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金纳米粒子的细胞毒性作用:多参数研究。

Cytotoxic effects of gold nanoparticles: a multiparametric study.

机构信息

Lab of General Biochemistry and Physical Pharmacy, Faculty of Pharmaceutical Sciences, Ghent University, B-9000 Ghent, Belgium.

出版信息

ACS Nano. 2012 Jul 24;6(7):5767-83. doi: 10.1021/nn301714n. Epub 2012 Jun 8.

DOI:10.1021/nn301714n
PMID:22659047
Abstract

The in vitro labeling of therapeutic cells with nanoparticles (NPs) is becoming more and more common, but concerns about the possible effects of the NPs on the cultured cells are also increasing. In the present work, we evaluate the effects of poly(methacrylic acid)-coated 4 nm diameter Au NPs on a variety of sensitive and therapeutically interesting cell types (C17.2 neural progenitor cells, human umbilical vein endothelial cells, and PC12 rat pheochromocytoma cells) using a multiparametric approach. Using various NP concentrations and incubation times, we performed a stepwise analysis of the NP effects on cell viability, reactive oxygen species, cell morphology, cytoskeleton architecture, and cell functionality. The data show that higher NP concentrations (200 nM) reduce cell viability mostly through induction of reactive oxygen species, which was significantly induced at concentrations of 50 nM Au NPs or higher. At these concentrations, both actin and tubulin cytoskeleton were deformed and resulted in reduced cell proliferation and cellular differentiation. In terms of cell functionality, the NPs significantly impeded neurite outgrowth of PC12 cells up to 20 nM concentrations. At 10 nM, no significant effects on any cellular parameter could be observed. These data highlight the importance of using multiple assays to cover the broad spectrum of cell-NP interactions and to determine safe NP concentrations and put forward the described protocol as a possible template for future cell-NP interaction studies under comparable and standardized conditions.

摘要

将纳米粒子(NPs)体外标记治疗细胞变得越来越普遍,但人们对 NPs 对培养细胞可能产生的影响的担忧也在增加。在本工作中,我们使用多参数方法评估了聚(甲基丙烯酸)包覆的 4nm 直径 Au NPs 对多种敏感且具有治疗意义的细胞类型(C17.2 神经祖细胞、人脐静脉内皮细胞和 PC12 大鼠嗜铬细胞瘤细胞)的影响。使用不同的 NP 浓度和孵育时间,我们对 NP 对细胞活力、活性氧、细胞形态、细胞骨架结构和细胞功能的影响进行了逐步分析。数据表明,较高的 NP 浓度(200nM)主要通过诱导活性氧来降低细胞活力,在 50nM Au NPs 或更高浓度时,活性氧的诱导显著增加。在这些浓度下,肌动蛋白和微管骨架都发生了变形,导致细胞增殖和细胞分化减少。就细胞功能而言,NP 显著抑制了 PC12 细胞的突起生长,直至 20nM 浓度。在 10nM 时,观察不到对任何细胞参数的显著影响。这些数据强调了使用多种测定方法来涵盖细胞-NP 相互作用的广泛范围并确定安全的 NP 浓度的重要性,并提出了所描述的方案作为在类似和标准化条件下进行未来细胞-NP 相互作用研究的可能模板。

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