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Influence of Embryonic Size and Manipulation on Pregnancy Rates of Mares After Transfer of Cryopreserved Equine Embryos
Institution:1. PS Pferdehaltung, Neustadt-Glewe, Germany;2. Clinic for Horses—Unit for Reproductive Medicine, University of Veterinary Medicine Hannover, Hannover, Germany;3. Clinic for Animal Reproduction Medicine, Vetsuisse Faculty, University of Zürich, Switzerland;4. Swiss Institute of Equine Medicine, Agroscope and University of Berne, Avenches, Switzerland;1. Laboratory of Reproductive Technologies, Avantea, Cremona, Italy;2. Department of Veterinary Medical Sciences, University of Bologna, Italy;3. Fondazione Avantea, Cremona, Italy;1. Department of Veterinary Physiology and Pharmacology, College of Veterinary Medicine & Biomedical Sciences, Texas A&M University, College Station, Texas, USA;2. Laboratorio de Reproducción Equina Prof. Robert M. Kenney, Doña Pilar Embriones, Lincoln (B), Argentina;3. William H. Miner Agricultural Research Institute, Chazy, New York, USA;1. Dipartimento di Scienze Veterinarie, Università degli Studi di Pisa, Pisa, Italy;2. Private practitioner, Pisa, Italy;1. Universidad de Buenos Aires, Instituto de Investigación y Tecnología en Reproducción Animal, Facultad de Ciencias Veterinarias, Cátedra de Teriogenología, Ciudad Autónoma de Buenos Aires, Argentina;2. BET Labs/Biorelease Technologies LLC, Lexington, KY
Abstract:Many years of poor results of equine embryo cryopreservation has produced a lack of confidence in this technique. Embryo cryopreservation has been successfully used for more than 20 years in other species like bovine and human. The large size of the embryos and the presence of a capsule impermeable to cryoprotectants have been the two main reasons for the failure. In the last few years, a mayor breakthrough for this technique was obtained when large equine embryos could be successfully cryopreserved after breaching the capsule and collapsing the blastocoel cavity. In the present study, we compared the pregnancy rates obtained by vitrification or cryopreservation by slow freezing of embryos smaller than 300 μm. No difference was found between vitrification and slow freezing of embryos <180 μm (pregnancy rate on day 16: 34/61, 55.7%; 6/8, 75%) but produced very low results for embryos between 180 and 300 μm in diameter (0/11, 0%; 1/7, 14.3%). Embryos larger than 300 μm were collapsed before cryopreservation, and two different types of carriers, hemi-straw or Stripper-Tip, were used for vitrification. High pregnancy rates were obtained when the hemi-straw was used as a carrier (7/10, 70% vs. 0/5, 0%), demonstrating that a minimum vitrification volume was essential to preserve the embryo viability. These findings establish that, due to the large range in diameter, equine embryos need to be cryopreserved using different protocols depending on their size.
Keywords:Equine embryo  Vitrification  Slow freezing  Embryo force collapsed
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