Morphokinetic changes in vitrified and non-vitrified in vitro-derived ovine embryos

Karolina Fryc; Agnieszka Nowak; Barbara Kij-Mitka; Joanna Kochan; Pawel M Bartlewski; Maciej Murawski

doi:10.1016/j.theriogenology.2022.04.027

Morphokinetic changes in vitrified and non-vitrified in vitro-derived ovine embryos

Theriogenology. 2022 Jul 15:187:58-63. doi: 10.1016/j.theriogenology.2022.04.027. Epub 2022 Apr 26.

Authors

Karolina Fryc¹, Agnieszka Nowak², Barbara Kij-Mitka², Joanna Kochan², Pawel M Bartlewski³, Maciej Murawski⁴

Affiliations

¹ Department of Animal Nutrition and Biotechnology, and Fisheries, University of Agriculture in Kraków, 24/28 Mickiewicza Ave., 30-059, Cracow, Poland. Electronic address: karolina.fryc@student.urk.edu.pl.
² Department of Animal Reproduction, Anatomy and Genomics, University of Agriculture in Kraków, 24/28 Mickiewicza Ave., 30-059, Cracow, Poland.
³ Department of Biomedical Sciences, Ontario Veterinary College, University of Guelph, 50 Stone Rd., Guelph, ON, N1G 2W1, Canada.
⁴ Department of Animal Nutrition and Biotechnology, and Fisheries, University of Agriculture in Kraków, 24/28 Mickiewicza Ave., 30-059, Cracow, Poland.

PMID: 35504088
DOI: 10.1016/j.theriogenology.2022.04.027

Abstract

The present experiment employed time-lapse (TL) imaging to assess the effects of vitrification on the development of ovine blastocysts and to see if the timing of blastocyst formation and expansion was correlated with the numbers of embryo- and trophoblasts determined through differential staining of the expanded blastocysts. Ovaries were obtained after slaughter from cycling (October-March) Polish Longwool ewes aged 1-3 years and cumulus-oocyte complexes were collected by ovarian scarification. In vitro maturation was performed in TCM 199 medium supplemented with Earle's Salt, 10% of FBS, and 5 μg/mL of LH/FSH at 38 °C for 24 h. After maturation, the oocytes were incubated with thawed ram semen (IVF) for 19 h and all presumptive zygotes were transferred to a 16-well dish containing Cult medium for monitoring with the Primo Vision TL system. A portion of ovine embryos were vitrified (Cryotop system) at the early cavitation stage and TL observations of warmed (n = 30) and non-vitrified (n = 32) blastocysts continued until the attainment of the expanded blastocyst stage, at which point they were differentially stained with bisbenzimide and propidium iodide for microscopic enumeration of embryoblasts (inner cell mass blastomeres) and trophoblast-cells. There were no statistically significant differences in the timing of blastulation (tB) and formation of expanded blastocysts (tEB) between vitrified and non-vitrified ovine embryos, but non-vitrified blastocysts exceeded (P < 0.05) their vitrified and warmed counterparts in the mean number of embryo- and trophoblasts. In addition, the number of trophoblasts was negatively and moderately correlated with tB and tEB, for both vitrified and non-vitrified embryos. It can be concluded that even though vitrification of ovine embryos is associated with a significant reduction in the number of blastomeres, the rate of blastocyst development remains closely linked to the numbers of trophoblastic cells.

Keywords: Embryo; Inner cell mass; Sheep; Time-lapse imaging; Trophoblast; Vitrification.

MeSH terms

Animals
Blastocyst
Cryopreservation* / methods
Cryopreservation* / veterinary
Embryonic Development
Female
Male
Oocytes
Sheep
Sheep, Domestic
Vitrification*