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基因组编辑哺乳动物细胞中快速有效的网格蛋白介导的内吞作用。

Rapid and efficient clathrin-mediated endocytosis revealed in genome-edited mammalian cells.

机构信息

1] Department of Molecular and Cell Biology, University of California Berkeley, Berkeley, California 94720, USA.

出版信息

Nat Cell Biol. 2011 Mar;13(3):331-7. doi: 10.1038/ncb2175. Epub 2011 Feb 6.

Abstract

Clathrin-mediated endocytosis (CME) is the best-studied pathway by which cells selectively internalize molecules from the plasma membrane and surrounding environment. Previous live-cell imaging studies using ectopically overexpressed fluorescent fusions of endocytic proteins indicated that mammalian CME is a highly dynamic but inefficient and heterogeneous process. In contrast, studies of endocytosis in budding yeast using fluorescent protein fusions expressed at physiological levels from native genomic loci have revealed a process that is very regular and efficient. To analyse endocytic dynamics in mammalian cells in which endogenous protein stoichiometry is preserved, we targeted zinc finger nucleases (ZFNs) to the clathrin light chain A and dynamin-2 genomic loci and generated cell lines expressing fluorescent protein fusions from each locus. The genome-edited cells exhibited enhanced endocytic function, dynamics and efficiency when compared with previously studied cells, indicating that CME is highly sensitive to the levels of its protein components. Our study establishes that ZFN-mediated genome editing is a robust tool for expressing protein fusions at endogenous levels to faithfully report subcellular localization and dynamics.

摘要

网格蛋白介导的内吞作用(CME)是细胞从质膜和周围环境中选择性内化分子的研究得最多的途径。以前使用网格蛋白内吞蛋白的异位过表达荧光融合物进行的活细胞成像研究表明,哺乳动物的 CME 是一个高度动态但效率低下且异质的过程。相比之下,使用荧光蛋白融合物在生理水平上从天然基因组位点表达的出芽酵母内吞作用的研究揭示了一个非常规则且高效的过程。为了分析保留内源性蛋白质比例的哺乳动物细胞中的内吞动力学,我们将锌指核酸酶(ZFN)靶向网格蛋白轻链 A 和动力蛋白-2 基因组位点,并生成从每个位点表达荧光蛋白融合物的细胞系。与之前研究的细胞相比,基因组编辑的细胞表现出增强的内吞作用功能、动力学和效率,表明 CME 对其蛋白质成分的水平非常敏感。我们的研究表明,ZFN 介导的基因组编辑是一种在内源性水平表达融合蛋白的强大工具,可忠实地报告亚细胞定位和动力学。

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