Validation Study to Determine the Accuracy of Widespread Promoterless EGFP Reporter at Assessing CRISPR/Cas9-Mediated Homology Directed Repair |
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| Authors: | Wanqing Xu Qingxia Zuo Dongyan Feng Changsheng He Cailing Lin Dongchao Huang Yanbin Wan Feng Chen Guosheng Mo Qi Sun Hongli Du Lizhen Huang |
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| Institution: | School of Biology and Biological Engineering, South China University of Technology, Guangzhou 510006, China; (W.X.); (Q.Z.); (D.F.); (C.H.); (C.L.); (D.H.); (Y.W.); (F.C.); (G.M.); (Q.S.); (H.D.) |
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| Abstract: | An accurate visual reporter system to assess homology-directed repair (HDR) is a key prerequisite for evaluating the efficiency of Cas9-mediated precise gene editing. Herein, we tested the utility of the widespread promoterless EGFP reporter to assess the efficiency of CRISPR/Cas9-mediated homologous recombination by fluorescence expression. We firstly established a promoterless EGFP reporter donor targeting the porcine GAPDH locus to study CRISPR/Cas9-mediated homologous recombination in porcine cells. Curiously, EGFP was expressed at unexpectedly high levels from the promoterless donor in porcine cells, with or without Cas9/sgRNA. Even higher EGFP expression was detected in human cells and those of other species when the porcine donor was transfected alone. Therefore, EGFP could be expressed at certain level in various cells transfected with the promoterless EGFP reporter alone, making it a low-resolution reporter for measuring Cas9-mediated HDR events. In summary, the widespread promoterless EGFP reporter could not be an ideal measurement for HDR screening and there is an urgent need to develop a more reliable, high-resolution HDR screening system to better explore strategies of increasing the efficiency of Cas9-mediated HDR in mammalian cells. |
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| Keywords: | CRISPR/Cas9 homology-directed repair precise gene editing random integration promoterless EGFP reporter |
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