Cryopreservation of bovine ovarian tissue : Structural normality of follicles after thawing and culture in vitro

The recovery of viable follicles from cryopreserved ovarian tissue would be of benefit in many areas of assisted reproduction. Structural integrity needs to be maintained following cryopreservation of ovarian tissue in order to retrieve healthy follicles which can then be cultured in vitro to produc...

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Published inCryobiology Vol. 38; no. 4; pp. 301 - 309
Main Authors PAYNTER, S. J, COOPER, A, FULLER, B. J, SHAW, R. W
Format Journal Article
LanguageEnglish
Published San Diego, CA Elsevier 01.06.1999
Subjects
Animals
Biological and medical sciences
Cattle
Cryopreservation
Culture Techniques
dimethylsulphoxide
Female
Fundamental and applied biological sciences. Psychology
Mammalian female genital system
Morphology. Physiology
Ovarian Follicle - cytology
Vertebrates: reproduction
Ox
Thawing
Germinal cell
Ovary
Vertebrata
Mammalia
Investigation method
Cryopreservation
Female genital system
Artiodactyla
Ovarian follicle
Ungulata
Oocyte
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Summary:The recovery of viable follicles from cryopreserved ovarian tissue would be of benefit in many areas of assisted reproduction. Structural integrity needs to be maintained following cryopreservation of ovarian tissue in order to retrieve healthy follicles which can then be cultured in vitro to produce viable oocytes. We have assessed the effect of in vitro culture of bovine tissue for 0, 1, 4, 24, or 48 h after exposure to, or cryopreservation in, dimethylsulphoxide. Immediately after freezing, normality of primary and preantral follicles within the tissue was significantly lower than for tissue exposed to the cryoprotectant without freezing or for control tissue. After 4 h in culture, cryopreserved tissue appeared to have recovered from damage caused by freezing, although the percentage of tissue with normal morphology declined after 24 and 48 h of culture. There was no significant difference between percentage normality in control tissue and tissue exposed to the cryoprotectant without freezing for any of the culture times studied. These data indicate that it is possible to freeze/thaw bovine ovarian tissue while retaining a reasonable yield of morphologically intact follicles and that a short period of post-thaw culture may enhance follicle recovery.
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ISSN:0011-2240
1090-2392
DOI:10.1006/cryo.1999.2170