Clinical characteristics.

The first identified CACNA1C-related disorder, referred to as Timothy syndrome, consists of the combination of prolonged QT interval, autism, and cardiovascular malformation with syndactyly of the fingers and toes. Infrequent findings also include developmental and speech delay, seizures, and recurrent infections. With increased availability of molecular genetic testing, a wider spectrum of pathogenic variants and clinical findings associated with CACNA1C-related disorders has been recognized. Because CACNA1C is associated with calcium channel function, all individuals with a pathogenic variant in this gene are at risk for cardiac arrhythmia of a specific type. The clinical manifestations of a CACNA1C-related disorder include three phenotypes:

• Timothy syndrome with or without syndactyly
• QT prolongation (QTc >480 ms) and arrhythmias in the absence of other syndromic features
• Short QT syndrome (QTc <350 ms) or Brugada syndrome with short QT interval

These three phenotypes can be separated into two broad categories on the basis of the functional consequences of the pathogenic variants in CACNA1C:

• QT prolongation with or without a Timothy syndrome-associated phenotype associated with pathogenic variants inducing a gain of function at the cellular level (i.e., increased calcium current)
• Short QT interval with or without Brugada syndrome EKG pattern associated with pathogenic variants causing loss of function (i.e., reduced calcium current)

Diagnosis/testing.

The diagnosis of a CACNA1C-related disorder is established in a proband with suggestive findings and a heterozygous pathogenic variant in CACNA1C identified by molecular genetic testing.

Management.

Treatment of manifestations: Treatment includes use of beta blockers and/or other antiarrhythmic drugs to maintain QT interval stability to prevent ventricular tachyarrhythmia. In some instances, pacemakers can be placed during the first days of life to control 2:1 atrioventricular block and resultant bradycardia, but an implantable cardioverter defibrillator to prevent sudden cardiac death should be considered in all affected persons. Standard care is recommended for cardiovascular malformations and extracardiac malformations such as syndactyly and hypoglycemia.

Prevention of primary manifestations: Arrhythmias must be prevented with the standard therapy. Because anesthesia is a known trigger for cardiac arrhythmia, close cardiac monitoring is warranted during surgery. Fever can be a trigger for arrhythmias in individuals with CACNA1C-related Brugada syndrome and requires aggressive treatment with standard antipyretic drugs.

Surveillance: Cardiac and neurologic evaluations every six to 12 months.

Agents/circumstances to avoid: Drugs reported to prolong QT interval; drugs and dietary practices that could lead to hypoglycemia.

Evaluation of relatives at risk: It is appropriate to clarify the genetic status of the older and younger at-risk relatives of a proband in order to identify as early as possible those who would benefit from a complete cardiac evaluation and institution of measures to prevent cardiac arrhythmias.

Genetic counseling.

CACNA1C-related disorders are autosomal dominant disorders. Many individuals diagnosed with a CACNA1C-related disorder – particularly those individuals with Timothy syndrome – represent simplex cases (i.e., a single affected family member) and have the disorder as the result of a pathogenic variant that occurred de novo in the proband or in a mosaic parent. If a parent of the proband is affected and/or is known to be heterozygous for the pathogenic variant identified in the proband, the risk to the sibs of inheriting the pathogenic variant is 50%. If the proband has a known CACNA1C pathogenic variant that cannot be detected in the leukocyte DNA of either parent, the recurrence risk to sibs is greater than that of the general population because of the possibility of parental germline mosaicism. Once the CACNA1C pathogenic variant has been identified in an affected family member, prenatal testing and preimplantation genetic testing for a pregnancy at increased risk for a CACNA1C-related disorder are possible.

Suggestive Findings

A CACNA1C-related disorder should be suspected in individuals with any of the following three major clinical findings and family history.

