AI Article Synopsis

  • * The study examines mitochondrial function's role in embryo development, showing that euploid embryos increased and mosaic embryos decreased during culture, alongside a lower number of mitochondrial DNA mutations in euploid embryos.
  • * Findings indicate that aneuploidy might reduce in embryos after implantation, and assessing mtDNA mutations could be a new strategy for selecting viable mosaic embryos for transfer.

Article Abstract

Several healthy euploid births have been reported following the transfer of mosaic embryos, including both euploid and aneuploid blastomeres. This has been attributed to a reduced number of aneuploid cells, as previously reported in mice, but remains poorly explored in humans. We hypothesized that mitochondrial function, one of the most critical factors for embryonic development, can influence human post-implantation embryonic development, including a decrease of aneuploid cells in mosaic embryos. To clarify the role of mitochondrial function, we biopsied multiple parts of each human embryo and observed the remaining embryos under culture as a model of post-implantation development ( = 27 embryos). Karyotyping, whole mitochondrial DNA (mtDNA) sequencing, and mtDNA copy number assays were performed on all pre- and post-culture samples. The ratio of euploid embryos was significantly enhanced during culture, whereas the ratio of mosaic embryos was significantly reduced. Furthermore, post-culture euploid and culturable embryos had significantly few mtDNA mutations, although mtDNA copy numbers did not differ. Our results indicate that aneuploid cells decrease in human embryos post-implantation, and mtDNA mutations might induce low mitochondrial function and influence the development of post-implantation embryos with not only aneuploidy but also euploidy. Analyzing the whole mtDNA mutation number may be a novel method for selecting a better mosaic embryo for transfer.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC10451077PMC
http://dx.doi.org/10.3389/fcell.2023.1215626DOI Listing

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