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Quantitative investigation of compartmentalized dynamics of ErbB2 targeting gold nanorods in live cells by single molecule spectroscopy

机译:通过单分子光谱定量研究活细胞中靶向ErbB2的金纳米棒的区室动力学

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Understanding the diffusion dynamics and receptor uptake mechanism of nanoparticles in cancer cells is crucial to the rational design of multifunctional nanoprobes for targeting and delivery. In this report, for the first time, we quantify the localization and evaluate the diffusion times of Herceptin-conjugated gold nanorods (H-GNRs) in different cell organelles by fluorescence correlation spectroscopy (FCS) and examine the endocytic diffusion of H-GNRs in live ErbB2 overexpressing SK-BR-3 cells. First, by colocalizing H-GNRs in different cellular organelles depicted by the respective markers, we demonstrate that H-GNRs colocalize with the endosome and lysosome but not with the Golgi apparatus. Our study shows that Herceptin-conjugated GNRs have similar intracellular localization characteristics as Herceptin - ErbB2 complex, with a higher concentration found in the endosome (72 ± 20.6 nM) than lysosome (9.4 ± 4.2 nM) after internalization. The demonstrated approach and findings not only lay the foundations for a quantitative understanding of the fate of nanoparticle-based targeting but also provide new insights into the rational design of nanoparticle delivery systems for effective treatment.
机译:了解纳米粒子在癌细胞中的扩散动力学和受体摄取机制对于多功能纳米探针靶向和递送的合理设计至关重要。在本报告中,我们首次通过荧光相关光谱法(FCS)量化了赫赛汀共轭金纳米棒(H-GNRs)在不同细胞细胞器中的定位和扩散时间,并检查了H-GNRs在细胞内的内吞扩散过表达ErbB2的SK-BR-3细胞。首先,通过将H-GNRs分别定位在各个标记所描绘的不同细胞器中,我们证明了H-GNRs与内体和溶酶体共定位,而不与高尔基体共定位。我们的研究表明,与赫赛汀-ErbB2复合物相似,与赫赛汀共轭的GNR具有相似的胞内定位特性,在内化后,内体中的浓度(72±20.6 nM)比溶酶体(9.4±4.2 nM)高。证明的方法和发现不仅为定量了解基于纳米粒子的靶向命运奠定了基础,而且还为有效治疗纳米粒子输送系统的合理设计提供了新的见解。

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