Vitrifying expanded equine embryos collapsed by blastocoel aspiration is less damaging than slow-freezing

M Umair; M Beitsma; M de Ruijter-Villani; C Deelen; C Herrera; T A E Stout; A Claes

doi:10.1016/j.theriogenology.2023.02.028

Vitrifying expanded equine embryos collapsed by blastocoel aspiration is less damaging than slow-freezing

M Umair^*, M Beitsma, M de Ruijter-Villani, C Deelen, C Herrera, T A E Stout, A Claes

^*Corresponding author for this work

University of Zurich

Research output: Contribution to journal › Article › Academic › peer-review

Abstract

The cryotolerance of equine blastocysts larger than 300 μm can be improved by aspirating blastocoele fluid prior to vitrification; however, it is not known whether blastocoele aspiration also enables successful slow-freezing. The aim of this study was therefore to determine whether slow-freezing of expanded equine embryos following blastocoele collapse was more or less damaging than vitrification. Grade 1 blastocysts recovered on day 7 or 8 after ovulation were measured (>300-550 μm, n = 14 and > 550 μm, n = 19) and blastocoele fluid was aspirated prior to slow-freezing in 10% glycerol (n = 14), or vitrification (n = 13) in 16.5% ethylene glycol/16.5% DMSO/0.5 M sucrose. Immediately after thawing or warming, embryos were cultured for 24 h at 38 °C and then graded and measured to assess re-expansion. Control embryos (n = 6) were cultured for 24 h following aspiration of blastocoel fluid, without cryopreservation or exposure to cryoprotectants. Subsequently, embryos were stained to assess live/dead cell proportion (DAPI/TOPRO-3), cytoskeleton quality (Phalloidin) and capsule integrity (WGA). For 300-550 μm embryos, quality grade and re-expansion were impaired after slow-freezing but not affected by vitrification. Slow-freezing embryos >550 μm induced additional cell damage as indicated by a significant increase in dead cell proportion and disruption of the cytoskeleton; neither of these changes were observed in vitrified embryos. Capsule loss was not a significant consequence of either freezing method. In conclusion, slow-freezing of expanded equine blastocysts collapsed by blastocoel aspiration compromises post-thaw embryo quality more than vitrification.

Original language	English
Pages (from-to)	28-35
Number of pages	8
Journal	Theriogenology
Volume	202
Early online date	2 Mar 2023
DOIs	https://doi.org/10.1016/j.theriogenology.2023.02.028
Publication status	Published - May 2023

Bibliographical note

Funding Information:
Authors acknowledge the help of Bart Leemans and Soledad Martin Pelaez with embryo flushing, and Jon de Rijk, Wilbert Beukens, Esther Akkermans and Leonie Arnold with semen collection. The authors thank the Punjab Educational Endowment Fund (PEEF), Punjab, Pakistan (PEEF/SSMS/18/222) for supporting this study. Confocal imaging and image analyses were performed at the Center for Cell Imaging (CCI) at the Faculty of Veterinary Medicine, Utrecht University (Utrecht, The Netherlands). The authors also thank Richard Wubbolts and Esther van t Veld for their help and technical support in confocal imaging and image analyses.

Publisher Copyright:
© 2023 The Authors

Keywords

Equine
Embryo
Blastocoel collapse
Cryopreservation
Slow-freezing
Vitrification

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1-s2.0-S0093691X23000778-mainFinal published version, 2.42 MBLicence: CC BY-NC-ND

Cite this

@article{3963fe925a4f40949d051b68ad78121b,

title = "Vitrifying expanded equine embryos collapsed by blastocoel aspiration is less damaging than slow-freezing",

abstract = "The cryotolerance of equine blastocysts larger than 300 μm can be improved by aspirating blastocoele fluid prior to vitrification; however, it is not known whether blastocoele aspiration also enables successful slow-freezing. The aim of this study was therefore to determine whether slow-freezing of expanded equine embryos following blastocoele collapse was more or less damaging than vitrification. Grade 1 blastocysts recovered on day 7 or 8 after ovulation were measured (>300-550 μm, n = 14 and > 550 μm, n = 19) and blastocoele fluid was aspirated prior to slow-freezing in 10\% glycerol (n = 14), or vitrification (n = 13) in 16.5\% ethylene glycol/16.5\% DMSO/0.5 M sucrose. Immediately after thawing or warming, embryos were cultured for 24 h at 38 °C and then graded and measured to assess re-expansion. Control embryos (n = 6) were cultured for 24 h following aspiration of blastocoel fluid, without cryopreservation or exposure to cryoprotectants. Subsequently, embryos were stained to assess live/dead cell proportion (DAPI/TOPRO-3), cytoskeleton quality (Phalloidin) and capsule integrity (WGA). For 300-550 μm embryos, quality grade and re-expansion were impaired after slow-freezing but not affected by vitrification. Slow-freezing embryos >550 μm induced additional cell damage as indicated by a significant increase in dead cell proportion and disruption of the cytoskeleton; neither of these changes were observed in vitrified embryos. Capsule loss was not a significant consequence of either freezing method. In conclusion, slow-freezing of expanded equine blastocysts collapsed by blastocoel aspiration compromises post-thaw embryo quality more than vitrification.",

keywords = "Equine, Embryo, Blastocoel collapse, Cryopreservation, Slow-freezing, Vitrification",

author = "M Umair and M Beitsma and \{de Ruijter-Villani\}, M and C Deelen and C Herrera and Stout, \{T A E\} and A Claes",

