ESHRE PGD consortium best practice guidelines for amplification-based PGD

Harton, G.; Rycke, Martine De; Fiorentino, Francesco; Moutou, Céline; SenGupta, Sioban; Traeger-Synodinos, Joanne; Harper, Joyce

doi:10.1093/humrep/deq231

Cited by 211 publications

(157 citation statements)

References 33 publications

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“…The robustness of the multiplex BRCA PCR tests are in accordance with the latest edition of the ESHRE PGD consortium guidelines, 16 with a PCR efficiency 490% and ADO rates o10%.…”

Section: Clinical Cyclesmentioning

confidence: 81%

“…All primers were mixed in one multiplex PCR following the ESHRE guidelines. 16 After optimization of the single-cell multiplex PCR, all protocols were validated by testing at least 50 single leucocytes heterozygous for each marker in at least three separate experiments to assess amplification efficiency and ADO rate. Additionally 15-20 PCR blanks were analyzed to determine contamination.…”

Section: Validation Of Pgd Protocolsmentioning

confidence: 99%

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PGD for hereditary breast and ovarian cancer: the route to universal tests for BRCA1 and BRCA2 mutation carriers

et al. 2013

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Preimplantation Genetic Diagnosis (PGD) is a method of testing in vitro embryos as an alternative to prenatal diagnosis with possible termination of pregnancy in case of an affected child. Recently, PGD for hereditary breast and ovarian cancer caused by BRCA1 and BRCA2 mutations has found its way in specialized labs. We describe the route to universal single-cell PGD tests for carriers of BRCA1/2 mutations. Originally, mutation-specific protocols with one or two markers were set up and changed when new couples were not informative. This route of changing protocols was finalized after 2 years with universal tests for both BRCA1 and BRCA2 mutation carriers based on haplotyping of, respectively, 6 (BRCA1) and 8 (BRCA2) microsatellite markers in a multiplex PCR. Using all protocols, 30 couples had a total of 47 PGD cycles performed. Eight cycles were cancelled upon IVF treatment due to hypostimulation. Of the remaining 39 cycles, a total of 261 embryos were biopsied and a genetic diagnosis was obtained in 244 (93%). In 34 of the 39 cycles (84.6%), an embryo transfer was possible and resulted in 8 pregnancies leading to a fetal heart beat per oocyte retrieval of 20.5% and a fetal heart beat per embryonic transfer of 23.5%. The preparation time and costs for set-up and validation of tests are minimized. The informativity of microsatellite markers used in the universal PGD-PCR tests is based on CEPH and deCODE pedigrees, making the tests applicable in 90% of couples coming from these populations.

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“…The robustness of the multiplex BRCA PCR tests are in accordance with the latest edition of the ESHRE PGD consortium guidelines, 16 with a PCR efficiency 490% and ADO rates o10%.…”

Section: Clinical Cyclesmentioning

confidence: 81%

Section: Validation Of Pgd Protocolsmentioning

confidence: 99%

PGD for hereditary breast and ovarian cancer: the route to universal tests for BRCA1 and BRCA2 mutation carriers

et al. 2013

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“…[2][3][4] With respect to monogenic diseases, PGD can theoretically be applied for any genetic disease with a definitive molecular diagnosis and/or defined linkage within a family. The quantity of sample available for the genetic analysis in PGD is minimal, and in most cases comprises no more than a single cell.…”

Section: Introductionmentioning

confidence: 99%

“…All technical aspects of the method should be addressed before the clinical application of any PGD PCR protocol, to ensure a reliable and accurate genotype result. 4 Besides the PCR-related pitfalls, adverse outcomes subsequent to a PGD diagnosis have been attributed to tube switching during the genotype analysis, transfer of the wrong embryo(s), inappropriate protocol design and chromosomal mosaicism in the embryo(s) being analysed. 5 During the two decades that PGD has been applied as a clinical diagnostic service, the PGD community has accumulated considerable experience, which indicates that the potential causes of misdiagnosis can be substantially addressed through careful assay design of optimised fluorescent and multiplexed robust PCR protocols, overall applied with the most stringent laboratory procedures to additionally preclude contamination and tube-switching.…”

Section: Introductionmentioning

confidence: 99%

“…5 During the two decades that PGD has been applied as a clinical diagnostic service, the PGD community has accumulated considerable experience, which indicates that the potential causes of misdiagnosis can be substantially addressed through careful assay design of optimised fluorescent and multiplexed robust PCR protocols, overall applied with the most stringent laboratory procedures to additionally preclude contamination and tube-switching. 4,5 However, the absence of universally standardsed protocols, compounded by the frequent need to set up case-specific protocols, especially for rare monogenic diseases, means that each PGD centre has its own 'in-house' protocols. This may present issues with quality control, standardisation of laboratory protocols and meeting accreditation standards ISO 15189:2007. www.iso.org/iso/home/store/catalogue_ics/ catalogue_detail_ics.htm?csnumber=42641.…”

Section: Introductionmentioning

confidence: 99%

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The experience of 3 years of external quality assessment of preimplantation genetic diagnosis for cystic fibrosis

Deans

Fiorentino²,

Biricik³

et al. 2012

Eur J Hum Genet

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Preimplantation genetic diagnosis (PGD) was first performed over 20 years ago and has become an accepted part of genetic testing and assisted reproduction worldwide. The techniques and protocols necessary to carry out genetic testing at the single-cell level can be difficult to master and have been developed independently by the laboratories worldwide offering preimplantation testing. These factors indicated the need for an external quality assessment (EQA) scheme for monogenic disease PGD. Toward this end, the European Society for Human Reproduction and Embryology came together with United Kingdom National External Quality Assessment Services for Molecular Genetics, to create a pilot EQA scheme followed by practical EQA schemes for all interested parties. Here, we detail the development of the pilot scheme as well as development and findings from the practical (clinical) schemes that have followed. Results were generally acceptable and there was marked improvement in results and laboratory scores for those labs that participated in multiple schemes. Data from the first three schemes indicate that the EQA scheme is working as planned and has helped laboratories improve their techniques and result reporting. The EQA scheme for monogenic PGD will continue to be developed to offer assessment for other monogenic disorders.

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