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接触特定的柠檬烯氧化产物:4-氧代对孟烷、对异丙基苯过氧化氢、4-(对甲苯磺酰氧基)-2-甲基-2-己烯醛会在人肺上皮细胞系中引发氧化应激和炎症。

Exposure to selected limonene oxidation products: 4-OPA, IPOH, 4-AMCH induces oxidative stress and inflammation in human lung epithelial cell lines.

作者信息

Lipsa Dorelia, Barrero-Moreno Josefa, Coelhan Mehmet

机构信息

Technische Universität München, Research Center Weihenstephan for Brewing and Food Quality, Alte Akademie 3, Freising-Weihenstephan, Germany; European Commission, DG Joint Research Centre, Ispra, Italy.

European Commission, DG Joint Research Centre, Ispra, Italy.

出版信息

Chemosphere. 2018 Jan;191:937-945. doi: 10.1016/j.chemosphere.2017.10.065. Epub 2017 Oct 11.

Abstract

Limonene oxidation products (LOPs) have gained interest on their harmful health effects over time. Recently, studies have shown that the selected LOPs: 4-oxopentanal (4-OPA), 3-isopropenyl-6-oxo-heptanal (IPOH) and 4-acetyl-1-methylcyclohexene (4-AMCH) have sensory irritation effects in mice and inflammatory effects in human lung cells. This study was therefore undertaken to investigate the potential capacity of 4-OPA, IPOH and 4-AMCH to cause cell membrane damage, oxidative stress and inflammation in human bronchial (16HBE14o-) and alveolar (A549) epithelial cell lines. Overall results suggest that 4-OPA, IPOH have cytotoxic effects on human lung cells that might be mediated by ROS: the highest concentration applied of IPOH [500 μM] enhanced ROS generation by 100-fold ± 7.7 (A549) and 230-fold ± 19.9 (16HBE14o-) compared to the baseline. 4-OPA [500 μM] increased ROS levels by 1.4-fold ± 0.3 (A549) and by 127-fold ± 10.5 (16HBE14o-), while treatment with 4-AMCH [500 μM] led to 0.9-fold ± 0.2 (A549) and 49-fold ± 12.8 (16HBE14o-) increase. IPOH [500 μM] caused a decrease in the thiol-state balance (e.g. after 2 h, GSH:GSSG was reduced by 37% compared to the untreated 16HBE14o-cells). 4-OPA [500 μM] decreased the GSH:GSSG by 1.3-fold change in A549 cells and 1.4-fold change in 16HBE14o-cells. No statistically significant decrease in the GSH:GSSG in A549 and 16HBE14o-cell lines was observed for 4-AMCH [500 μM]. In addition, IPOH and 4-OPA [31.2 μM] increased the amount of the inflammatory markers: RANTES, VEGF and EGF. On the other hand, 4-AMCH [31.2 μM] did not show inflammatory effects in A549 or 16HBE14o-cells. The 4-OPA, IPOH and 4-AMCH treatment concentration and time-dependently induce oxidative stress and/or alteration of inflammatory markers on human bronchial and alveolar cell lines.

摘要

随着时间的推移,柠檬烯氧化产物(LOPs)因其对健康的有害影响而受到关注。最近的研究表明,选定的LOPs:4-氧代戊醛(4-OPA)、3-异丙烯基-6-氧代庚醛(IPOH)和4-乙酰基-1-甲基环己烯(4-AMCH)对小鼠有感官刺激作用,对人肺细胞有炎症作用。因此,本研究旨在调查4-OPA、IPOH和4-AMCH在人支气管(16HBE14o-)和肺泡(A549)上皮细胞系中引起细胞膜损伤、氧化应激和炎症的潜在能力。总体结果表明,4-OPA、IPOH对人肺细胞具有细胞毒性作用,并可能由活性氧(ROS)介导:与基线相比,IPOH施加的最高浓度[500μM]使A549细胞中ROS生成增加了100倍±7.7,16HBE14o-细胞中增加了230倍±19.9。4-OPA[500μM]使A549细胞中ROS水平增加了1.4倍±0.3,16HBE14o-细胞中增加了127倍±10.5,而用4-AMCH[500μM]处理导致A549细胞中增加了0.9倍±0.2,16HBE14o-细胞中增加了49倍±12.8。IPOH[500μM]导致硫醇状态平衡下降(例如,2小时后,与未处理的16HBE14o-细胞相比,谷胱甘肽(GSH)与氧化型谷胱甘肽(GSSG)的比例降低了37%)。4-OPA[500μM]使A549细胞中GSH:GSSG降低了1.3倍,16HBE14o-细胞中降低了1.4倍。对于4-AMCH[500μM],在A549和16HBE14o-细胞系中未观察到GSH:GSSG有统计学意义的下降。此外,IPOH和4-OPA[31.2μM]增加了炎症标志物:调节激活正常T细胞表达和分泌因子(RANTES)、血管内皮生长因子(VEGF)和表皮生长因子(EGF)的量。另一方面,4-AMCH[31.2μM]在A549或16HBE14o-细胞中未显示出炎症作用。4-OPA、IPOH和4-AMCH的处理浓度和时间依赖性地诱导人支气管和肺泡细胞系中的氧化应激和/或炎症标志物改变。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/374c/5701770/28737feca696/egi10GH6H5P1JJ.jpg

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