%0 Journal Article
%T Cpf1 和 Cas9核酸酶靶向EGFR-L858R突变的研究<br>Targeting EGFR-L858R mutation by Cpf1 and Cas9 nuclease
%A 魏恒
%A 杨梅佳
%A 钟坤宏
%A 仝爱平
%J 四川大学学报 (自然科学版)
%D 2018
%X EGFR的突变是造成非小细胞肺癌的原因之一。EGFR第19个外显子的缺失和L858R (2573T>G)单核苷酸突变占所有EGFR突变的90%。选择性地使突变EGFR失活对这类突变的病人是非常有利的。这里，应用双荧光报告分析的方法分析CRISPR-Cpf1和CRISPR-Cas9系统在靶向EGFR-L858R突变的编辑效率。在EGFR-L858R突变位点的附近，有两个Cpf1前间区序列邻近基序（PAMs）――TTTN。并且，EGFR的2573T>G突变形成了一个Cas9的PAM――NGG。因此本文通过构建两条AsCpf1的gRNAs (gRNA1和gRNA2)和一条SpCas9的 gRNA (gRNA3) 在体外通过双荧光蛋白分析系统去评估SpCas9和 AsCpf1特异性靶向等位基因的能力。结果证实了AsCpf1和SpCas9 都能够特异性的编辑突变的EGFR（2573T>G）。实验结果显示Cpf1和Cas9 能够通过高特异性破坏突变癌基因，从而具有潜在的精准治疗价值。<br>Mutations in the EGFR kinase are a cause of non-small-cell lung cancer. Deletions in exon 19 and the L858R (2573T>G) single point mutation constitute about 90% of all EGFR mutations. Selectively inactivate only mutant, not normal allele, could benefit patients with such mutations. Here, the editing efficacy and selectivity of CRISPR-Cpf1 and -Cas9 systems on EGFR L858R mutant allele were analyzed by dual-reporter assay in vitro. Near the mutation site, there are two TTTN protospacer adjacent motifs (PAMs) for Cpf1. 2573T>G substitution also leads to occurrence of a novel NGG PAM for Cas9. Thus we designed two AsCpf1 gRNA (gRNA1 and gRNA2) and one SpCas9 gRNA (gRNA3) and evaluated their potency and allele specificity in vitro using a dual fluorescent protein-based bioassay system. As a result, both AsCpf1 and SpCas9 demonstrated robust activities to induce specific editing of only 2573T>G mutant EGFR, not wild-type sequence. Our results support the potential applicability of both Cpf1 and Cas9 in precision medicine through highly specific disruption of mutant oncogenes
%K CRISPR Cas9 CRISPR Cpf1 EGFR L858R 靶向治疗&lt
%K br&gt
%K CRISPR Cas9 CRISPR Cpf1 EGFR L858R Targeted therapy
%U http://science.ijournals.cn/jsunature_cn/ch/reader/view_abstract.aspx?file_no=B170156&flag=1