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细胞穿透肽在短暂的光诱导下可确保完整货物的有效内涵体逃逸。

Cell-penetrating peptide secures an efficient endosomal escape of an intact cargo upon a brief photo-induction.

机构信息

Institute of Molecular and Cell Biology, University of Tartu, 23 Riia Street, 51010, Tartu, Estonia,

出版信息

Cell Mol Life Sci. 2013 Dec;70(24):4825-39. doi: 10.1007/s00018-013-1416-z. Epub 2013 Jul 13.

Abstract

Since their discovery, cell-penetrating peptides (CPPs) have provided a novel, efficient, and non-invasive mode of transport for various (bioactive) cargos into cells. Despite the ever-growing number of successful implications of the CPP-mediated delivery, issues concerning their intracellular trafficking, significant targeting to degradative organelles, and limited endosomal escape are still hindering their widespread use. To overcome these obstacles, we have utilized a potent photo-induction technique with a fluorescently labeled protein cargo attached to an efficient CPP, TP10. In this study we have determined some key requirements behind this induced escape (e.g., dependence on peptide-to-cargo ratio, time and cargo), and have semi-quantitatively assessed the characteristics of the endosomes that become leaky upon this treatment. Furthermore, we provide evidence that the photo-released cargo remains intact and functional. Altogether, we can conclude that the photo-induced endosomes are specific large complexes-condensed non-acidic vesicles, where the released cargo remains in its native intact form. The latter was confirmed with tubulin as the cargo, which upon photo-induction was incorporated into microtubules. Because of this, we propose that combining the CPP-mediated delivery with photo-activation technique could provide a simple method for overcoming major limitations faced today and serve as a basis for enhanced delivery efficiency and a subsequent elevated cellular response of different bioactive cargo molecules.

摘要

自发现以来,细胞穿透肽(CPP)为各种(生物活性)货物进入细胞提供了一种新颖、高效和非侵入性的运输方式。尽管 CPP 介导的递呈的成功应用案例不断增加,但有关其细胞内转运、向降解性细胞器的有效靶向和有限的内体逃逸的问题仍然阻碍了它们的广泛应用。为了克服这些障碍,我们利用一种有效的光诱导技术,将荧光标记的蛋白货物附着到高效 CPP(TP10)上。在这项研究中,我们确定了这种诱导逃逸背后的一些关键要求(例如,依赖于肽与货物的比例、时间和货物),并对半定量评估了在这种处理下发生渗漏的内体的特征。此外,我们提供了证据表明,光释放的货物仍然完整且具有功能。总的来说,我们可以得出结论,光诱导的内体是特定的大复合物-凝聚的非酸性囊泡,其中释放的货物保持其天然完整的形式。这一点通过货物为微管蛋白得到了证实,在光诱导下,微管蛋白被整合到微管中。因此,我们提出将 CPP 介导的递呈与光激活技术相结合,可以为克服当前面临的主要限制提供一种简单的方法,并为提高不同生物活性货物分子的递呈效率和随后的细胞反应提供基础。

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