AI Article Synopsis

  • * Haploid embryonic stem cells (haESCs) can be created from uniparental blastocysts and have been used to replace sperm or oocyte genomes for generating mice.
  • * The study shows that deleting specific regions of DNA (IG-DMR and H19-DMR) from parthenogenetic haESCs allows the creation of fertile semi-cloned mice and highlights the issue of polyploidy in these embryos, which could impact further development.

Article Abstract

In mammals, the fusion of two gametes, an oocyte and a spermatozoon, during fertilization forms a totipotent zygote. There has been no reported case of adult mammal development by natural parthenogenesis, in which embryos develop from unfertilized oocytes. The genome and epigenetic information of haploid gametes are crucial for mammalian development. Haploid embryonic stem cells (haESCs) can be established from uniparental blastocysts and possess only one set of chromosomes. Previous studies have shown that sperm or oocyte genome can be replaced by haESCs with or without manipulation of genomic imprinting for generation of mice. Recently, these remarkable semi-cloning methods have been applied for screening of key factors of mouse embryonic development. While haESCs have been applied as substitutes of gametic genomes, the fundamental mechanism how haESCs contribute to the genome of totipotent embryos is unclear. Here, we show the generation of fertile semi-cloned mice by injection of parthenogenetic haESCs (phaESCs) into oocytes after deletion of two differentially methylated regions (DMRs), the IG-DMR and H19-DMR. For characterizing the genome of semi-cloned embryos further, we establish ESC lines from semi-cloned blastocysts. We report that polyploid karyotypes are observed in semi-cloned ESCs (scESCs). Our results confirm that mitotically arrested phaESCs yield semi-cloned embryos and mice when the IG-DMR and H19-DMR are deleted. In addition, we highlight the occurrence of polyploidy that needs to be considered for further improving the development of semi-cloned embryos derived by haESC injection.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC7482839PMC
http://journals.plos.org/plosone/article?id=10.1371/journal.pone.0233072PLOS

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