Vitrification of in vitro-produced and in vivo-recovered equine blastocysts in a clinical program.
Abstract: There is a clinical demand for cryopreservation of both in vivo-recovered and in vitro-produced (IVP) equine embryos. We previously reported successful vitrification of expanded equine blastocysts in fine-diameter microloader pipette tips (MPTs) after blastocoel collapse, in a research setting. Here, we report the results of clinical application of the MPT vitrification technique for both in vivo-recovered and IVP blastocysts. In vivo-recovered blastocysts were obtained by referring veterinarians on Days 6 to 8 after ovulation, and shipped 1 to 10 hours to the laboratory before vitrification. IVP blastocysts (<300 μm in diameter) were produced by intracytoplasmic sperm injection and in vitro embryo culture. All vitrified-warmed embryos were shipped (0.5-12 hours) for transfer to recipient mares. In experiment 1, 47 IVP embryos from our clinical intracytoplasmic sperm injection program were vitrified using the MPT and transferred. The rates of initial pregnancy (59%) and foaling (45%) were equivalent to those for 52 IVP embryos from the same mare aspiration sessions and shipped for the same duration but transferred fresh (75% and 45%, respectively). The pregnancy and foaling rates for in vivo-recovered embryos were 76 and 71%, respectively for 17 small blastocysts (<300 μm in diameter), and 55 and 45%, respectively for 11 large blastocysts (303-608 μm in diameter, collapsed before vitrification; P > 0.1). In experiment 2, the MPT was cut lengthwise to form an open vitrification device, designated "Sujo". Research IVP blastocysts were vitrified at 1, 2, or 3 embryos per Sujo (n = 34 embryos), or singly on a commercial open device (Cryolock; n = 11). After warming, 97% and 91% of embryos, respectively, grew in culture. Similarly, culture of two in vivo-recovered large blastocysts after collapse and vitrification on Sujos both resulted in embryo growth. However, transfer of four in vivo-recovered expanded blastocysts after collapse, vitrification on Sujos, and warming resulted in only one foal. These data indicate that vitrification of equine IVP embryos and small in vivo-recovered embryos is efficient under clinical conditions. Collapse and vitrification of in vivo-recovered large blastocysts in MPT under our clinical conditions resulted in a 45% foaling rate. While numbers are low, use of an open vitrification system did not appear to improve results for these embryos.
Copyright © 2016 Elsevier Inc. All rights reserved.
Publication Date: 2016-08-13 PubMed ID: 27634397DOI: 10.1016/j.theriogenology.2016.08.005Google Scholar: Lookup
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- Journal Article
Summary
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The abstract discusses a study about cryopreservation (freezing) of equine (horse) embryos produced both naturally and in a lab (in vitro). The researchers used a process called vitrification, freezing the embryos rapidly to preserve them, either in a microloader pipette tips (MPTs) or an open device called Sujo. The results showed that the procedure can be used efficiently to preserve both types of embryos.
Methodology
- Embryos used for the research came from two sources: some were obtained naturally from mares by veterinarians, and others were made artificially in a lab.
- Embryos were transported to the lab where the vitrification process was carried out.
- After vitrification, the embryos were shipped to recipient mares for pregnancy attempt.
Experiments and Results
- In the first experiment, 47 lab-made embryos were vitrified and transferred to mares. The rates of initially successful pregnancy (59%) and eventual foal births (45%) were comparable to embryos that were transferred without freezing (75% pregnancy and 45% foaling rates).
- Natural embryos also showed high success with a 76% pregnancy and 71% foaling rate for smaller embryos (<300 μm). Larger embryos (303-608 μm) had slightly lower rates at 55% for pregnancies and 45% for foal births.
- The second experiment tested a different freezing device, Sujo, which had a sizeable success rate in restoring embryos to viable conditions after warming, with 97% and 91% success for lab-made and natural embryos respectively.
- However, only one foal was born out of four embryos subjected to the Sujo process, suggesting it may not be as effective for natural, expanded blastocysts.
Conclusions
- The research demonstrates that vitrification is a feasible way to preserve equine embryos created both in vivo and in vitro.
- The freezing process did not drastically hinder the chances of successful pregnancy and foal births, making it a viable technique in a clinical setting.
- Still, results were worse for larger, in vivo-recovered embryos. And while the open vitrification system (Sujo) looked promising in preliminary lab-tests, it ultimately failed to improve results for these larger embryos.
Cite This Article
APA
Choi YH, Hinrichs K.
(2016).
Vitrification of in vitro-produced and in vivo-recovered equine blastocysts in a clinical program.
Theriogenology, 87, 48-54.
https://doi.org/10.1016/j.theriogenology.2016.08.005 Publication
Researcher Affiliations
- Department of Veterinary Physiology & Pharmacology, College of Veterinary Medicine & Biomedical Sciences, Texas A&M University, College Station, Texas, USA. Electronic address: yhchoi@cvm.tamu.edu.
- Department of Veterinary Physiology & Pharmacology, College of Veterinary Medicine & Biomedical Sciences, Texas A&M University, College Station, Texas, USA.
MeSH Terms
- Animals
- Blastocyst / physiology
- Cryopreservation / veterinary
- Female
- Fertilization in Vitro / veterinary
- Horses / embryology
- Oocytes
- Tissue and Organ Harvesting / veterinary
- Vitrification
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