氮芥诱导的角膜损伤涉及DNA损伤以及与炎症、上皮-基质分离和新生血管形成相关的信号通路。
Nitrogen Mustard-Induced Corneal Injury Involves DNA Damage and Pathways Related to Inflammation, Epithelial-Stromal Separation, and Neovascularization.
作者信息
Goswami Dinesh G, Tewari-Singh Neera, Dhar Deepanshi, Kumar Dileep, Agarwal Chapla, Ammar David A, Kant Rama, Enzenauer Robert W, Petrash J Mark, Agarwal Rajesh
机构信息
Departments of *Pharmaceutical Sciences; and †Ophthalmology, University of Colorado Anschutz Medical Campus, Aurora, CO.
出版信息
Cornea. 2016 Feb;35(2):257-66. doi: 10.1097/ICO.0000000000000685.
PURPOSE
To evaluate the toxic effects and associated mechanisms in corneal tissue exposed to the vesicating agent, nitrogen mustard (NM), a bifunctional alkylating analog of the chemical warfare agent sulfur mustard.
METHODS
Toxic effects and associated mechanisms were examined in maximally affected corneal tissue using corneal cultures and human corneal epithelial (HCE) cells exposed to NM.
RESULTS
Analysis of ex vivo rabbit corneas showed that NM exposure increased apoptotic cell death, epithelial thickness, epithelial-stromal separation, and levels of vascular endothelial growth factor, cyclooxygenase 2, and matrix metalloproteinase-9. In HCE cells, NM exposure resulted in a dose-dependent decrease in cell viability and proliferation, which was associated with DNA damage in terms of an increase in p53 ser15, total p53, and H2A.X ser139 levels. NM exposure also induced caspase-3 and poly ADP ribose polymerase cleavage, suggesting their involvement in NM-induced apoptotic death in the rabbit cornea and HCE cells. Similar to rabbit cornea, NM exposure caused an increase in cyclooxygenase 2, matrix metalloproteinase-9, and vascular endothelial growth factor levels in HCE cells, indicating a role of these molecules and related pathways in NM-induced corneal inflammation, epithelial-stromal separation, and neovascularization. NM exposure also induced activation of activator protein 1 transcription factor proteins and upstream signaling pathways including mitogen-activated protein kinases and Akt protein kinase, suggesting that these could be key factors involved in NM-induced corneal injury.
CONCLUSIONS
Results from this study provide insight into the molecular targets and pathways that could be involved in NM-induced corneal injuries laying the background for further investigation of these pathways in vesicant-induced ocular injuries, which could be helpful in the development of targeted therapies.
目的
评估角膜组织暴露于发泡剂氮芥(NM)(化学战剂硫芥的双功能烷基化类似物)后的毒性作用及相关机制。
方法
使用角膜培养物和暴露于NM的人角膜上皮(HCE)细胞,在受影响最大的角膜组织中检测毒性作用及相关机制。
结果
对离体兔角膜的分析表明,暴露于NM会增加凋亡细胞死亡、上皮厚度、上皮-基质分离以及血管内皮生长因子、环氧合酶2和基质金属蛋白酶-9的水平。在HCE细胞中,暴露于NM导致细胞活力和增殖呈剂量依赖性下降,这与DNA损伤有关,表现为p53丝氨酸15、总p53和H2A.X丝氨酸139水平升高。NM暴露还诱导了半胱天冬酶-3和聚ADP核糖聚合酶的裂解,表明它们参与了NM诱导的兔角膜和HCE细胞凋亡死亡。与兔角膜相似,NM暴露导致HCE细胞中环氧合酶2、基质金属蛋白酶-9和血管内皮生长因子水平升高,表明这些分子及相关途径在NM诱导的角膜炎症、上皮-基质分离和新生血管形成中起作用。NM暴露还诱导了激活蛋白1转录因子蛋白和上游信号通路(包括丝裂原活化蛋白激酶和Akt蛋白激酶)的激活,表明这些可能是参与NM诱导角膜损伤的关键因素。
结论
本研究结果深入了解了可能参与NM诱导角膜损伤的分子靶点和途径,为进一步研究这些途径在发泡剂诱导眼损伤中的作用奠定了基础,这可能有助于开发靶向治疗方法。
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