note = "Funding Information: Authors acknowledge the help of Bart Leemans and Soledad Martin Pelaez with embryo flushing, and Jon de Rijk, Wilbert Beukens, Esther Akkermans and Leonie Arnold with semen collection. The authors thank the Punjab Educational Endowment Fund (PEEF), Punjab, Pakistan (PEEF/SSMS/18/222) for supporting this study. Confocal imaging and image analyses were performed at the Center for Cell Imaging (CCI) at the Faculty of Veterinary Medicine, Utrecht University (Utrecht, The Netherlands). The authors also thank Richard Wubbolts and Esther van t Veld for their help and technical support in confocal imaging and image analyses. Publisher Copyright: {\textcopyright} 2023 The Authors",

year = "2023",

month = may,

doi = "10.1016/j.theriogenology.2023.02.028",

language = "English",

volume = "202",

pages = "28--35",

journal = "Theriogenology",

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T1 - Vitrifying expanded equine embryos collapsed by blastocoel aspiration is less damaging than slow-freezing

AU - Umair, M

AU - Beitsma, M

AU - de Ruijter-Villani, M

AU - Deelen, C

AU - Herrera, C

AU - Stout, T A E

AU - Claes, A

N1 - Funding Information: Authors acknowledge the help of Bart Leemans and Soledad Martin Pelaez with embryo flushing, and Jon de Rijk, Wilbert Beukens, Esther Akkermans and Leonie Arnold with semen collection. The authors thank the Punjab Educational Endowment Fund (PEEF), Punjab, Pakistan (PEEF/SSMS/18/222) for supporting this study. Confocal imaging and image analyses were performed at the Center for Cell Imaging (CCI) at the Faculty of Veterinary Medicine, Utrecht University (Utrecht, The Netherlands). The authors also thank Richard Wubbolts and Esther van t Veld for their help and technical support in confocal imaging and image analyses. Publisher Copyright: © 2023 The Authors

PY - 2023/5

Y1 - 2023/5

N2 - The cryotolerance of equine blastocysts larger than 300 μm can be improved by aspirating blastocoele fluid prior to vitrification; however, it is not known whether blastocoele aspiration also enables successful slow-freezing. The aim of this study was therefore to determine whether slow-freezing of expanded equine embryos following blastocoele collapse was more or less damaging than vitrification. Grade 1 blastocysts recovered on day 7 or 8 after ovulation were measured (>300-550 μm, n = 14 and > 550 μm, n = 19) and blastocoele fluid was aspirated prior to slow-freezing in 10% glycerol (n = 14), or vitrification (n = 13) in 16.5% ethylene glycol/16.5% DMSO/0.5 M sucrose. Immediately after thawing or warming, embryos were cultured for 24 h at 38 °C and then graded and measured to assess re-expansion. Control embryos (n = 6) were cultured for 24 h following aspiration of blastocoel fluid, without cryopreservation or exposure to cryoprotectants. Subsequently, embryos were stained to assess live/dead cell proportion (DAPI/TOPRO-3), cytoskeleton quality (Phalloidin) and capsule integrity (WGA). For 300-550 μm embryos, quality grade and re-expansion were impaired after slow-freezing but not affected by vitrification. Slow-freezing embryos >550 μm induced additional cell damage as indicated by a significant increase in dead cell proportion and disruption of the cytoskeleton; neither of these changes were observed in vitrified embryos. Capsule loss was not a significant consequence of either freezing method. In conclusion, slow-freezing of expanded equine blastocysts collapsed by blastocoel aspiration compromises post-thaw embryo quality more than vitrification.

AB - The cryotolerance of equine blastocysts larger than 300 μm can be improved by aspirating blastocoele fluid prior to vitrification; however, it is not known whether blastocoele aspiration also enables successful slow-freezing. The aim of this study was therefore to determine whether slow-freezing of expanded equine embryos following blastocoele collapse was more or less damaging than vitrification. Grade 1 blastocysts recovered on day 7 or 8 after ovulation were measured (>300-550 μm, n = 14 and > 550 μm, n = 19) and blastocoele fluid was aspirated prior to slow-freezing in 10% glycerol (n = 14), or vitrification (n = 13) in 16.5% ethylene glycol/16.5% DMSO/0.5 M sucrose. Immediately after thawing or warming, embryos were cultured for 24 h at 38 °C and then graded and measured to assess re-expansion. Control embryos (n = 6) were cultured for 24 h following aspiration of blastocoel fluid, without cryopreservation or exposure to cryoprotectants. Subsequently, embryos were stained to assess live/dead cell proportion (DAPI/TOPRO-3), cytoskeleton quality (Phalloidin) and capsule integrity (WGA). For 300-550 μm embryos, quality grade and re-expansion were impaired after slow-freezing but not affected by vitrification. Slow-freezing embryos >550 μm induced additional cell damage as indicated by a significant increase in dead cell proportion and disruption of the cytoskeleton; neither of these changes were observed in vitrified embryos. Capsule loss was not a significant consequence of either freezing method. In conclusion, slow-freezing of expanded equine blastocysts collapsed by blastocoel aspiration compromises post-thaw embryo quality more than vitrification.

KW - Equine

KW - Embryo

KW - Blastocoel collapse

KW - Cryopreservation

KW - Slow-freezing

KW - Vitrification

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DO - 10.1016/j.theriogenology.2023.02.028

M3 - Article

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SN - 0093-691X

VL - 202

SP - 28

EP - 35

JO - Theriogenology

JF - Theriogenology

ER -

Vitrifying expanded equine embryos collapsed by blastocoel aspiration is less damaging than slow-freezing

Abstract

Bibliographical note

Keywords

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