Genome-wide Single Cell Haplotyping as a Generic Method for Preimplantation Genetic Diagnosis
1 other identifier
observational
60
1 country
1
Brief Summary
The investigators previously developed approaches to SNP-, CNV- and haplo-type single human cells (Vanneste et al. 2009, Nature Medicine). These methods open the possibility to be developed into a novel generic diagnostic technique which broadens the spectrum of disease-alleles that can be selected against during preimplantation genetic diagnosis (PGD) and which enables to help those couples that cannot be supported by PGD yet. PGD is the genetic analysis of a single blastomere from an in vitro fertilized (IVF) embryo and it is offered to couples to avoid the transmission of heritable genetic disorders to their offspring. PGD analyses are performed for (1) autosomal dominant or recessive monogenic diseases, (2) X-linked disorders and (3) chromosomal aberrations that may result in aneuploid conceptions. This novel method is likely to outperform and hence, replace current techniques for preimplantation genetic diagnosis. In this project the investigators will bring the technology from a proof-of-principle to the clinical application. To this end the investigators will make computational improvements for accurate single blastomere SNP-, CNV- and haplo-typing and perform a large validation study. For the validation studythe investigators will analyse the genomes of the blastomeres derived from 60 spare embryos of different origin: (1) Embryos diagnosed as genetically abnormal using current PCR- and FISH-protocols. (2) Embryos diagnosed as normal for the investigated region using current PCR- and FISH-protocols, but not of sufficient quality to be transferred or frozen. (3) Embryos of the sex that is selected against following PGD based sex-selection, or embryos of the sex that is selected for but of insufficient quality to be transferred or frozen. (4) Embryos that were not biopsied in a PGD cycle since they suffer a slight growth delay. This validation study will allow us to evaluate (1) the clinical validity (false positive and negative rate) and (2) clinical applicability (in terms of ease of use, success rate, etc.). In addition, it will bring us essential further fundamental insights in the origins and mechanisms of chromosomal instability operating during early embryogenesis and its consequences for clinical applications of PGD. Finally, following the validation study, this project will clinically implement the technique to treat 10 families.
Trial Health
Trial Health Score
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participants targeted
Target at P25-P50 for all trials
Started Oct 2010
Typical duration for all trials
1 active site
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Trial Relationships
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Study Timeline
Key milestones and dates
Study Start
First participant enrolled
October 1, 2010
CompletedFirst Submitted
Initial submission to the registry
April 13, 2011
CompletedFirst Posted
Study publicly available on registry
April 15, 2011
CompletedPrimary Completion
Last participant's last visit for primary outcome
September 1, 2013
CompletedStudy Completion
Last participant's last visit for all outcomes
September 1, 2013
CompletedApril 15, 2011
April 1, 2010
2.9 years
April 13, 2011
April 14, 2011
Conditions
Keywords
Study Arms (2)
PGD-FISH
Following couples opting for preimplantation genetic diagnosis on the basis of FISH: * couples suffering a complex chromosomal rearrangement (CCR) * couples with X-linked recessive disorders * couples that carry a balanced chromosomal rearrangement
PGD-PCR
Following couples opting for preimplantation genetic diagnosis on the basis of PCR: -couples at risk for the transmission of monogenic diseases
Interventions
We aim to collect single blastomeres from spare IVF embryos of 30 couples to optimize and test methods for single cell haplotyping. We aim to collect 20 and 10 couples coming to the fertility centre for FISH- or PCR-based PGD respectively. In both groups, at least 5 different indications for PGD will be collected. Per couple, we will perform 10 SNP-arrays: 2 for the couple donating the embryo, 4 for family members (often parents of the couple) and 4 for blastomeres since we aim to pick 2 cells from 2 embryos per couple. For five couples, 2 blastomeres of all available embryos will be aspirated to validate and optimize the phasing methods. Finally, for some embryos, all blastomeres will be picked to be able to prove the reproducibility of single cell haplotyping.
Eligibility Criteria
We aim to collect spare embryos of 30 couples that opt for preimplantation genetic diagnosis (see Eligibility Criteria).
You may qualify if:
- Blastomeres biopsied from spare embryos ((A) Embryos diagnosed as genetically abnormal using current PCR- and FISH-protocols; (B) Embryos diagnosed as normal for the investigated region using current PCR- and FISH-protocols, but not of sufficient quality to be transferred or frozen; (C) Embryos of the sex that is selected against following PGD based sex-selection, or embryos of the sex that is selected for but of insufficient quality to be transferred or frozen; (D) Embryos that were not biopsied in a PGD cycle since they suffer a slight growth delay.) derived from following patient groups:
- The first patient group involve couples suffering a complex chromosomal rearrangement (CCR), which is defined as a structural chromosomal rearrangement with at least three breakpoints and an exchange of genetic material between two or more chromosomes.
- The second patient group involve couples with X-linked recessive disorders.
- The third patient group consists of couples that carry a balanced chromosomal rearrangement - a translocation, insertion or inversion - that may result in recurrent miscarriage or aneuploid, severely handicapped offspring.
- A fourth patient group are couples at risk for the transmission of monogenic diseases.
Contact the study team to confirm eligibility.
Sponsors & Collaborators
- Universitaire Ziekenhuizen KU Leuvenlead
- KU Leuvencollaborator
- Universitair Ziekenhuis Brusselcollaborator
- Vrije Universiteit Brusselcollaborator
Study Sites (1)
Universitaire Ziekenhuizen Leuven
Leuven, Vlaams Brabant, 3000, Belgium
Related Publications (2)
Vanneste E, Voet T, Le Caignec C, Ampe M, Konings P, Melotte C, Debrock S, Amyere M, Vikkula M, Schuit F, Fryns JP, Verbeke G, D'Hooghe T, Moreau Y, Vermeesch JR. Chromosome instability is common in human cleavage-stage embryos. Nat Med. 2009 May;15(5):577-83. doi: 10.1038/nm.1924. Epub 2009 Apr 26.
PMID: 19396175BACKGROUNDVanneste E, Voet T, Melotte C, Debrock S, Sermon K, Staessen C, Liebaers I, Fryns JP, D'Hooghe T, Vermeesch JR. What next for preimplantation genetic screening? High mitotic chromosome instability rate provides the biological basis for the low success rate. Hum Reprod. 2009 Nov;24(11):2679-82. doi: 10.1093/humrep/dep266. Epub 2009 Jul 24.
PMID: 19633308BACKGROUND
Biospecimen
Genomic DNA, single blastomere DNA
Study Officials
- PRINCIPAL INVESTIGATOR
Joris R Vermeesch, Professor
Universitaire Ziekenhuizen KU Leuven
- PRINCIPAL INVESTIGATOR
Thierry Voet, Professor
KU Leuven
- PRINCIPAL INVESTIGATOR
Thomas D'Hooghe, Professor
Universitaire Ziekenhuizen KU Leuven
- PRINCIPAL INVESTIGATOR
Yves Moreau, Professor
KU Leuven
- PRINCIPAL INVESTIGATOR
Karen Sermon, Professor
Vrije Universiteit Brussel
- PRINCIPAL INVESTIGATOR
De Rycke Martine, Professor
Universitair Ziekenhuis Brussel
Central Study Contacts
Study Design
- Study Type
- observational
- Observational Model
- CASE ONLY
- Time Perspective
- PROSPECTIVE
- Sponsor Type
- OTHER
Study Record Dates
First Submitted
April 13, 2011
First Posted
April 15, 2011
Study Start
October 1, 2010
Primary Completion
September 1, 2013
Study Completion
September 1, 2013
Last Updated
April 15, 2011
Record last verified: 2010-04