Clinical findings

• A prolonged QT interval on electrocardiogram (EKG) (rate-corrected QT [QTc] interval >480 ms) with or without the following findings:
  • Cardiovascular malformations such as patent ductus arteriosus, patent foramen ovale, ventricular septal defect, tetralogy of Fallot, or hypertrophic cardiomyopathy
  • Unilateral or bilateral cutaneous syndactyly variably involving fingers two (index), three (middle), four (ring), and five (little) and bilateral cutaneous syndactyly of toes two and three
  • Neurologic findings including autism, seizures, intellectual disability, hypotonia
  • Facial anomalies including depressed nasal bridge, low-set ears, thin vermilion of the upper lip, round face, and abnormal tooth development
• ST segment elevation in right precordial leads (V1-V2) diagnostic for Brugada syndrome (type 1 EKG) associated with a short QT interval
• Short QT interval (QTc <350 ms) and risk of sudden death

Family history is consistent with autosomal dominant inheritance (e.g., affected males and females in multiple generations). There may be a history of syncope, aborted cardiac arrest, or sudden death in a child or young adult relative in whom a diagnosis was not recognized. Absence of a known family history does not preclude the diagnosis.

Establishing the Diagnosis

The diagnosis of a CACNA1C-related disorder is established in a proband with suggestive findings and a heterozygous pathogenic (or likely pathogenic) variant in CACNA1C identified by molecular genetic testing (see Table 1).

Note: (1) Per ACMG/AMP variant interpretation guidelines, the terms "pathogenic variants" and "likely pathogenic variants" are synonymous in a clinical setting, meaning that both are considered diagnostic and both can be used for clinical decision making [Richards et al 2015]. Reference to "pathogenic variants" in this section is understood to include any likely pathogenic variants. (2) Identification of a heterozygous CACNA1C variant of uncertain significance does not establish or rule out the diagnosis.

Molecular genetic testing approaches can include a combination of gene-targeted testing (single-gene testing and multigene panel) and comprehensive genomic testing (exome sequencing, genome sequencing) depending on the phenotype.

Gene-targeted testing requires that the clinician determine which gene(s) are likely involved, whereas genomic testing does not. Individuals with the distinctive findings described in Suggestive Findings are likely to be diagnosed using gene-targeted testing (see Option 1), whereas those with a phenotype indistinguishable from many other inherited disorders with cardiac or neurologic findings are more likely to be diagnosed using genomic testing (see Option 2).

Clinical Description

The first CACNA1C-related disorder was referred to as Timothy syndrome [Splawski et al 2004], a condition with very high mortality with only few individuals who reached reproductive age. Timothy syndrome consisted of the combination of prolonged QT interval, autism, and congenital heart defect with syndactyly of the fingers and toes; all these individuals had the same pathogenic variant, while a similar phenotype but without syndactyly was subsequently identified in association with similar but distinct pathogenic variants (see Genotype-Phenotype Correlations).

With increased availability of molecular genetic testing, a wider spectrum of pathogenic variants and clinical findings associated with CACNA1C-related disorders has been recognized. Because CACNA1C is associated with calcium channel function, all individuals with a pathogenic variant in this gene are at risk for cardiac arrhythmia of a specific type.

The clinical manifestations of a CACNA1C-related disorder include three phenotypes:

• Timothy syndrome with or without syndactyly [Splawski et al 2004, Splawski et al 2005];
• QT prolongation (QTc >480 ms) and arrhythmias in the absence of other syndromic features [Wemhöner et al 2015]; and
• Short QT syndrome (QTc <350 ms) [Raschwitz et al 2020] or Brugada syndrome with short QT interval [Burashnikov et al 2010].

These three phenotypes can be separated into two broad categories on the basis of the functional consequences of the pathogenic variants:

• QT prolongation with or without a Timothy syndrome-associated phenotype associated with pathogenic variants inducing a gain of function at the cellular level (i.e., increased calcium current); and
• Short QT interval with or without Brugada syndrome EKG pattern associated with pathogenic variants causing loss of function (i.e., reduced calcium current).

The clinical phenotype associated with large deletions/duplications is less defined, as few individuals with this phenotype have been reported (see Table 1).

Age at diagnosis may vary depending on the associated phenotype.

