Developmental potential of murine germinal vesicle stage cumulus-oocyte complexes following exposure to dimethylsulphoxide or cryopreservation: loss of membrane integrity of cumulus cells after thawing

doi:10.1093/humrep/deg071

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Human Reproduction, Vol. 18, No. 2, 392-398, February 2003
© 2003 European Society of Human Reproduction and Embryology

Developmental potential of murine germinal vesicle stage cumulus–oocyte complexes following exposure to dimethylsulphoxide or cryopreservation: loss of membrane integrity of cumulus cells after thawing

C.J. Ruppert-Lingham¹^,3, S.J. Paynter¹, J. Godfrey¹, B.J. Fuller¹ and R.W. Shaw¹^,2

¹ Department of Obstetrics and Gynaecology, University of Wales College of Medicine, Heath Park, Cardiff CF14 4XN, UK

² Present address: Academic Division of Obstetrics and Gynaecology, Derby City General Hospital, Uttoxeter Road, Derby DE22 3NE, UK

³ To whom correspondence should be addressed. e-mail: Ruppert-LinghamCJ{at}cardiff.ac.uk

BACKGROUND: Cumulus cells of the cumulus–oocyte complex(COC) are important in oocyte maturation. Thus, in preservingimmature oocytes it is prudent to also preserve their associatedcumulus cells. The survival and function of oocytes and theirassociated cumulus cells was assessed following cryopreservationor exposure to cryoprotectant without freezing. METHODS: ImmatureCOCs were collected from mice primed with pregnant mare’sserum. COCs were either slow-cooled or exposed to 1.5 mol/ldimethylsulphoxide without freezing. Treated and fresh COCswere stained for membrane integrity or, after in-vitro maturationand IVF, were assessed for developmental capability. Developmentof cumulus-denuded fresh oocytes, as well as denuded and frozen–thawedoocytes co-cultured with fresh cumulus cells, was assessed.RESULTS: Slow-cooled oocytes had significantly reduced coverageby intact cumulus cells compared with fresh COCs. Cumulus cellassociation and developmental capability were not substantiallyaffected by exposure to cryoprotectant without freezing. Denudedfresh oocytes and cryopreserved COCs had decreased developmentalpotential that was not overcome by co-culture with fresh cumuluscells. CONCLUSIONS: Loss of association between oocyte and cumuluscells was induced by cryopreservation, but not by treatmentwith cryoprotectant alone. The data indicate that direct physicalcontact between cumulus cells and the oocyte, throughout maturation,improves subsequent embryo development.

Key words: cryopreservation/cumulus–oocyte complex/dimethylsulphoxide/GV-stage oocytes/maturation

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