| Literature DB >> 28854370 |
Zheng-Quan He1, Bao-Long Xia2, Yu-Kai Wang2, Jing Li3, Gui-Hai Feng1, Lin-Lin Zhang1, Yu-Huan Li1, Hai-Feng Wan2, Tian-Da Li2, Kai Xu1, Xue-Wei Yuan4, Yu-Fei Li1, Xin-Xin Zhang4, Ying Zhang2, Liu Wang1, Wei Li1, Qi Zhou5.
Abstract
The recent success of derivation of mammalian haploid embryonic stem cells (haESCs) has provided a powerful tool for large-scale functional analysis of the mammalian genome. However, haESCs rapidly become diploidized after differentiation, posing challenges for genetic analysis. Here, we show that the spontaneous diploidization of haESCs happens in metaphase due to mitotic slippage. Diploidization can be suppressed by small-molecule-mediated inhibition of CDK1 and ROCK. Through ROCK inhibition, we can generate haploid somatic cells of all three germ layers from haESCs, including terminally differentiated neurons. Using piggyBac transposon-based insertional mutagenesis, we generated a haploid neural cell library harboring genome-wide mutations for genetic screening. As a proof of concept, we screened for Mn2+-mediated toxicity and identified the Park2 gene. Our findings expand the applications of mouse haploid cell technology to somatic cell types and may also shed light on the mechanisms of ploidy maintenance.Entities:
Keywords: genetic screening; genome-wide; haploid cells; haploidy; stem cells
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Year: 2017 PMID: 28854370 DOI: 10.1016/j.celrep.2017.07.081
Source DB: PubMed Journal: Cell Rep Impact factor: 9.423