• In general, the diagnosis of Timothy syndrome is made within the first few days of life based on the markedly prolonged rate-corrected QT (QTc) interval in an infant with bradycardia and 2:1 atrioventricular (AV) block [Reichenbach et al 1992, Marks et al 1995a, Lo-A-Njoe et al 2005]. Rarely, diagnosis may be delayed until age two to four years [Marks et al 1995b, Splawski et al 2005].
• Individuals with QT prolongation only (no other Timothy syndrome features) or individuals with Brugada syndrome or short QT syndrome are generally associated with less severe EKG abnormalities and lower incidence of events. Therefore, the diagnosis may be established later in life, sometimes as an incidental finding during routine visits or sport pre-participation screening.
• Occasionally, the diagnosis of a CACNA1C-related disorder is suspected prenatally because of fetal distress secondary to cardiac findings of bradycardia with a heart rate that is usually 70-80 (normal fetal heart rate is 120-150) or 2:1 AV block. Biventricular hypertrophy and biventricular dysfunction have been observed on a fetal echocardiogram [Splawski et al 2005].

Genotype-Phenotype Correlations

The classic Timothy syndrome phenotype results from the p.Gly406Arg pathogenic variant in exon 8A, an exon contained in a specific splice variant of CACNA1C (see Molecular Genetics).

Timothy syndrome phenotype in the absence of syndactyly (also referred to in the literature as atypical Timothy syndrome) has been associated with the pathogenic variants p.Gly406Arg and p.Gly402Ser occurring in exon 8 of a CACNA1C alternate splice form.

All reported CACNA1C pathogenic variants associated with QT prolongation (with or without syndromic features) occur in the intracellular portion of the protein.

No specific genotype-phenotype correlation has been found for CACNA1C variants associated with Brugada syndrome or short QT syndrome.

Penetrance

The penetrance of pathogenic variants associated with typical Timothy syndrome is 100%. [Splawski et al 2005]. Nonsyndromic forms have lower penetrance that can be estimated in the range of 60%-80% on the basis of published literature [Fukuyama et al 2014, Wemhöner et al 2015].

Penetrance is not known to differ between males and females.

Nomenclature

The term Timothy syndrome (also referred to as Timothy syndrome type 1) was named for Katherine Timothy, who followed children with that phenotype for more than 14 years, identifying the non-cardiac manifestations and collecting samples that led to the discovery of the gene in which pathogenic variants are causative.

Atypical Timothy syndrome (formerly referred to as Timothy syndrome type 2) was the term used to describe individuals who had QT interval prolongation without syndactyly.

LQT8. The term LQT8 is used in medical literature to refer to both Timothy syndrome and nonsyndromic CACNA1C-related long QT syndrome.

BRGDA3 refers to CACNA1C-related Brugada syndrome.

SQT6 refers to CACNA1C-related short QT syndrome [Templin et al 2011].

Prevalence

Timothy syndrome is a very rare condition probably because of its very high mortality. Fewer than 100 cases have been described worldwide.

The prevalence of nonsyndromic CACNA1C-related disorders (long QT syndrome, Brugada syndrome, and short QT syndrome) is not known. Indirect evidence based on genomic sequencing data and available in vitro expression data suggest a prevalence of around 1:10,000 or lower [Author, personal observation].

Evaluations Following Initial Diagnosis

To establish the extent of disease and needs in an individual diagnosed with a CACNA1C-related disorder, the evaluations summarized in Table 4 (if not performed as part of the evaluation that led to the diagnosis) are recommended.

Treatment of Manifestations

Standard care is recommended for cardiovascular malformations, surgical release of syndactyly, and hypoglycemia.

Note: All medical procedures requiring anesthesia should be performed with caution (see Prevention of Primary Manifestations).

Prevention of Primary Manifestations

Arrhythmias must be prevented with the standard therapy described in Treatment of Manifestations.

Anesthesia is a known trigger for cardiac arrhythmia in individuals with a CACNA1C-related disorder. Therefore, any surgical intervention must be performed under close cardiac monitoring. Because clinical experience with CACNA1C-related disorders is scarce, all compounds used for general anesthesia should be regarded as potentially dangerous.

Fever can be a trigger for arrhythmias in individuals with CACNA1C-related Brugada syndrome (as in Brugada syndrome in general) and requires aggressive treatment with standard antipyretic drugs.

Surveillance

Agents/Circumstances to Avoid

The following should be avoided:

• All drugs reported to prolong QT interval (See CredibleMeds^®.)
• Drugs and dietary practices that could lead to hypoglycemia

Evaluation of Relatives at Risk

It is appropriate to clarify the genetic status of the older and younger at-risk relatives of a proband in order to identify as early as possible those who would benefit from a complete cardiac evaluation and institution of measures to prevent cardiac arrhythmias.

