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电穿孔转染后单个质粒 DNA 颗粒的细胞内追踪。

Intracellular tracking of single-plasmid DNA particles after delivery by electroporation.

机构信息

1] Department of Chemistry, University of Konstanz, Konstanz, Germany [2] CNRS, Institut de Pharmacologie et de Biologie Structurale, Toulouse, France [3] University of Toulouse III Paul Sabatier, Toulouse, France.

出版信息

Mol Ther. 2013 Dec;21(12):2217-26. doi: 10.1038/mt.2013.182. Epub 2013 Aug 14.

Abstract

Electroporation is a physical method of transferring molecules into cells and tissues. It takes advantage of the transient permeabilization of the cell membrane induced by electric field pulses, which gives hydrophilic molecules access to the cytoplasm. This method offers high transfer efficiency for small molecules that freely diffuse through electrically permeabilized membranes. Larger molecules, such as plasmid DNA, face several barriers (plasma membrane, cytoplasmic crowding, and nuclear envelope), which reduce transfection efficiency and engender a complex mechanism of transfer. Our work provides insight into the way electrotransferred DNA crosses the cytoplasm to reach the nucleus. For this purpose, single-particle tracking experiments of fluorescently labeled DNA were performed. Investigations were focused on the involvement of the cytoskeleton using drugs disrupting or stabilizing actin and tubulin filaments as the two relevant cellular networks for particle transport. The analysis of 315 movies (~4,000 trajectories) reveals that DNA is actively transported through the cytoskeleton. The large number of events allows a statistical quantification of the DNA motion kinetics inside the cell. Disruption of both filament types reduces occurrence and velocities of active transport and displacements of DNA particles. Interestingly, stabilization of both networks does not enhance DNA transport.

摘要

电穿孔是一种将分子转移到细胞和组织中的物理方法。它利用电场脉冲诱导的细胞膜瞬时通透性,使亲水分子进入细胞质。该方法对可自由扩散穿过电穿孔膜的小分子具有较高的转移效率。对于较大的分子,如质粒 DNA,则面临多种障碍(质膜、细胞质拥挤和核膜),这会降低转染效率并引发复杂的转移机制。我们的工作深入了解了电转移 DNA 穿过细胞质到达细胞核的方式。为此,进行了荧光标记 DNA 的单颗粒跟踪实验。研究集中于使用破坏或稳定肌动蛋白和微管蛋白丝的药物来参与细胞骨架,因为这两种细胞骨架网络是用于颗粒运输的。对 315 部电影(约 4000 条轨迹)的分析表明,DNA 是通过细胞骨架主动运输的。大量的事件允许对细胞内 DNA 运动动力学进行统计量化。两种丝状结构的破坏都会降低主动运输的发生频率和速度以及 DNA 颗粒的位移。有趣的是,两种网络的稳定都不会增强 DNA 运输。

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