Regional and developmental characteristics of human embryo mosaicism revealed by single cell sequencing

生物 胚泡 内细胞团 胚胎 胚胎干细胞 遗传学 非整倍体 胚胎发生 核型 嵌合体 一致性 男科 表型 基因 染色体 医学
作者
Yixuan Ren,Zhiqiang Yan,Ming Yang,Laura Keller,Xiaohui Zhu,Ying Lian,Qi Liu,Rong Li,Fan Zhai,Yanli Nie,Liying Yan,Gary D. Smith,Jie Qiao
出处
期刊:PLOS Genetics 卷期号:18 (8): e1010310-e1010310 被引量:7
标识
DOI:10.1371/journal.pgen.1010310
摘要

Chromosomal mosaicism is common throughout human pre- and post-implantation development. However, the incidence and characteristics of mosaicism in human blastocyst remain unclear. Concerns and confusions still exist regarding the interpretation of chromosomal mosaicism on preimplantation genetic testing for aneuploidy (PGT-A) results and embryo development. Here, we aimed to estimate the genetic concordance between trophectoderm (TE), inner cell mass (ICM) and the corresponding human embryonic stem cells (hESCs), and to explore the characteristics of mosaicism in human blastocyst and hESCs on a single cell level. The single cell sequencing results of TE cells indicated that 65.71% of the blastocysts were mosaic (23 in 35 embryos), while the ICM sequencing results suggested that 60.00% of the blastocysts were mosaic (9 in 15 embryos). The incidence of mosaicism for the corresponding hESCs was 33.33% (2 in 6 embryos). No significant difference was observed between the mosaic rate of TE and that of ICM. However, the mosaic rate of the corresponding hESCs was significantly lower than that of TE and ICM cells, suggesting that the incidence of mosaicism may decline during embryonic development. Upon single cell sequencing, we found several "complementary" copy number variations (CNVs) that were usually not revealed in clinical PGT-A which used multi-cell DNA sequencing (or array analysis). This indicates the potential diagnostic risk of PGT-A based multi-cell analysis routinely in clinical practice. This study provided new insights into the characteristics, and considerable influences, of mosaicism on human embryo development, as well as the clinical risks of PGT-A based on multi-cell biopsies and bulk DNA assays.
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