See Genetic Counseling for issues related to testing of at-risk relatives for genetic counseling purposes.

Therapies Under Investigation

Search ClinicalTrials.gov in the US and EU Clinical Trials Register in Europe for access to information on clinical studies for a wide range of diseases and conditions. Note: There may not be clinical trials for this disorder.

Mode of Inheritance

CACNA1C-related disorders are autosomal dominant disorders.

Risk to Family Members

Parents of a proband

• Many individuals diagnosed with a CACNA1C-related disorder – particularly those individuals with Timothy syndrome – represent simplex cases (i.e., a single affected family member) and have the disorder as the result of a de novo pathogenic variant.
• Some individuals diagnosed with a CACNA1C-related disorder have an affected parent.
• Molecular genetic testing is recommended for the parents of the proband to confirm their genetic status and to allow reliable recurrence risk counseling.
• If the pathogenic variant identified in the proband is not identified in either parent, the following possibilities should be considered:
  • The proband has a de novo pathogenic variant. Note: A pathogenic variant is reported as "de novo" if: (1) the pathogenic variant found in the proband is not detected in parental DNA; and (2) parental identity testing has confirmed biological maternity and paternity. If parental identity testing is not performed, the variant is reported as "assumed de novo" [Richards et al 2015].
  • The proband inherited a pathogenic variant from a parent with germline (or somatic and germline) mosaicism. Parental mosaicism for a CACNA1C pathogenic variant has been reported [Splawski et al 2004]. Note: Testing of parental leukocyte DNA may not detect all instances of somatic mosaicism and will not detect a pathogenic variant that is present in the germ cells only.
• The family history of some individuals diagnosed with a CACNA1C-related disorder may appear to be negative because of failure to recognize the disorder in family members, reduced penetrance, early death of the parent before the onset of symptoms, or late onset of the disease in the affected parent. Therefore, an apparently negative family history cannot be confirmed unless molecular genetic testing has demonstrated that neither parent is heterozygous for the pathogenic variant identified in the proband.

Sibs of a proband. The risk to the sibs of the proband depends on the genetic status of the proband's parents:

• If a parent of the proband is affected and/or is known to have the pathogenic variant identified in the proband, the risk to the sibs of inheriting the pathogenic variant is 50%.
• Penetrance in sibs who inherit a familial CACNA1C pathogenic variant ranges from 100% (for sibs of a proband with Timothy syndrome) to approximately 60%-80% (for sibs of a proband with a nonsyndromic CACNA1C-related cardiac arrhythmia).
• If the proband has a known CACNA1C pathogenic variant that cannot be detected in the leukocyte DNA of either parent, the recurrence risk to sibs is greater than that of the general population because of the possibility of parental germline mosaicism. Parental mosaicism has been reported [Splawski et al 2004].
• If the parents are clinically unaffected but have not been tested for the pathogenic variant, recurrence risk in sibs is estimated to be 50% because a heterozygous parent may be clinically unaffected due to reduced penetrance of long QT syndrome-related EKG changes and symptoms.

Offspring of a proband. Each child of an individual with a CACNA1C-related disorder has a 50% chance of inheriting the CACNA1C pathogenic variant.

Other family members. The risk to other family members depends on the status of the proband's parents: if a parent has the CACNA1C pathogenic variant, the parent's family members may be at risk.

Specific risk issues. With the reduced penetrance of symptoms in individuals with a CACNA1-related disorder, careful EKG evaluation including exercise EKG is often necessary to identify affected family members accurately. The absence of a family history of sudden death is common and does not negate the diagnosis or preclude the possibility of sudden death in relatives.

Related Genetic Counseling Issues

See Management, Evaluation of Relatives at Risk for information on evaluating at-risk relatives for the purpose of early diagnosis and treatment.

Family planning

• The optimal time for determination of genetic risk and discussion of the availability of prenatal/preimplantation genetic testing is before pregnancy.
• It is appropriate to offer genetic counseling (including discussion of potential risks to offspring and reproductive options) to young adults who are affected or at risk.

