AIM:To develop a simple and accurate method for quantifying 8-isoprostane in plasma by employing a combination of two-step solid-phase extraction of samples and a commercially available ELISA kit, and by this method to examine the effects of drinking and smoking habits against the levels of plasma 8-isoprostane in healthy Japanese volunteers.
METHODS:Plasma 8-isoprostane was extracted with ODS gel suspension followed by NH(2) Sep-Pak column. The 8-isoprostane fractions were assayed using a commercially available ELISA kit. We measured plasma 8-isoprostane levels in 157 healthy Japanese volunteers divided into three groups (64 non-habitual drinkers, 56 moderate drinkers and 37 habitual drinkers) according to their alcohol consumption per week. Genotypes of aldehyde dehydrogenase 2 (ALDH2) were also determined to investigate the plasma 8-isoprostane levels with reference to drinking habits. In addition, the plasma 8-isoprostane levels of 96 non-smokers and 61 smokers from the same subjects were compared.
RESULTS:Our method fulfilled all the requirements for use in routine clinical assays with respect to sensitivity, intra- and inter-assay reproducibility, accuracy and dynamic assay range. Significant increases of plasma 8-isoprostane levels were observed in female habitual drinkers when compared with those of non-habitual drinkers (t = 5.494, P<0.0001) as well as moderate drinkers (t = 3.542, P<0.005), and 8-isoprostane levels were also significantly different between ALDH2*2/1 and ALDH2*1/1 in the female habitual drinkers (t = 6.930, P<0.0001), suggesting that excessive drinking of alcohol may increase oxidization stress, especially in females. On the contrary, no significant difference of the plasma 8-isoprostane levels was observed between non-smokers and smokers.
CONCLUSION:Our present method was proved to be a simple and accurate tool for measuring plasma 8-isoprostane. However, the clinical utility of plasma 8-isoprostane for drinking and smoking habits was limited since elevated 8-isoprostane levels were observed in female heavy drinkers, and no association was found between smokers and nonsmokers.
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【Improved method of plasma 8-Isoprostane measurement and association analyses with habitual drinking and smoking.].
【血浆8-异前列腺素的测量方法的改进以及与惯常饮酒和吸烟的关联分析。】
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DOI:10.3748/wjg.v12.i36.5846文章类型:杂志文章
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目的:通过结合两步固相萃取样品和市售ELISA试剂盒,开发一种简单,准确的定量血浆中8-异前列腺素的方法,并以此方法检查饮酒和吸烟习惯的影响健康的日本志愿者中血浆8-异前列腺素水平的变化。
方法:用ODS凝胶悬浮液,然后用NH(2)Sep-Pak柱提取血浆8-异前列腺素。使用市售ELISA试剂盒测定8-异前列腺素级分。我们根据每周的酒精摄入量,对157名健康的日本志愿者的血浆8-异前列腺素水平进行了测量,这些志愿者分为三组(64名非习惯性饮酒者,56名中度饮酒者和37名习惯性饮酒者)。还确定了醛脱氢酶2(ALDH2)的基因型,以参考饮酒习惯研究血浆8-异前列腺素水平。此外,比较了来自同一受试者的96名非吸烟者和61名吸烟者的血浆8-异前列腺素水平。
结果:我们的方法满足了常规临床测定中灵敏度,测定内和测定间重现性,准确性和动态测定范围的所有要求。与非惯常饮酒者(t = 5.494,P <0.0001)和中度饮酒者(t = 3.542,P <0.005)和8-习惯饮酒者相比,女性惯常饮酒者血浆8-异前列腺素水平显着增加。在女性习惯性饮酒者中,ALDH2 * 2/1和ALDH2 * 1/1之间的异前列腺素水平也存在显着差异(t = 6.930,P <0.0001),这表明过量饮酒可能会增加氧化应激,尤其是女性。相反,在非吸烟者和吸烟者之间未观察到血浆8-异前列腺素水平的显着差异。
结论:我们的现有方法被证明是一种简单而准确的测量血浆8-异前列腺素的工具。但是,血浆8-异前列腺素在饮酒和吸烟习惯中的临床应用受到限制,因为在女性大量饮酒者中观察到8-异前列腺素水平升高,并且在吸烟者和不吸烟者之间未发现关联。
方法:用ODS凝胶悬浮液,然后用NH(2)Sep-Pak柱提取血浆8-异前列腺素。使用市售ELISA试剂盒测定8-异前列腺素级分。我们根据每周的酒精摄入量,对157名健康的日本志愿者的血浆8-异前列腺素水平进行了测量,这些志愿者分为三组(64名非习惯性饮酒者,56名中度饮酒者和37名习惯性饮酒者)。还确定了醛脱氢酶2(ALDH2)的基因型,以参考饮酒习惯研究血浆8-异前列腺素水平。此外,比较了来自同一受试者的96名非吸烟者和61名吸烟者的血浆8-异前列腺素水平。
结果:我们的方法满足了常规临床测定中灵敏度,测定内和测定间重现性,准确性和动态测定范围的所有要求。与非惯常饮酒者(t = 5.494,P <0.0001)和中度饮酒者(t = 3.542,P <0.005)和8-习惯饮酒者相比,女性惯常饮酒者血浆8-异前列腺素水平显着增加。在女性习惯性饮酒者中,ALDH2 * 2/1和ALDH2 * 1/1之间的异前列腺素水平也存在显着差异(t = 6.930,P <0.0001),这表明过量饮酒可能会增加氧化应激,尤其是女性。相反,在非吸烟者和吸烟者之间未观察到血浆8-异前列腺素水平的显着差异。
结论:我们的现有方法被证明是一种简单而准确的测量血浆8-异前列腺素的工具。但是,血浆8-异前列腺素在饮酒和吸烟习惯中的临床应用受到限制,因为在女性大量饮酒者中观察到8-异前列腺素水平升高,并且在吸烟者和不吸烟者之间未发现关联。
