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Zinc finger nucleases: custom-designed molecular scissors for genome engineering of plant and mammalian cells

机译:锌指核酸酶:定制设计的分子剪刀,用于植物和哺乳动物细胞的基因组工程

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摘要

Custom-designed zinc finger nucleases (ZFNs), proteins designed to cut at specific DNA sequences, are becoming powerful tools in gene targeting—the process of replacing a gene within a genome by homologous recombination (HR). ZFNs that combine the non-specific cleavage domain (N) of FokI endonuclease with zinc finger proteins (ZFPs) offer a general way to deliver a site-specific double-strand break (DSB) to the genome. The development of ZFN-mediated gene targeting provides molecular biologists with the ability to site-specifically and permanently modify plant and mammalian genomes including the human genome via homology-directed repair of a targeted genomic DSB. The creation of designer ZFNs that cleave DNA at a pre-determined site depends on the reliable creation of ZFPs that can specifically recognize the chosen target site within a genome. The (Cys2His2) ZFPs offer the best framework for developing custom ZFN molecules with new sequence-specificities. Here, we explore the different approaches for generating the desired custom ZFNs with high sequence-specificity and affinity. We also discuss the potential of ZFN-mediated gene targeting for ‘directed mutagenesis’ and targeted ‘gene editing’ of the plant and mammalian genome as well as the potential of ZFN-based strategies as a form of gene therapy for human therapeutics in the future.
机译:定制设计的锌指核酸酶(ZFN),旨在切割特定DNA序列的蛋白质,正在成为基因靶向的强大工具,该过程是通过同源重组(HR)替换基因组内基因的过程。将FokI核酸内切酶的非特异性切割域(N)与锌指蛋白(ZFP)结合的ZFN提供了将位点特异性双链断裂(DSB)传递至基因组的一般方法。 ZFN介导的基因靶向的发展为分子生物学家提供了通过同源基因组定向修复基因组DSB进行位点特异性和永久性修饰植物和哺乳动物基因组(包括人类基因组)的能力。在预定位点切割DNA的设计者ZFN的产生取决于可特异性识别基因组中所选靶位点的ZFP的可靠产生。 (Cys2His2)ZFP提供了开发具有新序列特异性的定制ZFN分子的最佳框架。在这里,我们探索了产生具有高序列特异性和亲和力的所需定制ZFN的不同方法。我们还讨论了ZFN介导的基因靶向对植物和哺乳动物基因组的“定向诱变”和靶向“基因编辑”的潜力,以及基于ZFN的策略作为未来人类疗法的一种基因疗法的潜力。

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