Different pre-implantation phenotypes of bovine blastocysts produced in vitro

Author:

Hue Isabelle1,Dufort Isabelle2,Vitorino Carvalho Anaïs13,Laloe Denis4,Peynot Nathalie1,Degrelle Séverine Aude567,Viebahn Christoph8,Sirard Marc-André2

Affiliation:

1. 1UMR BDR, INRA, ENVA, Université Paris Saclay, Jouy en Josas, France

2. 2Centre de Recherche en Biologie de la Reproduction, Département des Sciences Animales, Faculté des Sciences de l’Agriculture et de l’Alimentation, Université Laval, Quebec City, Québec, Canada

3. 3UMR PRC, INRA, CNRS, IFCE, Université de Tours, Nouzilly, France

4. 4UMR GABI, INRA, Université Paris Saclay, Jouy en Josas, France

5. 5INSERM, UMR-S1139, Faculté de Pharmacie de Paris, Paris, France

6. 6Université Paris Descartes, Sorbonne Paris Cité, Paris, France

7. 7Inovarion, Paris, France

8. 8Institute of Anatomy and Embryology, University Medical Centre Göttingen, Göttingen, Germany

Abstract

Embryo transfer in cattle is performed with blastocysts produced in vivo or in vitro using defined media. However, outdated systems such as those that use serum and co-culture remain of interest for research purposes. Here, we investigated the effect of additional culture time on in vitro-produced embryos. Specifically, we compared embryos that formed a blastocoel at different times after fertilisation to those that stayed in culture for up to two additional days with respect to their development in vivo after temporary transfer to oestrus-synchronised recipients. A pre-transfer set (D6, D6+1, D6+2, D7, D7+1, D8) was examined using microarray analyses and correlated with a post-transfer set that included two different days of transfer (D6-T6, D6+2-T8, D7+1-T8, D8-T8). All surviving conceptuses reached primitive-streak stages and filamentous sizes similarly to in vivo (D18) or in vitro controls (D7/T7). The recovery rate differed between D6 and D8 embryos that were immediately transferred (58 vs 25%). With an intermediate survival rate (33%), the D6 embryos with two additional days in culture produced nine times more IFN-tau (IFNT) at D18 than the D6 embryos that were immediately transferred. At the end of culture, D6 and D6+2 embryos displayed the highest number of gene expression differences. Despite a mortality of 40–60%, no signature was detectable in any of the transferred groups that would account for the embryos’ fates. Initially reputed to be beneficial in producing more blastocysts, our culture system of B2 medium plus serum and co-culture generated blastocysts that were distinct from those developed in vivo (D7).

Publisher

Bioscientifica

Subject

Cell Biology,Obstetrics and Gynaecology,Endocrinology,Embryology,Reproductive Medicine

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