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表面涂层对金纳米粒子细胞内行为的影响:荧光相关光谱研究。

Influence of surface coating on the intracellular behaviour of gold nanoparticles: a fluorescence correlation spectroscopy study.

机构信息

CNR - ISTM, Nanotechnology Lab., Via G. Fantoli 16/15, 20138, Milan, Italy.

出版信息

Nanoscale. 2017 Oct 5;9(38):14730-14739. doi: 10.1039/c7nr04640e.

DOI:10.1039/c7nr04640e
PMID:28948261
Abstract

In the biomedical applications of nanoparticles (NPs), the proper choice of surface chemistry is a crucial aspect in their design. The nature of the coating can heavily impact the interaction of NPs with biomolecules, affect the state of aggregation, and ultimately determine their biological fate. As such, protein corona formation and the aggregation behaviour of gold NPs (Au NPs) are studied here. Au NPs are prepared with four distinct surface functionalisations, namely mercaptosuccinic acid (MSA), N-4-thiobutyroil glucosamine, HS-PEG and HS-alkyl-PEG. Corona formation, aggregation, and the intracellular behaviour of the Au NPs are then investigated by means of Fluorescence Correlation Spectroscopy (FCS) in cell culture media and in live cells. To evaluate the state of aggregation and the formation of a protein corona, the Au NPs are incubated in cell media and the diffusion coefficient is determined via FCS. The in vitro behaviour is compared with the level of aggregation of the NPs in cells. Diffusion times of the NPs are estimated at different positions in the cell after a one hour incubation period. It is found that the majority of MSA and glucose-Au NPs are present inside the cell as slowly diffusing species with diffusion times (τ) greater than 6000 μs (hydrodynamic diameter >250 nm). PEGylated Au NPs adsorb a small amount of protein and manifest low agglomeration both in media and in living cells. In particular, the HS-alkyl-PEG coating shows an excellent correlation between lower protein adsorption, 4-fold lower compared to the MSA coated NPs, and limited intracellular aggregation. In the case of single HS-alkyl-PEG coated NPs, it is found that typical intracellular τ values range from 500 to 1500 μs, indicating that these particles display reduced aggregation in the intracellular environment.

摘要

在纳米粒子(NPs)的生物医学应用中,表面化学的正确选择是其设计的关键方面。涂层的性质会严重影响 NPs 与生物分子的相互作用、影响聚集状态,并最终决定它们的生物命运。因此,本文研究了金纳米粒子(Au NPs)的蛋白冠形成和聚集行为。通过四种不同的表面功能化方法制备 Au NPs,即巯基琥珀酸(MSA)、N-4-硫代丁酰葡萄糖胺、HS-PEG 和 HS-烷基-PEG。然后通过荧光相关光谱(FCS)在细胞培养介质和活细胞中研究了 Au NPs 的冠形成、聚集和细胞内行为。为了评估聚集状态和蛋白冠的形成,将 Au NPs 孵育在细胞培养基中,并通过 FCS 确定扩散系数。将体外行为与细胞内 NPs 的聚集水平进行比较。在孵育 1 小时后,在细胞的不同位置估计 NP 的扩散时间。结果发现,大多数 MSA 和葡萄糖-Au NPs 作为扩散缓慢的物质存在于细胞内,扩散时间(τ)大于 6000 μs(水动力直径>250nm)。PEG 化 Au NPs 吸附少量的蛋白质,在介质和活细胞中表现出低聚集。特别是 HS-烷基-PEG 涂层表现出良好的相关性,即蛋白吸附量低(与 MSA 涂层 NPs 相比低 4 倍),细胞内聚集有限。在单 HS-烷基-PEG 涂层 NPs 的情况下,发现典型的细胞内 τ 值范围为 500 至 1500 μs,表明这些颗粒在细胞内环境中显示出较低的聚集。

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