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利用细胞穿透性Cys2-His2锌指结构域将蛋白质直接递送至哺乳动物细胞。

Direct protein delivery to mammalian cells using cell-permeable Cys2-His2 zinc-finger domains.

作者信息

Gaj Thomas, Liu Jia

机构信息

Departments of Chemistry and Cell and Molecular Biology, The Scripps Research Institute;

Departments of Chemistry and Cell and Molecular Biology, The Scripps Research Institute; Shanghai Institute for Advanced Immunochemical Studies, ShanghaiTech University.

出版信息

J Vis Exp. 2015 Mar 25(97):52814. doi: 10.3791/52814.

Abstract

Due to their modularity and ability to be reprogrammed to recognize a wide range of DNA sequences, Cys2-His2 zinc-finger DNA-binding domains have emerged as useful tools for targeted genome engineering. Like many other DNA-binding proteins, zinc-fingers also possess the innate ability to cross cell membranes. We recently demonstrated that this intrinsic cell-permeability could be leveraged for intracellular protein delivery. Genetic fusion of zinc-finger motifs leads to efficient transport of protein and enzyme cargo into a broad range of mammalian cell types. Unlike other protein transduction technologies, delivery via zinc-finger domains does not inhibit enzyme activity and leads to high levels of cytosolic delivery. Here a detailed step-by-step protocol is presented for the implementation of zinc-finger technology for protein delivery into mammalian cells. Key steps for achieving high levels of intracellular zinc-finger-mediated delivery are highlighted and strategies for maximizing the performance of this system are discussed.

摘要

由于其模块化特性以及能够被重新编程以识别广泛的DNA序列,Cys2-His2锌指DNA结合域已成为靶向基因组工程的有用工具。与许多其他DNA结合蛋白一样,锌指也具有穿越细胞膜的固有能力。我们最近证明,这种内在的细胞通透性可用于细胞内蛋白质递送。锌指基序的基因融合导致蛋白质和酶货物有效转运到广泛的哺乳动物细胞类型中。与其他蛋白质转导技术不同,通过锌指结构域进行递送不会抑制酶活性,并导致高水平的胞质递送。本文介绍了将锌指技术用于向哺乳动物细胞递送蛋白质的详细分步方案。强调了实现高水平细胞内锌指介导递送的关键步骤,并讨论了最大化该系统性能的策略。

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