Effect of oocyte vitrification on embryo quality: time-lapse analysis and morphokinetic evaluation

Ana Cobo; Aila Coello; Jose Remohí; Jose Serrano; Jose Maria de Los Santos; Marcos Meseguer

doi:10.1016/j.fertnstert.2017.06.024

Effect of oocyte vitrification on embryo quality: time-lapse analysis and morphokinetic evaluation

Fertil Steril. 2017 Sep;108(3):491-497.e3. doi: 10.1016/j.fertnstert.2017.06.024.

Authors

Ana Cobo¹, Aila Coello², Jose Remohí², Jose Serrano², Jose Maria de Los Santos², Marcos Meseguer²

Affiliations

¹ Instituto Valenciano de Infertilidad Valencia, INCLIVA-University of Valencia, Valencia, Spain. Electronic address: ana.cobo@ivi.es.
² Instituto Valenciano de Infertilidad Valencia, INCLIVA-University of Valencia, Valencia, Spain.

PMID: 28865549
DOI: 10.1016/j.fertnstert.2017.06.024

Abstract

Objective: To analyze whether oocyte vitrification may affect subsequent embryo development from a morphokinetic standpoint by means of time-lapse imaging.

Design: Observational cohort study.

Setting: University-affiliated private IVF center.

Patient(s): Ovum donation cycles conducted with the use of vitrified (n = 631 cycles; n = 3,794 embryos) or fresh oocytes (n = 1,359 cycles; n = 9,935 embryos) over 2 years.

Interventions(s): None.

Main outcome measure(s): Embryo development was analyzed in a time-lapse imaging incubator. The studied variables included time to 2 cells (t2), 3 cells (t3), 4 cells (t4), 5 cells (t5), morula (tM), and cavitated, early, and hatching blastocyst (tB, tEB, tHB) as well as 2nd cell cycle duration (cc2 = t3 - t2). All of the embryos were classified according to the hierarchic tree model currently used for embryo selection. The analyzed variables were compared with the use of analysis of variance or chi-square and included 95% confidence intervals (CIs).

Result(s): The embryos that originated from vitrified oocytes showed a delay of ∼1 hour from the first division to 2 cells (t2) to the time of blastulation (tB). The embryos that originated from vitrified oocytes showed a delay of ∼1 hour from the 1st division to 2 cells (t2) to the time of blastulation (tB) (P<.05). The proportions of embryos allocated to categories A-E in the hierarchical tree were similar between groups. No differences in implantation rates between the fresh (51.3% [95% CI 47.1%-55.7%]) and vitrified (46.4% [95% CI 38.4%-54.4%]) groups were found.

Conclusion(s): The embryo quality of vitrified oocytes was not impaired: cc2, quality according to our hierarchic morphokinetic model, and implantation rates were similar between fresh and vitrified oocytes. However, morphokinetic differences were observed from t2 to tB. Our main study limitation was the retrospective nature of the analysis, although a large database was studied.

Keywords: Vitrification; embryo; morphokinetics; oocyte; time-lapse.

Publication types

Observational Study
Research Support, Non-U.S. Gov't

MeSH terms

Cells, Cultured
Cohort Studies
Cryopreservation / methods*
Embryo Implantation / physiology*
Embryo, Mammalian / cytology*
Embryo, Mammalian / physiology
Embryonic Development / physiology*
Female
Humans
Image Interpretation, Computer-Assisted / methods
Oocytes / cytology*
Time-Lapse Imaging / methods*