乙醇对胎盘绒毛氧化应激的影响。

Helen H Kay, Stephen Tsoi, Kreg Grindle, Ronald R Magness
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引用次数: 16

摘要

目的:妊娠期乙醇暴露可能导致胎儿酒精综合征(FAS)。这种现象发生的机制尚不清楚。最近对包括胎盘在内的几个器官系统的研究表明,氧化应激与此有关。在这项研究中,我们研究了暴露于乙醇的胎盘绒毛组织中三种氧化应激标志物的存在和水平。方法:将正常胎盘的绒毛组织灌注到含有HEPES缓冲液、碳酸氢钠和pH为7.4的葡萄糖的Dulbeco's modified Eagle's培养基(DMEM)中。稳定后,向灌注液中加入100 mM乙醇。灌注2小时后,取出组织,固定并染色硝基酪氨酸、4-羟基-2-壬烯醛(4HNE)和8-羟基鸟苷(8-OHDG)。用密度测定法定量滋养细胞内的染色。结果:滋养细胞可见硝基酪氨酸和4HNE免疫染色。基质中也可见4HNE。相反,8-OHDG仅在胎儿循环的基质细胞和内皮细胞中可见。乙醇暴露显著增加了滋养细胞中的硝基酪氨酸水平,超过了对照组织中的水平。基质中硝基酪氨酸和8-OHDG水平也升高。结论:短时间乙醇暴露后,胎盘绒毛内滋养细胞和间质中存在氧化应激标志物。氧化应激增加,主要涉及滋养细胞中的一氧化氮途径以及基质中的DNA损伤。脂质过氧化在我们的2小时暴露窗口内没有急剧改变。
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Markers of oxidative stress in placental villi exposed to ethanol.

Objective: Ethanol exposure during pregnancy may result in fetal alcohol syndrome (FAS). The mechanism by which this occurs is unknown. Recent studies in several organ systems, including the placenta, suggest that oxidative stress is involved. In this study we investigated the presence and levels of three oxidative stress markers in placental villous tissue exposed to ethanol.

Methods: Villous tissues from normal placentas were perfused with Dulbeco's modified Eagle's medium (DMEM) with HEPES buffer, sodium bicarbonate, and glucose at pH 7.4. After stabilization, 100 mM ethanol was added to the perfusate. After 2 hours of perfusion, the tissue was removed, fixed and stained for nitrotyrosine, 4-hydroxy-2-nonenal (4HNE) and 8-hydroxyguanosine (8-OHDG). Staining within the trophoblasts was quantified with densitometry.

Results: Nitrotyrosine and 4HNE immunostaining was seen in the trophoblasts. 4HNE was also seen in the stroma. In contrast, 8-OHDG was seen only in the stroma and endothelial cells in the fetal circulation. Ethanol exposure significantly increased nitrotyrosine levels in the trophoblasts beyond levels in the control tissue. Nitrotyrosine and 8-OHDG levels were also increased in stroma.

Conclusion: Within the placental villi, markers of oxidative stress are present in the trophoblasts and stroma after a short period of ethanol exposure. There is an increase in oxidative stress, primarily involving the nitric oxide pathway, in the trophoblasts as well as DNA damage in the stroma. Lipid peroxidation is not acutely changed in our 2-hour exposure window.

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