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首页> 外文期刊>Journal of nanoparticle research: An interdisciplinary forum for nanoscale science and technology >Quantification of Al_2O_3 nanoparticles in human cell lines applying inductively coupled plasma mass spectrometry (neb-ICP-MS, LA-ICP-MS) and flow cytometry-based methods
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Quantification of Al_2O_3 nanoparticles in human cell lines applying inductively coupled plasma mass spectrometry (neb-ICP-MS, LA-ICP-MS) and flow cytometry-based methods

机译:应用感应耦合等离子体质谱法(neb-ICP-MS,LA-ICP-MS)和基于流式细胞仪的方法对人类细胞系中Al_2O_3纳米颗粒进行定量

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摘要

In order to quantify and compare the uptake of aluminum oxide nanoparticles of three different sizes into two human cell lines (skin keratinocytes (HaCaT) and lung epithelial cells (A549)), three analytical methods were applied: digestion followed by nebulization inductively coupled plasma mass spectrometry (neb-ICP-MS), direct laser ablation ICP-MS (LA-ICP-MS), and flow cytometry. Light and electron microscopy revealed an accumulation and agglomeration of all particle types within the cell cytoplasm, whereas no particles were detected in the cell nuclei. The internalized Al_2O_3 particles exerted no toxicity in the two cell lines after 24 h of exposure. The smallest particles with a primary particle size (x_(BET)) of 14 nm (Alu1) showed the lowest sedimentation velocity within the cell culture media, but were calculated to have settled completely after 20 h. Alu2 (x_(BET) = 111 nm) and Alu3 (x_(BET) = 750 nm) were calculated to reach the cell surface after 7 h and 3 min, respectively. The internal concentrations determined with the different methods lay in a comparable range of 2-8 μg Al_2O_3/cm~2 cell layer, indicating the suitability of all methods to quantify the nanoparticle uptake. Nevertheless, particle size limitations of analytical methods using optical devices were demonstrated for LA-ICP-MS and flow cytometry. Furthermore, the consideration and comparison of particle properties as parameters for particle internalization revealed the particle size and the exposure concentration as determining factors for particle uptake.
机译:为了量化和比较三种不同尺寸的氧化铝纳米粒子在两种人类细胞系(皮肤角质形成细胞(HaCaT)和肺上皮细胞(A549))中的吸收,采用了三种分析方法:消化,然后雾化电感耦合血浆质量光谱分析(neb-ICP-MS),直接激光烧蚀ICP-MS(LA-ICP-MS)和流式细胞仪。光镜和电子显微镜显示细胞质内所有颗粒类型的积累和聚集,而在细胞核中未检测到颗粒。暴露24 h后,内在化的Al_2O_3颗粒在这两个细胞系中均未表现出毒性。一次粒径(x_(BET))为14 nm(Alu1)的最小颗粒在细胞培养基中的沉降速度最低,但经计算在20 h后已完全沉降。计算Alu2(x_(BET)= 111 nm)和Alu3(x_(BET)= 750 nm)分别在7小时和3分钟后到达细胞表面。用不同方法测定的内部浓度在2-8μgAl_2O_3 / cm〜2细胞层的可比范围内,表明所有方法都适用于量化纳米颗粒的吸收。但是,对于LA-ICP-MS和流式细胞仪,已经证明了使用光学设备的分析方法的粒径限制。此外,作为颗粒内在化参数的颗粒性质的考虑和比较表明颗粒大小和暴露浓度是决定颗粒吸收的因素。

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