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Poly(l-lysine)-Coated Liquid CrystalDroplets for Sensitive Detection of DNA and Their Applications inControlled Release of Drug Molecules

机译:聚(L-赖氨酸)涂层液晶DNA灵敏检测的液滴及其应用药物分子的控制释放

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摘要

Interactions between DNA and adsorbed poly(l-lysine) (PLL) on liquid crystal (LC) droplets were investigated using polarizing optical microcopy and epi-fluorescence microscopy. Earlier, we demonstrated that adsorption of PLL to the LC/aqueous interface resulted in homeotropic orientation of the LC and thus exhibited a radial configuration of the LC confined within the droplets. Subsequent adsorption of DNA (single-stranded DNA/double-stranded DNA) at PLL-coated LC droplets was found to trigger an LC reorientation within the droplets, leading to preradial/bipolar configuration of those droplets. To our surprise, subsequent exposure of complementary ssDNA to ssDNA/adsorbed PLL-modified LC droplets did not cause the LC reorientation. This is likely due to the formation of polyplexes (DNA–PLL complex) as confirmed by fluorescence microscopy and atomic force microscopy. In addition, dsDNA-adsorbed PLL droplets have been found to be effectively useful to displace (controlled release) propidium iodide (a model drug) encapsulated within dsDNA over time. These observations suggest the potential fora label-free droplet-based LC detection system that can respond toDNA and may provide a simple method to develop DNA-based drug nanocarriers.
机译:使用偏振光学显微镜和落射荧光显微镜研究了DNA与液晶(LC)液滴上吸附的聚(1-赖氨酸)(PLL)之间的相互作用。早些时候,我们证明了PLL在LC /水界面上的吸附导致LC的垂直取向,因此显示出LC的径向构型局限在液滴内。发现随后在涂有PLL的LC液滴上吸附DNA(单链DNA /双链DNA)会触发液滴内的LC重新定向,从而导致这些液滴的辐射前/双极性构型。令我们惊讶的是,随后将互补ssDNA暴露于ssDNA /吸附的PLL修饰的LC小滴中并没有引起LC重新定向。如荧光显微镜和原子力显微镜所证实的,这可能是由于形成了多链体(DNA-PLL复合体)。此外,已发现dsDNA吸附的PLL液滴可有效地随时间推移置换(控制释放)dsDNA中封装的碘化丙锭(一种模型药物)。这些观察结果表明无标签的基于液滴的LC检测系统,可以响应DNA,并可能提供开发基于DNA的药物纳米载体的简单方法。

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