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Culture time to optimize embryo cell-free DNA analysis for frozen-thawed blastocysts undergoing noninvasive preimplantation genetic testing for aneuploidy.
Ardestani, Goli; Banti, Maria; García-Pascual, Carmen M; Navarro-Sánchez, Luis; Van Zyl, Estee; Castellón, Jose Antonio; Simón, Carlos; Sakkas, Denny; Rubio, Carmen.
Afiliación
  • Ardestani G; Boston IVF - IVIRMA Global Research Alliance, Waltham, Massachusetts. Electronic address: gardestani@bostonivf.com.
  • Banti M; Orchid Reproductive and Andrology Services, Dubai Healthcare, City, Dubai, United Arab Emirates.
  • García-Pascual CM; R&D Department, Igenomix, Paterna, Valencia, Spain.
  • Navarro-Sánchez L; R&D Department, Igenomix, Paterna, Valencia, Spain.
  • Van Zyl E; Orchid Reproductive and Andrology Services, Dubai Healthcare, City, Dubai, United Arab Emirates.
  • Castellón JA; R&D Department, Igenomix, Paterna, Valencia, Spain.
  • Simón C; Department of Obstetrics and Gynecology, University of Valencia, Spain; BIDMC Harvard University, Boston, Massachusetts; Carlos Simon Foundation, INCLIVA, Valencia, Spain.
  • Sakkas D; Boston IVF - IVIRMA Global Research Alliance, Waltham, Massachusetts.
  • Rubio C; R&D Department, Igenomix, Paterna, Valencia, Spain.
Fertil Steril ; 2024 May 07.
Article en En | MEDLINE | ID: mdl-38718960
ABSTRACT

OBJECTIVE:

To investigate the ideal time in culture to optimize embryo cell-free deoxyribonucleic acid (cfDNA) analysis in frozen-thawed blastocysts undergoing noninvasive preimplantation genetic testing for aneuploidy (PGT-A). Cell-free DNA is released into the spent blastocyst media (spent media) by the embryo. However, the optimal timing to determine maximal cfDNA in the case of frozen-thawed blastocysts undergoing noninvasive PGT-A remains to be elucidated.

DESIGN:

In this prospective observational study, 135 spent media and corresponding whole blastocysts were collected from January 2021 through March 2022.

SETTING:

Private fertility clinics. PATIENTS Day-5 frozen-thawed blastocysts were cultured for 8 hours (Day-5 Short) or 24 hours (Day-5 Long), whereas day-6 frozen-thawed blastocysts were cultured for 8 hours (Day-6 Short). The spent media and whole blastocysts were then collected for further analysis. Spent media and whole blastocysts were amplified using whole genome amplification and sequenced using next-generation sequencing. MAIN OUTCOME

MEASURES:

Informativity and concordance rates between cfDNA in spent media and whole blastocyst DNA were compared according to the different times in culture.

RESULTS:

When comparing time in culture, informativity rates for spent media were significantly higher for Day-5 Long and Day-6 Short (>91%) compared with the Day-5 Short group (<60%). A similar trend was observed for cases with and without a previous PGT-A. Regarding blastocyst expansion grade, informativity rates were lower on Day-5 Short compared with Day-5 Long and Day-6 Short, regardless of expansion degree. This decrease was significant for Gardner-grade expansion grades 3, 4, and 5-6. In addition, for a similar time in culture, the grade of expansion did not have an impact on the informativity rates. For concordance rates, no significant differences were observed among the 3 groups. In all cases, concordance rates were 90.5% for Day-5 Short, 93.6% for Day-5 Long, and 92.3% for Day-6 Short. No impact of the expansion grade was observed on concordance rates.

CONCLUSION:

Noninvasive PGT-A in frozen-thawed blastocysts yields very high concordance rates with whole blastocysts, possibly limiting the need for invasive PGT-A and making it available for a wider range of patients.
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Texto completo: 1 Base de datos: MEDLINE Idioma: En Revista: Fertil Steril Año: 2024 Tipo del documento: Article

Texto completo: 1 Base de datos: MEDLINE Idioma: En Revista: Fertil Steril Año: 2024 Tipo del documento: Article