnosis and counseling of families with arrhythmia.

Acknowledgements

The authors of the present study would like to acknowledge the State Key Laboratory of Medical Genetics of China (Changsha, China), for technical assistance. The present study was supported by the Fundamental Research Funds for Central Universities of Central South University (grant no. 2016zzts163).

References 1

Smits

Veldkamp

Wilde

Mechanisms of inherited cardiac conduction disease

Europace71221372005

10.1016/j.eupc.2004.11.004

15763526

Kawaguchi

Hayashi

Miyamoto

Yoshino

Taniguchi

Naiki

Sugimoto

Ito

Xue

Murakami

Horie

Prognostic implications of progressive cardiac conduction disease

Circ J7760672013

10.1253/circj.CJ-12-0849

23018635

den Hoed

Eijgelsheim

Esko

Brundel

Peal

Evans

Nolte

Segrè

Holm

Handsaker

Identification of heart rate-associated loci and their effects on cardiac conduction and rhythm disorders

Nat Genet456216312013

10.1038/ng.2610

23583979

3696959

Beltran-Alvarez

Tarradas

Chiva

Pérez-Serra

Batlle

Pérez-Villa

Schulte

Sabidó

Brugada

Pagans

Identification of N-terminal protein acetylation and arginine methylation of the voltage-gated sodium channel in end-stage heart failure human heart

J Mol Cell Cardiol761261292014

10.1016/j.yjmcc.2014.08.014

25172307

Xiong

Cao

Marian

Hong

A rare loss-of-function SCN5A variant is associated with lidocaine-induced ventricular fibrillation

Pharmacogenomics J143723752014

10.1038/tpj.2013.50

24445991

4105333

Wang

Zhang

Liu

Fang

Yang

Mutations of the SCN4B-encoded sodium channel β4 subunit in familial atrial fibrillation

Int J Mol Med321441502013

23604097

Riuró

Campuzano

Arbelo

Iglesias

Batlle

Pérez-Villa

Brugada

Pérez

Scornik

Brugada

A missense mutation in the sodium channel β1b subunit reveals SCN1B as a susceptibility gene underlying long QT syndrome

Heart Rhythm11120212092014

10.1016/j.hrthm.2014.03.044

24662403

Bezzina

Barc

Mizusawa

Remme

Gourraud

Simonet

Verkerk

Schwartz

Crotti

Dagradi

Common variants at SCN5A-SCN10A and HEY2 are associated with Brugada syndrome, a rare disease with high risk of sudden cardiac death

Nat Genet45104410492013

10.1038/ng.2712

23872634

3869788

Blich

Efrati

Marai

Suleiman

Gepstein

Boulous

Novel Clinical Manifestation of the Known SCN5A D1790G Mutation

Cardiology1322282322015

10.1159/000437089

26304620

Ilkhanoff

Arking

Lemaitre

Alonso

Chen

Durda

Hesselson

Kerr

Magnani

Marcus

A common SCN5A variant is associated with PR interval and atrial fibrillation among African Americans

J Cardiovasc Electrophysiol25115011572014

10.1111/jce.12483

25065297

4454499

Mann

Castro

Ohanian

Guo

Zodgekar

Sheu

Stockhammer

Thompson

Playford

Subbiah

R222Q SCN5A mutation is associated with reversible ventricular ectopy and dilated cardiomyopathy

J Am Coll Cardiol60156615732012

10.1016/j.jacc.2012.05.050

22999724

Hothi

Ara

Timperley

p.Y1449C SCN5A mutation associated with overlap disorder comprising conduction disease, Brugada syndrome, and atrial flutter

J Cardiovasc Electrophysiol2693972015

10.1111/jce.12470

24903439

Liu

Chen

Shen

Exome Sequencing Identifies a Novel DES Mutation (R227C) in a Chinese Dilated Cardiomyopathy Family

Cardiology13778822017

10.1159/000455181

28171858

Adsit

Vaidyanathan

Galler

Kyle

Makielski

Channelopathies from mutations in the cardiac sodium channel protein complex

J Mol Cell Cardiol6134432013

10.1016/j.yjmcc.2013.03.017

23557754

3720718

Amin

Asghari-Roodsari

Tan

Cardiac sodium channelopathies

Pflugers Arch4602232372010

10.1007/s00424-009-0761-0

20091048

Shy

Gillet

Abriel

Cardiac sodium channel NaV1.5 distribution in myocytes via interacting proteins: The multiple pool model

Biochim Biophys Acta18338868942013

10.1016/j.bbamcr.2012.10.026

23123192

van Hoorn

Campian

Spijkerboer

Blom

Planken

van Rossum

de Bakker

Wilde

Groenink

Tan

SCN5A mutations in Brugada syndrome are associated with increased cardiac dimensions and reduced contractility

PLoS One7e420372012

10.1371/journal.pone.0042037

22876298

3410911

Smits

Eckardt

Probst

Bezzina

Schott

Remme

Haverkamp

Breithardt

Escande

Schulze-Bahr

Genotype-phenotype relationship in Brugada syndrome: Electrocardiographic features differentiate SCN5A-related patients from non-SCN5A-related patients

J Am Coll Cardiol403503562002

10.1016/S0735-1097(02)01962-9

12106943

Kapplinger

Tester

Alders

Benito

Berthet

Brugada

Fressart

Guerchicoff

Harris-Kerr

An international compendium of mutations in the SCN5A-encoded cardiac sodium channel in patients referred for Brugada syndrome genetic testing

Heart Rhythm733462010

10.1016/j.hrthm.2009.09.069

20129283

Vatta

Dumaine

Varghese

Richard

Shimizu

Aihara

Nademanee

Brugada

Veerakul

Genetic and biophysical basis of sudden unexplained nocturnal death syndrome (SUNDS), a disease allelic to Brugada syndrome

Hum Mol Genet113373452002

10.1093/hmg/11.3.337

11823453

Hofman-Bang

Behr

Hedley

Tfelt-Hansen

Kanters

Haunsøe

McKenna

Christiansen

High-efficiency multiplex capillary electrophoresis single strand conformation polymorphism (multi-CE-SSCP) mutation screening of SCN5A: A rapid genetic approach to cardiac arrhythmia

Clin Genet695045112006

10.1111/j.1399-0004.2006.00621.x

16712702

Figure 1.

Clinical features of family members with cardiac conduction diseases. Electrocardiograms of the family members III-1, II-6 and II-4. Family members are identified by generations and numbers.

Figure 2.

SCNA5 sequencing and alignment. (A) Pedigree of the family affected by arrhythmia. Family members are identified by generations and numbers. Squares, male family members; circles, female members; closed symbols, affected members; open symbols, unaffected members; arrow, proband. (B) Sequencing results of the SCN5A mutation. The sequence chromatogram indicates a C to G transition of nucleotide 1099. (C) Alignment of multiple SCN5A protein sequences across multiple species. The R367 affected amino acid is located in a highly-conserved amino acid region in different mammals. Red indicates the R367 site. P. troglodytes, Pan troglodytes; M. mulatta, Macaca mulatta; F. catus, Felis catus; M. musculus, Mus musculus; G. gallus, Gallus gallus.