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无标记共焦拉曼映射法研究转铁蛋白在黑素瘤细胞中的转运。

Label-Free Confocal Raman Mapping of Transportan in Melanoma Cells.

出版信息

Mol Pharm. 2018 Mar 5;15(3):851-860. doi: 10.1021/acs.molpharmaceut.7b00601. Epub 2018 Feb 13.

Abstract

Cell-penetrating peptides (CPPs) are promising vectors for the intracellular delivery of a variety of membrane-impermeable bioactive compounds. The mechanisms by which CPPs cross the cell membrane, and the effects that CPPs may have on cell function, still remain to be fully clarified. In this work, we employed confocal Raman microscopy (CRM) and atomic force microscopy (AFM) to study the infiltration and physiological effects of the amphipathic CPP transportan (Tp) on the metastatic melanoma cell line SK-Mel-2. CRM enabled the detection of label-free Tp within the cells. Raman maps of live cells revealed rapid entry (within 5 min) and widespread distribution of the peptide throughout the cytoplasm and the presence of the peptide within the nucleus after ∼20 min. Principal component analysis of the CRM data collected from Tp-treated and untreated cells showed that Tp Raman bands were not positively correlated with lipid Raman bands, indicating that Tp entered the cells via a nonendocytic mechanism. Analysis of intracellularly recovered Tp by mass spectrometry showed that Tp remained intact in SK-Mel-2 cells for up to 24 h. The Raman spectroscopic data also showed that, although Tp was predominantly unstructured (random coil) in aqueous solution, it accumulated to high densities within the cells with mostly β-sheet and α-helical structures. AFM was employed to measure the effect of Tp treatment on cell stiffness. These data showed that Tp induced a significant increase in cell stiffness within the first hour of treatment, which was partially abated after 2 h. It is hypothesized that the increase in cell stiffness was the result of cytoskeletal changes triggered by Tp.

摘要

细胞穿透肽 (CPPs) 是将各种不可渗透细胞膜的生物活性化合物递送到细胞内的有前途的载体。CPP 穿过细胞膜的机制以及 CPP 对细胞功能可能产生的影响仍有待充分阐明。在这项工作中,我们使用共聚焦拉曼显微镜 (CRM) 和原子力显微镜 (AFM) 研究了两亲性 CPP 转铁蛋白 (Tp) 对转移性黑色素瘤细胞系 SK-Mel-2 的渗透和生理作用。CRM 能够检测细胞内无标记的 Tp。活细胞的拉曼图谱显示,该肽在 5 分钟内快速进入 (within 5 min) 并广泛分布于细胞质中,约 20 分钟后该肽存在于细胞核内。对 Tp 处理和未处理细胞的 CRM 数据进行主成分分析表明,Tp 的 Raman 带与脂质 Raman 带没有正相关,表明 Tp 通过非内吞机制进入细胞。通过质谱分析从 SK-Mel-2 细胞中回收的细胞内 Tp 表明,Tp 在细胞内长达 24 小时保持完整。拉曼光谱数据还表明,尽管 Tp 在水溶液中主要是无规卷曲 (random coil),但它在细胞内以主要的 β-折叠和 α-螺旋结构积累到高密度。AFM 用于测量 Tp 处理对细胞刚性的影响。这些数据表明,Tp 在处理后的第一个小时内显著增加了细胞刚性,在 2 小时后部分减轻。据推测,细胞刚性的增加是 Tp 触发细胞骨架变化的结果。

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