改造CRISPR-Cas12b系统用于哺乳动物基因组编辑

实验样品均来自于人类胚胎肾细胞系(HEK293)和小鼠胚胎干细胞(mES)，瞬时转染不同的Cas12b和靶向gRNA质粒，用于分析Cas12b系统的编辑效率和脱靶效应。

All experimental samples were derived from human embryonic kidney cell line (HEK293) and mouse embryonic stem cells (mES), and were transiently transfected with different Cas12b and targeting gRNA plasmids to analyze the editing efficiency and off-target effects of the Cas12b system.