Comparison of three in vitro culture systems for maturation of early preantral mouse ovarian follicles

The aim of this study was to compare three different culture systems for in vitro follicular growth and oocyte maturation in ovarian follicles of mice in order to assess the technique with the optimal growth and improved rate of meiotic maturation. The three systems tested were culture under oil, on...

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Bibliographic Details
Published in:Zygote (Cambridge) 2005-05, Vol.13 (2), p.167-175
Main Authors: Mousset-Siméon, Nathalie, Jouannet, Pierre, Le Cointre, Laëtitia, Coussieu, Christiane, Poirot, Catherine
Format: Article
Language:English
Subjects:
Agar
Animals
Culture
Culture Media
Estradiol
Female
Maturation
Membranes, Artificial
Mice
Mice, Inbred C57BL
Mineral Oil
Mouse
Oocyte
Oocytes - cytology
Oocytes - growth & development
Organic Chemicals
Ovarian Follicle - cytology
Ovarian Follicle - growth & development
Preantral follicle
Tissue Culture Techniques - methods
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Summary:The aim of this study was to compare three different culture systems for in vitro follicular growth and oocyte maturation in ovarian follicles of mice in order to assess the technique with the optimal growth and improved rate of meiotic maturation. The three systems tested were culture under oil, on a hydrophobic membrane and on agar respectively. Early preantral follicles were cultured for 12 days in α-MEM GlutaMAX medium. Follicular growth, oocyte meiotic maturation, oocyte extrusion, atresia and estradiol production were analysed. Follicular development showed two phases in the three systems, with slow growth before day 5 and subsequent acceleration. The percentage of follicles transferred into oocyte maturation medium was significantly higher after culture under oil. The proportion of oocytes that achieved nuclear maturation (metaphase II) was higher when follicles were cultured under oil or on a hydrophobic membrane than on agar. Our results support the use of culture under oil for in vitro follicular growth from the early preantral stage in order to obtain metaphase II oocytes. Fertilization ability of these oocytes and the capacity to obtain healthy mice in a reproducible manner warrants further investigation.
ISSN:0967-1994
1469-8730
DOI:10.1017/S0967199405003151