Transient Neonatal Diabetes Mellitus; Russell-Silver Syndrome; Silver-Russell Syndrome; Prader-Willi Syndrome; Angelman Syndrome

Uniparental disomy 6 (UPD6): Approximately 40% of 6q-linked transient neonatal diabetes mellitus (TNDM) is associated with paternal UPD6.

Uniparental disomy 7 (UPD7): Approximately 7-10% of individuals with Russell-Silver syndrome have maternal UPD7.

Uniparental disomy 14 (UPD14): Uniparental disomy of chromosome 14 is rare although phenotypes have been described for both maternal and paternal UPD14. Maternal UPD14 is associated with premature birth; growth retardation; short stature; developmental delay; and precocious puberty. Paternal UPD14 is associated with polyhydramnios; omphalocoele; characteristic facial features; a small, bell-shaped chest with short ribs; and developmental delay.

Uniparental disomy 15 (UPD15): Maternal and paternal UPD15 result in different phenotypes: maternal UPD15 gives rise to approximately 25-30% of cases of Prader-Willi syndrome while paternal UPD15 is the cause of 3-5% of cases of Angelman syndrome.

UPD typically arises from the rescue of a trisomic or monosomic zygote resulting in a conception with both copies of a chromosome from a single parent, rather than one copy from each parent. Parents of children with UPD usually have normal karyotypes; however, carrying a structurally abnormal chromosome (such as in the case of certain translocations) may increase the risk of UPD in offspring.

Please see Additional Requirements (below), for information about what samples are required to perform this analysis.

1. Confirmation of diagnosis:
   1. UPD6: infants with transient neonatal diabetes mellitus
   2. UPD7: individuals with features consistent with Russell-Silver syndrome
   3. UPD14: individuals with features suggestive of the clinical phenotype of either maternal or paternal UPD14
   4. UPD15: following positive methylation analysis for either Prader-Willi syndrome or Angelman syndrome, and negative deletion analysis (fluorescent in situ hybridization performed in a Cytogenetics laboratory), UPD testing may be requested to determine if this could be the underlying genetic mechanism for the abnormal methylation pattern. See PWS and AS test algorithms for further details.
2. Prenatal testing (prenatal diagnosis requests are not normally accepted from physicians other than Medical Geneticists):
   1. Pregnancies at increased risk of a clinically-signficant UPD, where cytogenetic analysis has confirmed a normal karyotype. Examples include:
      1. Pregnancies where one of the parents carries a Robertsonian translocation involving chromosome(s) 14 or 15.
      2. Pregnancies where confined placental mosaicism for chromosome 7, 14, or 15 has been identified.
      3. Pregnancies where one of the parents carries a balanced reciprocal translocation AND a certified Cytogeneticist has recommended UPD testing for chromosomes 6, 7, 14, or 15.

This assay assesses the inheritance of polymorphic microsatellite markers located across the appropriate chromosome (6, 7, 14 or 15); at least two microsatellite markers must be informative for interpretation. For assessment of UPD7 and 15, this test is performed using the ABI Linkage mapping set ABI HD5 v.2.5.

Pregnancy-related/Prenatal

If pregnancy management will be altered, 3 weeks; otherwise, routine TAT.

Blood: 4 mL EDTA is optimal (Minimum: 1 mL EDTA)
DNA: 100 μL at 200 ng/μL is optimal (Minimum: 30 μL at 200 ng/μL)

Label each sample with three patient identifiers; preferably patient name, PHN, and date of birth and ship to the address below. Samples should be shipped at room temperature with a completed MGL Requisition to arrive Monday to Friday (not on Canadian statutory holidays).  

Prenatal Specimens
Prenatal testing REQUIRES LABORATORY CONSULTATION PRIOR TO THE PROCEDURE and can only be ordered by a Medical Geneticist. Contact the laboratory at 604-875-2852 and choose the appropriate option for the Molecular Geneticist on service.
Chorionic Villi: 20 mg.
Direct Amniotic fluid: 25 mL collected in two separate tubes of equal volume.
Cultured Amniocytes: Two (2) 100% confluent T-25 flasks.
DNA extracted from prenatal specimens: 100 μL at 200 ng/μL is optimal (Minimum: 30 μL at 200 ng/μL)

Label each sample with three patient identifiers; preferably patient name, PHN, and date of birth. Ship samples by overnight courier with a completed MGL Requisition to arrive Monday to Friday (not on Canadian statutory holidays) as follows:

• Villi – on wet ice or in media at room temperature
• Amniocytes, Amniotic fluid, DNA – at room temperature

Samples from both biological parents as well as the patient/fetus are required to perform these analyses. If only one parent is available, please consult the on-service Molecular Geneticist.

Testing is only available to residents of Canada, except in very specific circumstances where testing is urgent or emergent.  Payment is not required when requests are made for individuals who are insured by Health Insurance BC (administered through the BC Medical Services Plan (MSP)) AND eligible for testing according to the test utilization guidelines / policy. If the individual undergoing testing is not insured by these providers or does not meet utilization guidelines or policy, please complete a billing form; testing will only commence after receipt of billing informationTest prices can be found here.

Molecular genetic testing is limited by the current understanding of the genome and the genetics of a particular disease, as well as by the method of detection used.

Rare single nucleotide variants or polymorphisms could lead to false-negative or false-positive results. If results obtained do not match the clinical findings, consult the on-service Molecular Geneticist.

A previous bone marrow transplant from an allogenic donor will result in molecular data that reflects the donor genotype rather than the recipient (patient) genotype. Consult the on-service Molecular Geneticist for approach to testing in such individuals.

Transfusions performed with packed red blood cells will generally not affect the outcome of molecular genetic testing. However, if there is no clinical urgency, the cautious approach is to wait one week post packed red cell transfusion before collecting a sample for genetic testing. Consult the on-service Molecular Geneticist as needed.

Test results should be interpreted in the context of clinical findings, family history, and other laboratory data. Errors in our interpretation of results may occur if information given is inaccurate or incomplete.