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Autonomous zinc-finger nuclease pairs for targeted chromosomal deletion

机译:自主锌指核酸酶对靶向的染色体缺失

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摘要

Zinc-finger nucleases (ZFNs) have been successfully used for rational genome engineering in a variety of cell types and organisms. ZFNs consist of a non-specific FokI endonuclease domain and a specific zinc-finger DNA-binding domain. Because the catalytic domain must dimerize to become active, two ZFN subunits are typically assembled at the cleavage site. The generation of obligate heterodimeric ZFNs was shown to significantly reduce ZFN-associated cytotoxicity in single-site genome editing strategies. To further expand the application range of ZFNs, we employed a combination of in silico protein modeling, in vitro cleavage assays, and in vivo recombination assays to identify autonomous ZFN pairs that lack cross-reactivity between each other. In the context of ZFNs designed to recognize two adjacent sites in the human HOXB13 locus, we demonstrate that two autonomous ZFN pairs can be directed simultaneously to two different sites to induce a chromosomal deletion in ∼10% of alleles. Notably, the autonomous ZFN pair induced a targeted chromosomal deletion with the same efficacy as previously published obligate heterodimeric ZFNs but with significantly less toxicity. These results demonstrate that autonomous ZFNs will prove useful in targeted genome engineering approaches wherever an application requires the expression of two distinct ZFN pairs.
机译:锌指核酸酶(ZFN)已成功用于多种细胞类型和生物体中的合理基因组工程。 ZFN由非特异性FokI核酸内切酶结构域和特定的锌指DNA结合结构域组成。因为催化结构域必须二聚化才具有活性,所以两个ZFN亚基通常在切割位点组装。在单一位点基因组编辑策略中,专性异二聚体ZFN的产生可显着降低ZFN相关的细胞毒性。为了进一步扩展ZFN的应用范围,我们采用了计算机模拟蛋白质建模,体外裂解测定和体内重组测定的组合,以识别彼此之间缺乏交叉反应性的自主ZFN对。在设计为识别人类HOXB13基因座中两个相邻位点的ZFN的背景下,我们证明了两个自治ZFN对可以同时定向到两个不同位点,以在约10%的等位基因中诱导染色体缺失。值得注意的是,自主ZFN对诱导了靶向的染色体缺失,其功效与先前发表的专性异二聚ZFN相同,但毒性明显降低。这些结果表明,自主ZFN在应用中需要表达两个不同ZFN对的情况下,将在靶向基因组工程方法中有用。

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