Development of an In Vitro Sensitisation Test Using a Coculture System of Human Bronchial Epithelium and Immune Cells.

IF 2.4 4区 医学 Q3 MEDICINE, RESEARCH & EXPERIMENTAL Atla-Alternatives To Laboratory Animals Pub Date : 2023-11-01 Epub Date: 2023-10-05 DOI:10.1177/02611929231204823
Ikuya Tanabe, Kunitaka Yoshida, Shinkichi Ishikawa, Kanae Ishimori, Tsuneo Hashizume, Takayuki Yoshimoto, Takao Ashikaga
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引用次数: 1

Abstract

Chemical respiratory sensitisation is a serious health problem. However, to date, there are no validated test methods available for identifying respiratory sensitisers. The aim of this study was to develop an in vitro sensitisation test by modifying the human cell line activation test (h-CLAT) to detect respiratory sensitisers and distinguish them from skin sensitisers. THP-1 cells were exposed to the test chemicals (two skin sensitisers and six respiratory sensitisers), either as monocultures or as cocultures with air-liquid interface-cultured reconstructed human bronchial epithelium. The responses were analysed by measuring the expression levels of surface markers on THP-1 cells (CD86, CD54 and OX40L) and the concentrations of cytokines in the culture media (interleukin (IL)-8, IL-33 and thymic stromal lymphopoietin (TSLP)). The cocultures exhibited increased CD54 expression on THP-1 cells; moreover, in the cocultures but not in the monocultures, exposure to two uronium salts (i.e. respiratory sensitisers) increased CD54 expression on THP-1 cells to levels above the criteria for a positive h-CLAT result. Additionally, exposure to the respiratory sensitiser abietic acid, significantly increased IL-8 concentration in the culture medium, but only in the cocultures. Although further optimisation of the method is needed to distinguish respiratory from skin sensitisers by using these potential markers (OX40L, IL-33 and TSLP), the coculture of THP-1 cells with bronchial epithelial cells offers a potentially useful approach for the detection of respiratory sensitisers.

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使用人支气管上皮和免疫细胞的共培养系统开发体外致敏试验。
化学性呼吸道致敏是一个严重的健康问题。然而,到目前为止,还没有经过验证的检测方法可用于识别呼吸道致敏剂。本研究的目的是通过修改人类细胞系激活试验(h-CLAT)来开发一种体外致敏试验,以检测呼吸道致敏剂并将其与皮肤致敏剂区分开来。THP-1细胞暴露于测试化学物质(两种皮肤致敏剂和六种呼吸致敏剂),无论是单培养还是与气液界面培养的重建人支气管上皮共培养。通过测量THP-1细胞表面标志物(CD86、CD54和OX40L)的表达水平和培养基中细胞因子(白细胞介素(IL)-8、IL-33和胸腺基质淋巴细胞生成素(TSLP))的浓度来分析反应。共培养物在THP-1细胞上表现出CD54表达增加;此外,在共培养物中而不是单培养物中,暴露于两种糖醛酸盐(即呼吸增敏剂)使THP-1细胞上CD54的表达增加到高于h-CLAT阳性结果标准的水平。此外,暴露于呼吸道致敏剂枞酸显著增加了培养基中的IL-8浓度,但仅在共培养物中。尽管需要进一步优化该方法,通过使用这些潜在的标记物(OX40L、IL-33和TSLP)来区分呼吸道和皮肤致敏剂,但THP-1细胞与支气管上皮细胞的共培养为检测呼吸道致敏剂提供了潜在的有用方法。
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来源期刊
CiteScore
3.80
自引率
3.70%
发文量
60
审稿时长
>18 weeks
期刊介绍: Alternatives to Laboratory Animals (ATLA) is a peer-reviewed journal, intended to cover all aspects of the development, validation, implementation and use of alternatives to laboratory animals in biomedical research and toxicity testing. In addition to the replacement of animals, it also covers work that aims to reduce the number of animals used and refine the in vivo experiments that are still carried out.
期刊最新文献
Development of an In Vitro Sensitisation Test Using a Coculture System of Human Bronchial Epithelium and Immune Cells. Optimisation of a Method for the Differentiation of Human Umbilical Cord-derived Mesenchymal Stem Cells Toward Renal Epithelial-like Cells. Editorial. Resources Round-up. Spotlight on Three Rs Progress.
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