基于CRISPR-Cas9定向编辑TRAC基因的研究  

作　　者：徐畅[1] 覃启富 向静[1] 瞿创 张丹[1] 徐鹏程[1] 张文峰[1] 沈晗[1] 邵红伟[1] 

机构地区：[1]广东药科大学生命科学与生物制药学院/广东省生物技术候选药物研究重点实验室,广东广州510006

出　　处：《广东药科大学学报》2017年第2期255-261,共7页Journal of Guangdong Pharmaceutical University

基　　金：国家自然科学基金项目(31100664;31300737;81303292);广东省自然科学基金项目(10151022401000024;2014A030313586);广东省科技计划项目(2016A020215157)

摘　　要：目的针对人源TCRαC基因(TRAC)进行CRISPR/Cas9-gRNA的设计,并验证设计的gRNA的有效性及其脱靶率。方法利用CRISPR网站(http://crispr.mit.edu/)提供的靶向编辑位点筛选工具,针对TCRαC区各设计出了3个编辑位点,并据此构建CRISPR-Cas9-TCR敲除质粒,将构建好的质粒转染293T细胞系,通过流式细胞术结合PCR产物的T-A克隆测序等方法验证各个gRNA序列的编辑效率。再根据所预测的潜在脱靶位点,设计相应的上下游引物进行PCR扩增后测序,检测其是否出现脱靶。结果在3组针对TCRαC区的gRNA中,site2-gRNA的编辑效率最高,并且无脱靶现象。结论针对人源TCRαC基因设计的site2-gRNA对TCRαC区具有很好的编辑效果,且无脱靶现象,为消除杂合TCR分子的产生和改善TCR修饰的T细胞(TCR-T)过继性免疫治疗奠定了基础。Objective To design a CRISPR/Cas9-gRNA targeting human TCR alpha gene, and evaluate the editing effectiveness and the off-target loci of the gRNA candidates. Methods 3 spacer sequences of gRNA targeting TCR alpha C gene were designed with a CRISPR website （ http：//crispr.mit.edu/）, and CRISPR- Cas9-TCR editing plasmids were respectively constructed based on pX458 plasmid. The recombinant plasmids were separately transfected into 293T cells. After three days of transfection the genomic DNA were extracted, and the fragments containing editing sites were amplified by PCR and subject to T-A cloning and sequencing to evaluate the editing efficiency of each gRNA. To investigate whether there is off-target cleavage mediated by gRNA, the DNA fragments containing the potential off-target sites predicted by online tools were amplified by PCR and subject to sequencing analysis. Results In three candidate gRNAs targeting TCR alpha C region, the site2-gRNA displayed the highest editing efficiency, and no off-target cleavage was found. Conclusion The site2-gRNA targeting human TCR alpha C gene shows good editing efficiency without off-target cleavage, which provides an important basis for eliminating the production of hybrid TCR in TCR gene-modified T cell （TCR-T） and improving the therapeutic effect of TCR-T.

关 键 词：CRISPR 引导RNA TRAC基因 基因组编辑 脱靶 

分 类 号：Q78[生物学—分子生物学] R457.2[医药卫生—治疗学]