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转染过程中基因传递载体聚乙烯亚胺的细胞内动力学:双光子荧光相关光谱法研究

Intracellular dynamics of the gene delivery vehicle polyethylenimine during transfection: investigation by two-photon fluorescence correlation spectroscopy.

作者信息

Clamme Jean-Pierre, Krishnamoorthy Guruswamy, Mély Yves

机构信息

UMR 7034 CNRS, Faculté de Pharmacie, Université Louis Pasteur, Strasbourg 1, 74 Route du Rhin, B.P. 24, F-67401 Cedex Illkirch, France.

出版信息

Biochim Biophys Acta. 2003 Oct 31;1617(1-2):52-61. doi: 10.1016/j.bbamem.2003.09.002.

Abstract

Though polyethylenimine (PEI) is one of the most efficient nonviral vectors, one concern is the significant cytotoxicity of free PEI that represents about 80% of the PEI molecules in PEI/DNA mixtures used for transfection. In this respect, the aim of this work was to further investigate the intracellular fate of PEI during transfection of L929 fibroblasts. To this end, we analyzed by fluorescence correlation spectroscopy (FCS) using two-photon excitation the intracellular concentration and diffusion properties of labeled PEI and PEI/DNA complexes in various compartments of L929 cells. High initial fluorescence intensity, rapid photobleaching and the absence of measurable autocorrelation curves in most selected locations in cytoplasm suggest that PEI/DNA complexes and PEI accumulate (up to 30 times the concentration in the extracellular medium) in late endosomes bound to the inner membrane face. This feature, together with membrane destabilizing properties of PEI, may explain the release of PEI into cytoplasm and subsequent diffusion into the nucleus. In the nucleus, the concentration of PEI was found to be about 2.5- to 3.5-fold higher than the one in the incubation medium. Moreover, autocorrelation curves obtained in the nuclear compartment can be analyzed with either a two-component model (with the major fraction undergoing free Brownian diffusion) or an anomalous diffusion model. Both the endosomal disruption and the large intranuclear PEI concentration may contribute to PEI cytotoxicity.

摘要

尽管聚乙烯亚胺(PEI)是最有效的非病毒载体之一,但一个问题是游离PEI具有显著的细胞毒性,在用于转染的PEI/DNA混合物中,游离PEI占PEI分子的约80%。在这方面,这项工作的目的是进一步研究PEI在L929成纤维细胞转染过程中的细胞内命运。为此,我们通过双光子激发荧光相关光谱(FCS)分析了L929细胞各个区室中标记的PEI和PEI/DNA复合物的细胞内浓度及扩散特性。细胞质中大多数选定位置的初始荧光强度高、光漂白快且没有可测量的自相关曲线,这表明PEI/DNA复合物和PEI在内质体晚期与内膜表面结合处积累(浓度高达细胞外培养基中的30倍)。这一特征,连同PEI的膜去稳定特性,可能解释了PEI释放到细胞质中并随后扩散到细胞核中的现象。在细胞核中,发现PEI的浓度比孵育培养基中的浓度高约2.5至3.5倍。此外,在核区室获得的自相关曲线可以用双组分模型(主要部分进行自由布朗扩散)或反常扩散模型进行分析。内质体破裂和核内高浓度的PEI都可能导致PEI的细胞毒性。

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