The effect of male factors on embryo morphokinetics: a retrospective analysis of 2726 blastocysts.

Fecha de publicación: 07/10/2024 Fecha Ahead of Print: 07/10/2024

Autores de IIS La Fe

Irene Hervás Herrero

Autor
Daniela Galliano

Autor
Mauro Cozzolino

Autor

Participantes ajenos a IIS La Fe

Pellegrini, Livia
Gatti, Simona
Navarro, Nuria
Marcos, Meseguer
Viviana, Vasquez
Toschi, Marco

Grupos

Biología Reproductiva y Bioingeniería en Reproducción Humana

Leader

Nicolás Garrido Puchalt
Endocrinología Reproductiva e Infertilidad

Leader

José Remohí Giménez

Abstract

PURPOSE: Male infertility may influence fertilization rates, embryo morphology, and implantation rates in in vitro fertilization (IVF) cycles. Oocyte competence plays a major role in embryo development, but there is a limited understanding of the connection between sperm quality, embryo development, and morphokinetic parameters using donor oocytes. The study evaluated if sperm quality may influence the morphokinetic parameters in IVF cycles. METHODS: A retrospective multicentric observational cohort study included 747 ICSI cycles using donor oocytes with fresh or frozen sperm. Embryos were cultured in time-lapse incubators until the blastocyst stage. The population was divided into three groups according to sperm concentration, as control group (>16 mill/mL), severe oligospermia (0-5 mill/mL), and moderate oligospermia group (5-16 mill/mL). RESULTS: Morphokinetic analysis showed no difference in the time from the 2-cell to 6-cell stage of embryo development. A significant difference was observed on day 3 of embryo development, specifically at the 7-cell stage (t7), severe oligospermia 53.37±9.81, moderate oligospermia 56.95±9.78, and control 55.1±8.85h post-insemination (hpi) (p=0.024), and 8-cell stage (t8), severe oligospermia 55.41±10.83, moderate oligospermia 61.86±12.38 hpi (p<0.001), and control 58.61±11.33. Accordingly, the synchrony of the four cleavages going from 4 to 8 cells (s3) was found statistically different among the groups in the severe oligospermia 8.05±9.99, moderate oligospermia 11.66±11.04 hpi, and control 8.55±8.58 (p=0.009). Morphokinetic time ranges were obtained for t6, t7, t8, and s3 in order to identify the good-quality blastocysts. CONCLUSIONS: Poor sperm quality is associated with alterations in morphokinetic parameters on day 3 in IVF cycles with donor oocytes, underlining the important role of spermatozoa during embryo development.