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阳离子表面活性剂介导的基因转移基本上受限于表面活性剂/DNA复合物在细胞膜上的滞留:一项荧光研究。

Gene transfer by cationic surfactants is essentially limited by the trapping of the surfactant/DNA complexes onto the cell membrane: a fluorescence investigation.

作者信息

Clamme J P, Bernacchi S, Vuilleumier C, Duportail G, Mély Y

机构信息

Laboratoire Pharmacologie et physico-chimie des interactions cellulaires et moléculaires', UMR 7034 du CNRS, Faculté de Pharmacie, Université Louis Pasteur de Strasbourg, Illkirch, France.

出版信息

Biochim Biophys Acta. 2000 Aug 25;1467(2):347-61. doi: 10.1016/s0005-2736(00)00230-3.

Abstract

The interaction between complexes of plasmid DNA with cetyltrimethylammonium bromide (CTAB) and L929 fibroblasts was first examined using confocal microscopy. The complexes labeled with the DNA intercalator, YOYO-1, were found to be trapped onto the external face of the plasma membrane; a feature that may constitute a major limiting step in transfection. Moreover, since no cytotoxic effect appeared in these conditions, we further inferred that the CTAB molecules remained bound to the DNA. The interaction of the complexes with the membranes was best modeled with neutral vesicles. From anisotropy thermotropic curves of DPHpPC-labeled vesicles and fluorescence resonance energy transfer measurements between these vesicles and YOYO-labeled complexes, we evidenced that the binding of the complexes to the vesicle surface opened the micelle-like domains and unwound DNA. However, DNA was not released but remained stably bound via electrostatic interactions to the CTAB molecules incorporated in the external liposome leaflet. Consequently, the large diameter of the unwound plasmid DNA is likely the major factor that precludes its internalization into the cells by endocytosis. In contrast, anionic vesicles that mimic the cytoplasmic facing monolayer of the plasma membrane rapidly released DNA from the complex. This may explain the previously reported high transfection efficiency of DNA complexed with liposomes composed of neutral lipids and cationic surfactants, since the latter may destabilize the endosomal membrane and induce the release of DNA in the cytoplasm.

摘要

首先使用共聚焦显微镜检查了质粒DNA与十六烷基三甲基溴化铵(CTAB)的复合物与L929成纤维细胞之间的相互作用。发现用DNA嵌入剂YOYO-1标记的复合物被困在质膜的外表面;这一特征可能是转染过程中的一个主要限制步骤。此外,由于在这些条件下未出现细胞毒性作用,我们进一步推断CTAB分子仍与DNA结合。复合物与膜的相互作用用中性囊泡进行模拟最为合适。从DPHpPC标记囊泡的各向异性热致曲线以及这些囊泡与YOYO标记复合物之间的荧光共振能量转移测量结果,我们证明复合物与囊泡表面的结合打开了类似胶束的结构域并使DNA解旋。然而,DNA并未释放,而是通过静电相互作用稳定地结合在掺入外部脂质体小叶中的CTAB分子上。因此,解旋的质粒DNA的大直径可能是阻止其通过内吞作用内化到细胞中的主要因素。相比之下,模拟质膜面向细胞质单层的阴离子囊泡会迅速从复合物中释放DNA。这可能解释了先前报道的与由中性脂质和阳离子表面活性剂组成的脂质体复合的DNA具有高转染效率的原因,因为后者可能会破坏内体膜的稳定性并诱导DNA在细胞质中释放。

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