Endes Carola, Schmid Otmar, Kinnear Calum, Mueller Silvana, Camarero-Espinosa Sandra, Vanhecke Dimitri, Foster E Johan, Petri-Fink Alke, Rothen-Rutishauser Barbara, Weder Christoph, Clift Martin J D
Part Fibre Toxicol. 2014 Sep 23;11:40. doi: 10.1186/s12989-014-0040-x.
The challenge remains to reliably mimic human exposure to high aspect ratio nanoparticles (HARN) via inhalation. Sophisticated, multi-cellular in vitro models are a particular advantageous solution to this issue, especially when considering the need to provide realistic and efficient alternatives to invasive animal experimentation for HARN hazard assessment. By incorporating a systematic test-bed of material characterisation techniques, a specific air-liquid cell exposure system with real-time monitoring of the cell-delivered HARN dose in addition to key biochemical endpoints, here we demonstrate a successful approach towards investigation of the hazard of HARN aerosols in vitro.
Cellulose nanocrystals (CNCs) derived from cotton and tunicates, with differing aspect ratios (~9 and ~80), were employed as model HARN samples. Specifically, well-dispersed and characterised CNC suspensions were aerosolised using an "Air Liquid Interface Cell Exposure System" (ALICE) at realistic, cell-delivered concentrations ranging from 0.14 to 1.57 μg/cm2. The biological impact (cytotoxicity, oxidative stress levels and pro-inflammatory effects) of each HARN sample was then assessed using a 3D multi-cellular in vitro model of the human epithelial airway barrier at the air liquid interface (ALI) 24 hours post-exposure. Additionally, the testing strategy was validated using both crystalline quartz (DQ12) as a positive particulate control in the ALICE system and long fibre amosite asbestos (LFA) to confirm the susceptibility of the in vitro model to a fibrous insult.
A rapid (≤ 4 min), controlled nebulisation of CNC suspensions enabled a dose-controlled and spatially homogeneous CNC deposition onto cells cultured under ALI conditions. Real-time monitoring of the cell-delivered CNC dose with a quartz crystal microbalance was accomplished. Independent of CNC aspect ratio, no significant cytotoxicity (p>0.05), induction of oxidative stress, or (pro)-inflammatory responses were observed up to the highest concentration of 1.57 μg/cm2. Both DQ12 and LFA elicited a significant (p<0.05) pro-inflammatory response at sub-lethal concentrations in vitro.
In summary, whilst the present study highlights the benign nature of CNCs, it is the advanced technological and mechanistic approach presented that allows for a state of the art testing strategy to realistically and efficiently determine the in vitro hazard concerning inhalation exposure of HARN.
通过吸入可靠模拟人类对高纵横比纳米颗粒(HARN)的暴露仍是一项挑战。复杂的多细胞体外模型是解决该问题的一种特别有利的方法,尤其是考虑到需要为HARN危害评估提供侵入性动物实验的现实且高效的替代方案时。通过纳入材料表征技术的系统测试平台,以及一个能够实时监测细胞所接触的HARN剂量和关键生化终点的特定气液细胞暴露系统,我们在此展示了一种成功的体外研究HARN气溶胶危害的方法。
使用来自棉花和被囊动物、具有不同纵横比(约9和约80)的纤维素纳米晶体(CNC)作为模型HARN样本。具体而言,使用“气液界面细胞暴露系统”(ALICE)将充分分散且已表征的CNC悬浮液雾化,使其以0.14至1.57μg/cm²的实际细胞接触浓度存在。然后在暴露24小时后,使用人上皮气道屏障的3D多细胞体外模型在气液界面(ALI)评估每个HARN样本的生物学影响(细胞毒性、氧化应激水平和促炎作用)。此外,通过在ALICE系统中使用结晶石英(DQ12)作为阳性颗粒对照以及长纤维铁石棉(LFA)来验证测试策略,以确认体外模型对纤维损伤的敏感性。
CNC悬浮液能够快速(≤4分钟)、可控地雾化,从而实现剂量可控且在空间上均匀地将CNC沉积到在ALI条件下培养的细胞上。利用石英晶体微天平对细胞所接触的CNC剂量进行了实时监测。在高达1.57μg/cm²的最高浓度下,无论CNC的纵横比如何,均未观察到显著的细胞毒性(p>0.05)、氧化应激诱导或(促)炎反应。在体外亚致死浓度下,DQ12和LFA均引发了显著的(p<0.05)促炎反应。
总之,虽然本研究突出了CNC的良性性质,但所提出的先进技术和机制方法使得能够采用一种先进的测试策略,以现实且高效地确定关于吸入暴露HARN的体外危害。
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