Cryopreservation of canine ovarian tissue by slow freezing and vitrification: Evaluation of follicular morphology and apoptosis rate

Cryopreservation of canine ovarian tissue by slow freezing and vitrification: Evaluation of follicular morphology and apoptosis rate

In this study, we aimed to evaluate the efficacy of cryopreserving canine ovarian tissue using vitrification and slow freezing methods while investigating potential differences in cryotolerance based on follicular type and cryopreservation technique. Twenty-eight ovaries were collected from 14 anoes...

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Bibliographic Details
Published in:Theriogenology Vol. 230; pp. 8 - 14
Main Authors: Luizari Stábile, Nicole A., Oliveira, Frederico Rocha de, Furtado, Ricardo Andrade, Felippe, Carolina Barretto M.L., Tavares, Mariana Riboli, Martinelli, Paulo E.B., Fonseca-Alves, Carlos Eduardo, Souza, Fabiana Ferreira de, Colombo, Martina, Luvoni, Gaia Cecilia, Apparício, Maricy
Format: Journal Article
Language:English
Published: United States Elsevier Inc 01-12-2024
Subjects:
Bitches
Caspase-3
Gonadal tissue
Histology
Immunohistochemistry
Immunohistochemistry
Bitches
Gonadal tissue
Histology
Caspase-3
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Summary:In this study, we aimed to evaluate the efficacy of cryopreserving canine ovarian tissue using vitrification and slow freezing methods while investigating potential differences in cryotolerance based on follicular type and cryopreservation technique. Twenty-eight ovaries were collected from 14 anoestrus bitches of various breeds, aged between 2 and 5 years, and undergoing elective ovariohysterectomy. The ovaries were sectioned into small fragments and randomly assigned to three groups: vitrification, slow freezing, and a control group (fresh tissue). Vitrification was performed using cryotubes containing DAP 213 solution (2M DMSO, 1M acetamide, 3M propylene glycol) in two stages, while slow freezing involved cryotubes with 1.5M DMSO solution inserted into a programmable machine. The effects of cryopreservation were evaluated by histology and immunohistochemistry (cleaved caspase-3), to determine the percentage of cells undergoing apoptosis. Histological examination revealed that the slow freezing group exhibited a significantly higher percentage of intact follicles (45.75 %) compared to those subjected to vitrification (38.17 %; P = 0.01). Immunohistochemical evaluation further indicated that 84.21 % of the follicles in the slow freezing group did not express caspase-3, suggesting the absence of apoptosis. Conversely, vitrified samples exhibited significantly more apoptotic cells compared to other groups (P < 0.001). Furthermore, early antral follicles displayed a higher susceptibility to degeneration regardless of the cryopreservation method employed. Nevertheless, when comparing the cryopreserved groups, early antral follicles showed greater degeneration in slow freezing group, while preantral follicles were the most affected in the vitrification group. In conclusion, slow freezing demonstrated superior preservation of viable follicles compared to vitrification and emerged as the preferred technique for cryopreserving canine ovarian tissue. These findings contribute valuable insights into optimizing cryopreservation methods for canine ovarian tissue, potentially benefiting reproductive technologies and fertility preservation in canines. •There are differences in follicular cryotolerance according to the cryopreservation technique used.•Primordial and immature follicles are less prone to degeneration when cryopreserved by slow freezing.•Mature follicles are more sensitive to cryodamage and better preserved by vitrification.
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ISSN:0093-691X
1879-3231
1879-3231
DOI:10.1016/j.theriogenology.2024.08.032