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The precise magic of CRISPR

机译:CRISPR的精确魔力

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In this issue of FEBS Open Bio , Shen Li et al. , in the laboratory of Hector L. Franco (University of North Carolina), provide a proof-of-principle solution for correcting all copies of a gene in the widely used MCF7 breast cancer cell line. The gene for the FOXA1 pioneer transcription factor is localised on chromosome 14, which is present at least 4–5 times in MCF7 cells. To achieve their goal, the authors used a ‘classical’ version of the CRISPR/Cas9 system. Both sgRNA and Cas9 components were expressed from a single vector, which also has a puromycin resistance cassette; this is an essential module for the chosen strategy, because it ensures expression of both sgRNA and Cas9 in selected cells. A targeting template in the form of nonlinearised plasmid was shown to have the best efficiency and was used to introduce a substitution at position 295 in the gene encoding FOXA1 to change a codon encoding lysine into a codon encoding glutamine (K295Q). The strategy suggested by Li and co-authors is an important development towards genome editing of multiple copy genes in a polyploid environment like cancer cells. One important application of the technique could be in creating models to study the role of single nucleotide polymorphisms in cancer progression and metastasis. Isogenic cancer lines carrying polymorphic variants of key drug targets could be used to optimise anticancer treatment protocols, laying a foundation for personalised therapy.
机译:在本期FEBS Open Bio中,Hector L. Franco(北卡罗来纳大学)实验室的Shen Li等人提供了一种原理验证解决方案,用于纠正广泛使用的MCF7乳腺癌细胞系中基因的所有拷贝。FOXA1 先驱转录因子的基因位于 14 号染色体上,该染色体在 MCF7 细胞中至少存在 4-5 次。为了实现他们的目标,作者使用了CRISPR / Cas9系统的“经典”版本。sgRNA 和 Cas9 组分均由单个载体表达,该载体还具有嘌呤霉素抗性盒;这是所选策略的基本模块,因为它确保了所选细胞中 sgRNA 和 Cas9 的表达。非线性质粒形式的靶向模板被证明具有最佳效率,并用于在编码 FOXA1 的基因中 295 位引入替换,以将编码赖氨酸的密码子转变为编码谷氨酰胺的密码子 (K295Q)。Li和合著者提出的策略是在多倍体环境(如癌细胞)中对多个拷贝基因进行基因组编辑的重要发展。该技术的一个重要应用可能是创建模型来研究单核苷酸多态性在癌症进展和转移中的作用。携带关键药物靶点多态性变异的同基因癌症细胞系可用于优化抗癌治疗方案,为个性化治疗奠定基础。

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