| Literature DB >> 29886029 |
Jing Luo1, Liaoxun Lu2, Yanrong Gu1, Rong Huang1, Lin Gui1, Saichao Li1, Xinhui Qi1, Wenping Zheng1, Tianzhu Chao3, Qianqian Zheng1, Yinming Liang4, Lichen Zhang5.
Abstract
Genetic engineering of cell lines and model organisms has been facilitated enormously by the CRISPR/Cas9 system. However, in cell lines it remains labor intensive and time consuming to obtain desirable mutant clones due to the difficulties in isolating the mutated clones and sophisticated genotyping. In this study, we have validated fluorescent protein reporter aided cell sorting which enables the isolation of maximal diversity in mutant cells. We further applied two spectrally distinct fluorescent proteins DsRed2 and ECFP as reporters for independent CRISPR/Cas9 mediated targeting, which allows for one-cell-one-well sorting of the mutant cells. Because of ultra-high efficiency of the CRISPR/Cas9 system with dual reporters and large DNA fragment deletion resulting from independent loci cleavage, monoclonal mutant cells could be easily identified by conventional PCR. In the speed genome editing method presented here, sophisticated genotyping methods are not necessary to identify loss of function mutations after CRISPR/Cas9 genome editing, and desirable loss of function mutant clones could be obtained in less than one month following transfection.Entities:
Keywords: CRISPR/Cas9; Fluorescent reporter; Large DNA fragment deletion; Single cell sorting; Speed genome editing
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Year: 2018 PMID: 29886029 DOI: 10.1016/j.jbiotec.2018.06.308
Source DB: PubMed Journal: J Biotechnol ISSN: 0168-1656 Impact factor: 3.307