Distinct Post-Insemination Dynamics Between Fresh and Frozen-Derived Gametes Using Testicular Sperm - Beyond the Abstract
A total of 980 metaphase-II oocytes were inseminated using either fresh or frozen-thawed TESE sperm, with embryos cultured in time-lapse incubators and analyzed for preimplantation genetic testing for aneuploidy (PGT-A) by next-generation sequencing (NGS). Fertilization and blastulation rates per inseminated oocyte were significantly lower when frozen sperm were used, though euploidy rates per biopsied blastocyst were comparable between groups.
Time-lapse morphokinetic analyses revealed distinct post-fertilization dynamics. Embryos from frozen-TESE sperm exhibited a prolonged pronuclear (2PN) phase, with a mean delay of 2.1 hours (P = 0.008), suggesting potential nuclear repair mechanisms or cryo-induced DNA damage responses. Similar prolongation was observed in embryos from vitrified oocytes. Beyond this early lag, embryos fertilized with frozen testicular sperm progressed to the 6-cell stage more quickly but required slightly more time to reach full blastocyst expansion than embryos generated with fresh sperm.
These findings emphasize that synchronizing fresh-TESE with oocyte retrieval, when clinically feasible, optimizes fertilization outcomes without compromising euploidy. Cryopreserved TESE remains a viable option but may introduce subtle developmental delays that warrant further study. The observed 2PN lag could represent a novel morphokinetic biomarker reflecting gamete integrity after freezing.
Overall, this intra-patient controlled study provides critical insights into how cryopreservation of testicular sperm affects early embryonic events, guiding clinical decision-making for TESE timing and cryostorage strategies in severe male infertility.
Written by: Daniela Nogueira, MD, IVF Department, ART Fertility Clinics, Abu Dhabi, UAE; INOVIE Fertilité, Toulouse, France
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