Genomic assessment of follicular marker genes as pregnancy predictors for human IVF

doi:10.1093/molehr/gap079

Mol. Hum. Reprod. Advance Access published online on September 24, 2009
Molecular Human Reproduction, doi:10.1093/molehr/gap079

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© The Author 2009. Published by Oxford University Press on behalf of the European Society of Human Reproduction and Embryology. All rights reserved. For Permissions, please email: journals.permissions@oxfordjournals.org

Genomic assessment of follicular marker genes as pregnancy predictors for human IVF

Mélanie Hamel¹, Isabelle Dufort¹, Claude Robert¹, Marie-Claude Leveillé², Arthur Leader² and Marc-André Sirard¹^,3

¹Centre de recherche en biologie de la reproduction, Université Laval, Québec, Canada ²Ottawa Fertility Centre, Ottawa, Canada

³ Corresponding author : Marc-André Sirard, Département des Science Animales, Centre de Recherche en Biologie de la Reproduction (CRBR), Université Laval, QC, Canada, G1K 7P4. Tel: 418-656-7359. Fax: 418-656-3766. E-mail: Marc-Andre.Sirard{at}fsaa.ulaval.ca

Embryo selection efficiency in human IVF procedure is stillsuboptimal as shown by low pregnancy rates with single embryotransfer (SET). Bidirectional communication between the oocyteand follicular cells (FC) is essential to achieve developmentalcompetence of the oocyte. Differences in the gene expressionprofile of FCs from follicles leading to pregnancy could provideuseful markers of oocyte developmental competence. FCs wererecovered by individual follicle puncture. FC expression levelsof potential markers were assessed by Q-PCR with an intra-patientand an inter-patient analysis approach. Using gene expression,a predictive model of ongoing pregnancy was investigated. Usingintra-patient analysis, 4 candidate genes, phosphoglyceratekinase 1 (PGK1), regulator of G-protein signalling 2 (RGS2),regulator of G-protein signalling 3 (RGS3) and cell divisioncycle 42 (CDC42) showed a difference between FCs from folliclesleading to a pregnancy or developmental failure. The best predictorsfor ongoing pregnancy were PGK1 and RGS2. Additionally, inter-patientanalysis revealed differences in FC expression for PGK1 andCDC42 between follicles leading to a transferred embryo withpositive pregnancy results and those with negative results.Both inter-patient and intra-patient approaches must be takeninto consideration to delineate gene expression variations inthe context of follicular competence. A predictor model usingbiomarkers could improve the efficiency of predicting developmentalcompetence of oocytes. These new approaches provide useful toolsin the context of embryo selection and in the improvement ofpregnancy rates with SET.

Submitted on April 7, 2009; resubmitted on August 30, 2009; accepted on September 3, 2009.

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