Cellular damage suffered by equine embryos after exposure to cryoprotectants or cryopreservation by slow-freezing or vitrification

W K Hendriks; B A J Roelen; B Colenbrander; T A E Stout

doi:10.1111/evj.12341

Cellular damage suffered by equine embryos after exposure to cryoprotectants or cryopreservation by slow-freezing or vitrification

Equine Vet J. 2015 Nov;47(6):701-7. doi: 10.1111/evj.12341. Epub 2014 Oct 19.

Authors

W K Hendriks¹, B A J Roelen², B Colenbrander¹, T A E Stout²

Affiliations

¹ Department of Equine Sciences, Faculty of Veterinary Medicine, Utrecht University, The Netherlands.
² Department of Farm Animal Health, Faculty of Veterinary Medicine, Utrecht University, The Netherlands.

PMID: 25187202
DOI: 10.1111/evj.12341

Abstract

Reasons for performing study: Equine embryos are cryopreserved by slow-freezing or vitrification. While small embryos (<300 μm) survive cryopreservation reasonably well, larger embryos do not. It is not clear if slow-freezing or vitrification is less damaging to horse embryos.

Objectives: To compare the type and extent of cellular damage suffered by small and large embryos during cryopreservation by slow-freezing vs. vitrification.

Study design: Sixty-three Day 6.5-7 embryos were subdivided by size and assigned to one of 5 treatments: control, exposure to slow-freezing or vitrification cryoprotectants (CPs), and cryopreservation by either technique.

Methods: After thawing/CP removal, embryos were stained with fluorescent stains for various parameters of cellular integrity, and assessed by multiphoton microscopy.

Results: Exposing large embryos to vitrification CPs resulted in more dead cells (6.8 ± 1.3%: 95% confidence interval [CI], 3.1-10.4%) than exposure to slow-freezing media (0.3 ± 0.1%; 95% CI 0.0-0.6%: P = 0.001). Cryopreservation by either technique induced cell death and cytoskeleton disruption. Vitrification of small embryos resulted in a higher proportion of cells with fragmented or condensed (apoptotic) nuclei (P = 0.002) than slow-freezing (6.7 ± 1.5%, 95% CI 3.0-10.4% vs. 5.0 ± 2.1%, 95% CI 4.0-14.0%). Slow-freezing resulted in a higher incidence of disintegrated embryos (P = 0.01) than vitrification. Mitochondrial activity was low in control embryos, and was not differentially affected by cryopreservation technique, whereas vitrification changed mitochondrial distribution from a homogenous crystalline pattern in control embryos to a heterogeneous granulated distribution in vitrified embryos (P = 0.05).

Conclusions: Cryopreservation caused more cellular damage to large embryos than smaller ones. While vitrification is more practical, it is not advisable for large embryos due to a higher incidence of dead cells. The choice is less obvious for small embryos, as vitrification led to occasionally very high percentages of dead or damaged cells, but a lower incidence of embryo disintegration. Modifications that reduce the level of cellular damage induced by vitrification are required before it can be considered the method of choice for cryopreserving equine embryos.

Keywords: cryopreservation; embryo; horse; slow-freezing; vitrification.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Cryopreservation / veterinary*
Cryoprotective Agents / adverse effects*
Embryo Culture Techniques
Embryo, Mammalian / drug effects*
Embryonic Development
Freezing*
Horses / embryology*
Time Factors
Vitrification*

Substances

Cryoprotective Agents