Efficient generation of Knock-in/Knock-out marmoset embryo via CRISPR/Cas9 gene editing

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作者
Wakako Kumita
Kenya Sato
Yasuhiro Suzuki
Yoko Kurotaki
Takeshi Harada
Yang Zhou
Noriyuki Kishi
Kengo Sato
Atsu Aiba
Yasubumi Sakakibara
Guoping Feng
Hideyuki Okano
Erika Sasaki
机构
[1] Central Institute for Experimental Animals,Department of Molecular Biology and Biochemistry, Graduate School of Medicine
[2] Osaka University,Laboratory of Animal Resources, Center for Disease Biology and Integrative Medicine, Graduate School of Medicine
[3] The University of Tokyo,McGovern Institute for Brain Research, Department of Brain and Cognitive Sciences
[4] Massachusetts Institute of Technology,Laboratory for Marmoset Neural Architecture
[5] RIKEN Center for Brain Science,Department of Biosciences and Informatics
[6] Keio University,Department of Physiology
[7] Keio University School of Medicine,Advanced Research Center
[8] Keio University,undefined
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摘要
Genetically modified nonhuman primates (NHP) are useful models for biomedical research. Gene editing technologies have enabled production of target-gene knock-out (KO) NHP models. Target-gene-KO/knock-in (KI) efficiency of CRISPR/Cas9 has not been extensively investigated in marmosets. In this study, optimum conditions for target gene modification efficacies of CRISPR/mRNA and CRISPR/nuclease in marmoset embryos were examined. CRISPR/nuclease was more effective than CRISPR/mRNA in avoiding mosaic genetic alteration. Furthermore, optimal conditions to generate KI marmoset embryos were investigated using CRISPR/Cas9 and 2 different lengths (36 nt and 100 nt) each of a sense or anti-sense single-strand oligonucleotide (ssODN). KIs were observed when CRISPR/nuclease and 36 nt sense or anti-sense ssODNs were injected into embryos. All embryos exhibited mosaic mutations with KI and KO, or imprecise KI, of c-kit. Although further improvement of KI strategies is required, these results indicated that CRISPR/Cas9 may be utilized to produce KO/KI marmosets via gene editing.
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