| Literature DB >> 30970262 |
Robert J Ihry1, Max R Salick2, Daniel J Ho3, Marie Sondey4, Sravya Kommineni5, Steven Paula6, Joe Raymond3, Beata Henry3, Elizabeth Frias6, Qiong Wang6, Kathleen A Worringer3, Chaoyang Ye7, Carsten Russ6, John S Reece-Hoyes6, Robert C Altshuler3, Ranjit Randhawa8, Zinger Yang9, Gregory McAllister10, Gregory R Hoffman10, Ricardo Dolmetsch3, Ajamete Kaykas11.
Abstract
Human pluripotent stem cells (hPSCs) generate a variety of disease-relevant cells that can be used to improve the translation of preclinical research. Despite the potential of hPSCs, their use for genetic screening has been limited by technical challenges. We developed a scalable and renewable Cas9 and sgRNA-hPSC library in which loss-of-function mutations can be induced at will. Our inducible mutant hPSC library can be used for multiple genome-wide CRISPR screens in a variety of hPSC-induced cell types. As proof of concept, we performed three screens for regulators of properties fundamental to hPSCs: their ability to self-renew and/or survive (fitness), their inability to survive as single-cell clones, and their capacity to differentiate. We identified the majority of known genes and pathways involved in these processes, as well as a plethora of genes with unidentified roles. This resource will increase the understanding of human development and genetics. This approach will be a powerful tool to identify disease-modifying genes and pathways.Entities:
Keywords: CRISPR genome-wide screening; DDR; PAWR; PMAIP1; hESC; human pluripotent stem cells; iPSC
Mesh:
Year: 2019 PMID: 30970262 DOI: 10.1016/j.celrep.2019.03.043
Source DB: PubMed Journal: Cell Rep Impact factor: 9.423