F. Berthelot scite author profile

Morphological and molecular signs of injury and cell death and subsequent regeneration following vitrification of porcine blastocysts were evaluated by light (LM) and transmission electron microscopy (TEM) as well as TUNEL/propidium iodide (PI) nuclear staining followed by confocal microscopy (CSM). In vivo derived blastocysts were assigned to one of the following four groups: Controls-(1) fixed immediately after collection (C0h) and (2) after 24 hr culture in vitro (C24h) and vitrified embryos-(3) fixed immediately after vitrification and warming (V0h), and (4) after 24 hr of culture upon warming after vitrification (V24h). Observation by LM and TEM showed that the V0h embryos displayed collapse of the blastocoele cavity (BC) and cell swelling, a general distension or shrinkage of mitochondria and massive increase in the amount of vesicles, vacuoles, and secondary lysosomes (SLs). Approximately 2/3 of the V24h embryos had recovered, whereas the remaining 1/3 were degenerated. Recovered embryos displayed almost normal blastocyst morphology, except for a widening of the perivitelline space, accumulation of debris and partial distension of mitochondria, whereas degenerated embryos were disintegrated into a poorly defined mass of cells and debris including cells with abundant degeneration of mitochondria and other organelles. Both recovered and degenerated embryos displayed a persistent abundance of presence of small membrane bounded vesicles, vacuoles, and SLs. Evaluation of TUNEL/PI stained embryos showed only occasional appearance of TUNEL positive nuclei with typical apoptotic morphology in controls (C0h 0.67%, C24h 1.22%) and in the V0h embryos (0.93%). The percentage of apoptotic nuclei in embryos at V24h was significantly higher than in all other groups (2.64%). Vitrified embryos showed significantly increased appearance of DNA fragmented nuclei without typical morphological features of apoptosis (V0h 1.43%, V24h 4.30%) compared with controls (C0h 0.26%, C24h 0.45%). The observed morphological changes and increased DNA fragmentation observed immediately after vitrification and warming probably reflects a direct damaging effect of vitrification. During 24 hr of culture a portion of the embryos was able to regenerate and along with the regenerative process, apoptosis--a possible pathway for elimination of damaged cells--became evident.

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Birth of piglets after OPS vitrification and transfer of compacted morula stage embryos with intact zona pellucida

Berthelot

Martinat-Botté

Perreau

et al. 2001

Reprod. Nutr. Dev.

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-In swine, five to six days post-insemination, morulae and blastocysts are collected together after uterine flushing. The purpose of this study was to vitrify zona pellucida-intact morulae with Open Pulled Straw (OPS) technology and obtain piglets after transfer. Morulae (200) were vitrified after a two-step equilibration in ethylene glycol, dimethyl sulfoxide and sucrose in Hepesbuffered TCM199 + 20% NBCS medium (TCM). 2-6 morulae were loaded into OPS and plunged into liquid nitrogen. At embryo warming, a three-step dilution with decreasing concentrations of sucrose was applied. In each of 10 recipients, 20 morulae were transferred surgically. Day 25, gestation rate and the farrowing rate were 80% and 70%, respectively. The pregnant recipients farrowed from 1 to 8 piglets and the survival of total transferred embryos was 13%. Although survival rates are still compromised, OPS technology is therefore appropriate to cryopreserve porcine morulae with intact zona pellucida. pig / embryo / morula / OPS vitrification / cryopreservationRésumé -Naissance de porcelets après transfert de morulae dans la zone pellucide intacte et vitrification par la méthode OPS. Chez la truie, 5 à 6 jours après l'insémination, il est récolté des embryons aux stades morula et blastocyste associés. Le but de ce travail est de transférer des morulae vitrifiées et d'obtenir des porcelets. Des morulae (200) sont vitrifiées par la méthode OPS après 2 étapes d'équilibration dans un mélange égal d'éthylène glycol, de DMSO et de sucrose dilués dans du TCM199 Hépès + 20 % de sérum de veau nouveau-né (TCM). Pour le réchauffement, les paillettes sont sorties de l'azote et plongées immédiatement dans du TCM + sucrose, l'élimination des cryoprotecteurs se faisant en 3 étapes. Pour évaluer la viabilité des morulae vitrifiées/réchauffées, 10 receveuses reçoivent chacune 20 morulae après transfert chirurgical. Le pourcentage de mises-bas Reprod. Nutr. Dev. 41 (2001) 267-272 267

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F. Berthelot

Piglets Born after Vitrification of Embryos Using the Open Pulled Straw Method

Piglets born after non-surgical deep intrauterine transfer of vitrified blastocysts in gilts

Ultrastructure and cell death of in vivo derived and vitrified porcine blastocysts

Birth of piglets after OPS vitrification and transfer of compacted morula stage embryos with intact zona pellucida

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