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SickKids

Beckwith-Wiedemann Syndrome

Alternate test name
Wiedemann-Beckwith Syndrome, IMAGe Syndrome
Gene name / Alternate gene name
  • H19
  • KCNQ1OT1
  • CDKN1C
BWS, WT2, H19DMR, KVDMR, IC1, IC2
Protein
Cyclin-dependent kinase inhibitor 1C; H19, imprinted maternally expressed transcript (non-protein coding); KCNQ1 opposite strand/antisense transcript 1 (non-protein coding), Cyclin-dependent kinase inhibitor 1C
Lab area
Genome Diagnostics - Molecular Genetics
Method and equipment
Sequencing; Methylation-Specific-MLPA of imprinting centers 1 and 2; UPD11 studies via STR (short tandem repeat) analysis
Expected turn-around time
Prenatal samples: 2 weeks Pregnancy/STAT: 2-3 weeks Routine: 4-6 weeks
Specimen type

Blood; extracted DNA is not accepted for Methylation and Copy Number Analysis. 

For details about specimen requirements, please refer to: Specimen Type & Requirements (PDF).

Specimen requirements
  • Blood: 5-10 mL in EDTA, 0.5 mL in EDTA (neonate);
  • DNA-minimum 10 ug in 100 uL low TE (pH8.0)- for CDKN1C or UPD11 analysis

DNA extracted at an external lab is not accepted for MLPA testing.

Storage and transportation

Room Temperature

For details about specimen requirements, please refer to: Specimen Type and Requirements

Special requirements

Special Instructions for Genome Diagnostics Samples

If sample shipment >48 hours, ship on ice.

Shipping information
The Hospital for Sick Children
Division of Genome Diagnostics
555 University Avenue, Black Wing, Room 3416
Toronto, ON
Canada
M5G 1X8
Phone: 416-813-7200 ext. 2
Hours: Monday to Friday, 8 a.m. to 4:30 p.m.
Off hours: Please send to Rapid Response Laboratory, 555 University Avenue, Room 3642
Email Molecular Lab: molecular.lab@sickkids.ca
Email Cytogenetics: cytogenetics.requests@sickkids.ca
Background and clinical significance

Beckwith-Wiedemann syndrome (BWS) is a growth disorder characterized by a number of features, including large body size, defects in the closure of the abdominal wall during development, and an enlarged tongue. A variety of other features may also present. Patients with BWS also show a significantly increased incidence of childhood tumours, especially Wilms’ tumor.

In 85 per cent of cases, there is no family history of BWS. However, in approximately 15 per cent of cases, BWS is transmitted from one generation to the next. In these families, BWS is inherited in an autosomal dominant fashion, usually through the mother. There is no way to predict which or how many of the features characteristic of BWS will be present in an individual with the mutation.

There are a number of genetic changes that cause BWS. To date, all of these occur on chromosome 11 at 11p15.

Methylation at KvDMR and H19
Methylation abnormalities at differentially methylated regions (DMR) in the 11p15 region have been shown to cause BWS. KCNQ1OT1 is a maternally imprinted non-coding antisense transcript. The 5’ region of KCNQ1OT1 (KvDMR) is differentially methylated. Normally, the maternally derived chromosome is methylated, whereas the paternally derived chromosome is unmethylated. Loss of maternal methylation at KvDMR is observed in 50- 60 per cent of individuals with BWS. H19 is a paternally imprinted gene encoding a biologically active non-coding transcript that may function as a tumour suppressor. Normally, the paternally derived chromosome is methylated and the maternally derived chromosome is unmethylated. Gain of maternal methylation at H19 is observed in ~5 per cent of BWS cases. For molecular analysis, the methylation status at KvDMR and H19 is measured. Individuals with UPD can be distinguished from individuals with abnormal methylation of either KvDMR or H19 since those with UPD have methylation abnormalities at both KvDMR and H19. If the methylation results are normal at both KvDMR and H19, this result indicates normal biparental contributions in the tissue sample tested (N.B. see Sensitivity of the Test below).

UPD 11
Approximately 10-20 per cent of BWS cases have received two copies of the 11p15 region from their father and none from their mother, which is called paternal uniparental disomy (patUPD). Paternal UPD patients have an imbalance of gene expression in the BWS critical region. Dosage analysis of paternal and maternal genes in the BWS critical region can be used to detect UPD.

CDKN1C
Patients with BWS may also have mutations in the CDKN1C (p57) gene. The CDKN1C gene is a member of the cyclin-dependent kinase inhibitor family, which acts to negatively regulate cell proliferation. Mutations in the CDKN1C gene have been reported in approximately 5-10 per cent of BWS cases with no known family history and in approximately 40 per cent of cases in inherited autosomal dominant families.

See related information sheet: Beckwith-Wiedemann Syndrome

Disease condition

Beckwith-Wiedemann syndrome

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