Prenatal Testing and Preimplantation Genetic Testing

Molecular genetic testing. Once the CACNA1C pathogenic variant has been identified in an affected family member, prenatal and preimplantation genetic testing for a pregnancy at increased risk for a CACNA1C-related disorder are possible.

Fetal echocardiography. Monitoring of cardiac rate and function during pregnancy is appropriate.

Differences in perspective may exist among medical professionals and within families regarding the use of prenatal testing. While most centers would consider use of prenatal testing to be a personal decision, discussion of these issues may be helpful.

Molecular Pathogenesis

Excitable cells contain voltage-dependent calcium channels. These channels (also called CaV1.2) are involved in the control of the duration of the electrical activation (action potential duration), which is the counterpart of QT interval in the myocardium. Furthermore, in cardiac cells the calcium entry triggers the release of more calcium from the sarcoplasmic reticulum, leadin to the contraction of muscle fibers. The role of calcium current in the CNS is less well defined.

Most gain-of-function pathogenic variants impair Ca_V1.2 channel inactivation, leading to maintained depolarizing Ca²⁺ [Napolitano & Antzelevitch 2011]. Other pathogenic variants increase the current density [Napolitano & Antzelevitch 2011]. There is relatively little outward current during the plateau phase due to high membrane impedance, so even modest changes in inward calcium current lead to significant QT interval prolongation. This prolongation in turn leads to increased risk of spontaneous, abnormal secondary depolarizations (so-called after-depolarizations), arrhythmia, and sudden death.

Loss-of-function pathogenic variants have an opposite mechanism, with reduced current density [Napolitano & Antzelevitch 2011] that shortens the duration of electrical activation in myocardial cells. Therefore, a shortening of QT interval is the direct consequence of this kind of change. Less clear, due to the lack of experimental models, is the pathogenesis of ST segment elevation leading to a Brugada syndrome phenotype.

CACNA1C has a complex genomic structure that undergoes extensive alternative splicing, producing at least 36 different transcripts. Alternative splicing is regulated by a number of different factors, including a tissue-specific regulation [Napolitano & Antzelevitch 2011]. This may explain the variability of the clinical phenotypes associated with pathogenic variants occurring in alternatively spliced exons or in different regions of the protein.

The gene is also involved in the embryologic development of several organs: CNS [Panagiotakos et al 2019], bones [Ramachandran et al 2013, Atsuta et al 2019], and glucose metabolism [Pan et al 2016].

Mechanism of disease causation. CACNA1C-related disorders can occur via a gain-of-function mechanism and, in this case, clinically manifest with QT prolongation with or without Timothy syndrome phenotypes.

Loss-of-function pathogenic variants cause Brugada syndrome and short QT syndrome.

CACNA1C-specific laboratory technical considerations. Due to the possibility of alternative splicing, sequencing of the entire genomic region of CACNA1C is required for a thorough molecular analysis.

Author Notes

Carlo Napolitano is a senior investigator currently in Molecular Cardiology at the IRCCS Maugeri Scientific Institutes and the Department of Molecular Medicine at the University of Pavia. He has more than 400 publications with 20,000 citations in the field of the genetic basis of cardiac arrhythmias, cardiac electrophysiology, and sudden death (orcid.org/0000-0002-7643-4628).

Acknowledgments

We are grateful to all of the individuals with Timothy syndrome and their families for donated time and samples. We would also like to thank the physicians who identified and are providing care for individuals with Timothy syndrome.

Author History

Raffaella Bloise, MD (2006-present)
Carlo Napolitano, MD, PhD (2006-present)
Silvia G Priori, MD, PhD (2006-present)
Igor Splawski, PhD; Harvard Medical School (2006-2021)
Katherine W Timothy, BS (2006-present)

Revision History

• 11 February 2021 (ha) Comprehensive update posted live
• 16 July 2015 (me) Comprehensive update posted live
• 21 April 2011 (me) Comprehensive update posted live
• 20 August 2009 (cd) Revision: prenatal diagnosis available clinically
• 27 January 2009 (cd) Revision: sequence analysis available clinically
• 29 July 2008 (me) Comprehensive update posted live
• 15 February 2006 (me) Review posted live
• 5 July 2005 (is) Original submission

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