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两亲性环糊精与 pDNA 形成甘露糖修饰的纳米复合物用于靶向基因传递。

Mannosyl-coated nanocomplexes from amphiphilic cyclodextrins and pDNA for site-specific gene delivery.

机构信息

Instituto de Investigaciones Químicas, CSIC-Universidad de Sevilla, Sevilla, Spain.

出版信息

Biomaterials. 2011 Oct;32(29):7263-73. doi: 10.1016/j.biomaterials.2011.06.025. Epub 2011 Jul 7.

DOI:10.1016/j.biomaterials.2011.06.025
PMID:21741082
Abstract

Fully homogeneous facial amphiphiles consisting in a cyclodextrin (CD) platform onto which a polycationic cluster and a multi-tail hydrophobic moiety have been installed (polycationic amphiphilic CDs; paCDs) self-organized in the presence of plasmid DNA to form nanometric complexes (CDplexes) which exhibit broad-range transfection capabilities. We hypothesized that biorecognizable moieties located at the hydrophilic rim in the CD scaffold would be exposed at the surface of the corresponding nanoparticles after DNA-promoted aggregation, endowing the system with molecular recognition abilities towards cell receptors. This concept has been demonstrated by developing an efficient synthetic strategy for the preparation of multivalent polycationic glyco-amphiphilic CDs (pGaCDs). Self-assembled nanoparticles obtained from mannosylated pGaCDs and pDNA (average hydrodynamic diameter 80 nm) have been shown to be specifically recognized by mannose-specific lectins, including concanavalin A (Con A) and the human macrophage mannose receptor (MMR). Further macrophage adhesion studies indicated that unspecific binding, probably due to electrostatic interactions with negatively charged cell membrane components, can also operate. The relative specific versus non-specific internalization is dependent on the pGaCD:pDNA proportion, being optimal at a protonable nitrogen/phosphate (N/P) ratio of 5. The resulting GlycoCDplexes were shown to specifically mediate transfection in Raw 264.7 (murine macrophage) cells expressing the mannose-fucose receptor in vitro. FACS experiments confirmed that transfection using these nanoparticles is mannose-dependent, supporting the potential of the approach towards vectorized gene delivery.

摘要

由环糊精(CD)平台组成的完全均相两亲分子,其上安装了聚阳离子簇和多尾疏水部分(聚阳离子两亲性 CD;paCD),在质粒 DNA 的存在下自组装成纳米级复合物(CDplex),具有广泛的转染能力。我们假设,位于 CD 支架亲水边缘的生物识别部分在 DNA 促进聚集后会暴露在相应纳米颗粒的表面,赋予该系统对细胞受体的分子识别能力。通过开发一种用于制备多价聚阳离子糖基两亲性 CD(pGaCD)的有效合成策略,证明了这一概念。从甘露糖化 pGaCD 和 pDNA 获得的自组装纳米颗粒(平均水动力直径 80nm)被证明可被甘露糖特异性凝集素(包括刀豆球蛋白 A(Con A)和人巨噬细胞甘露糖受体(MMR))特异性识别。进一步的巨噬细胞黏附研究表明,非特异性结合(可能由于与带负电荷的细胞膜成分的静电相互作用)也可能发生。相对特异性与非特异性内化的比例取决于 pGaCD:pDNA 的比例,在质子化氮/磷酸(N/P)比为 5 时最佳。结果表明,糖基化 CDplex 可特异性介导体外表达甘露糖-岩藻糖受体的 Raw 264.7(鼠巨噬细胞)细胞的转染。FACS 实验证实,使用这些纳米粒子进行转染依赖于甘露糖,支持该方法在载体基因传递方面的潜力。

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