Please use this identifier to cite or link to this item: https://hdl.handle.net/1959.11/18835
Title: Optimization of a vitrification protocol for hatched blastocysts from the dromedary camel ('Camelus dromedarius')
Contributor(s): Herrid, Muren  (author); Billah, M (author); Malo, C (author); Skidmore, J A (author)
Publication Date: 2016
DOI: 10.1016/j.theriogenology.2015.09.048
Handle Link: https://hdl.handle.net/1959.11/18835
Abstract: The objective of this study was to modify and optimize a vitrification protocol (open pulled straw) that was originally designed for human oocytes and embryos, to make it suitable for the cryopreservation of camel hatched blastocysts. The original open pulled straw protocol was a complex process with 15-minute exposure of oocytes/embryos in 7.5% ethylene glycol (EG) and 7.5% dimethyl sulfoxide (Me₂SO) for equilibration, and cooling in 16% EG + 16% Me₂SO + 1 M sucrose. Recognizing a need to better control the cryoprotectant (CPA) concentrations, while avoiding toxicity to the embryos, the effects on the survival rate and developmental potential of camel embryos in vitro were investigated using two different methods of loading the CPAs into the embryos (stepwise and semicontinuous increase in concentration), two different loading temperature/time (room temperature ~°C/15 min and body 37°C/3 min), and the replacement of Me₂SO with EG alone or in combination with glycerol (Gly). A total of 145 in vivo-derived embryos were subjected to these processes, and after warming their morphological quality and integrity, and reexpansion was assessed after 0, 2, 24, 48, 72, and 96 hours of culture. Exposure of embryos in a stepwise method was more beneficial to the survival of embryos than was the semicontinuous process, and loading of CPAs at 37°C with a short exposure time (3 minutes) resulted in an outcome comparable to the original processing at room temperature with a longer exposure time (15 minutes). The replacement of the Me₂SO + EG mixture with EG only or a combination of EG + Gly in the vitrification medium significantly improved the outcome of all these evaluation criteria (P < 0.05). The modified protocol of loading EG at 37°C for 3 minutes has increased the embryo survival of the original protocol from 67% to 91% and the developmental rate from 57% to 83% at 5-day culture. These results were comparable to or better than those reported in human or other species, indicating that this optimized method is well suited to any commercial embryo transfer program in the dromedary camel.
Publication Type: Journal Article
Source of Publication: Theriogenology, 85(4), p. 585-590
Publisher: Elsevier Inc
Place of Publication: United States of America
ISSN: 1879-3231
0093-691X
Fields of Research (FoR) 2008: 070206 Animal Reproduction
070702 Veterinary Anatomy and Physiology
Fields of Research (FoR) 2020: 300305 Animal reproduction and breeding
300902 Veterinary anatomy and physiology
Socio-Economic Objective (SEO) 2008: 970106 Expanding Knowledge in the Biological Sciences
970111 Expanding Knowledge in the Medical and Health Sciences
970107 Expanding Knowledge in the Agricultural and Veterinary Sciences
Socio-Economic Objective (SEO) 2020: 280102 Expanding knowledge in the biological sciences
Peer Reviewed: Yes
HERDC Category Description: C1 Refereed Article in a Scholarly Journal
Appears in Collections:Journal Article
School of Environmental and Rural Science

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