[HTML][HTML] Improved method of plasma 8-Isoprostane measurement and association analyses with habitual drinking and smoking
S Kitano, H Hisatomi, N Hibi, K Kawano… - World Journal of …, 2006 - ncbi.nlm.nih.gov
S Kitano, H Hisatomi, N Hibi, K Kawano, S Harada
World Journal of Gastroenterology: WJG, 2006•ncbi.nlm.nih.govAIM: 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 …
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 …
Abstract
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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