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Capillary electrophoresis of cytochrome P-450 epoxygenase metabolites of arachidonic acid. 1. Resolution of regioisomers

机译:花生四烯酸的细胞色素P-450环氧酶代谢产物的毛细管电泳。 1.区域异构体的拆分

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The essential fatty acid arachidonate is oxidized by cytochrome P-450 epoxygenases to four epoxyeicosatrienoic acids (EETs): 14,15-, 11,12-, 8,9-, and 5,6-EETs. Each of the four EET regioisomers and their hydrolysis products (DHETs) has multiple paracrine and autocrine functions and may also potently dilate blood vessels and activate potassium channels. The present work describes a method to resolve EETs and DHETs by capillary electrophoresis (CE) using trimethyl-beta-cyclodextrin and CH3CN as buffer additives. While stored at 25 degreesC, most of the EET and DHET regioisomers remained intact when suspended in alkaline vehicle. However, under these same conditions, 5,6-EET rapidly broke down to a lactone and was slowly converted to 5,6-DHET. When subjected to CE, the EET and DHET regioisomers were baseline resolved (R greater than or equal to 1.3); 10 pg of an EET or a DHET regioisomer was readily detectable at 194 nm. In addition, the UV spectra were regiospecific and identical to those obtained during HPLC except that an additional, weak absorption occurred at 235 nm. Together, the high-sensitivity, high-resolution, and differential UV spectra permitted the identification and quantification of EETs in phospholipids isolated from murine liver. Thus, CE was successfully used for the trace analysis of eicosanoids. [References: 30]
机译:必需脂肪酸花生四烯酸酯被细胞色素P-450环氧合酶氧化为四种环氧二十碳三烯酸(EET):14,15-,11,12-,8,9-和5,6-EET。四种EET区域异构体及其水解产物(DHET)均具有多种旁分泌和自分泌功能,还可能有效扩张血管并激活钾通道。本工作描述了一种使用三甲基-β-环糊精和CH3CN作为缓冲添加剂通过毛细管电泳(CE)拆分EET和DHET的方法。当储存在25摄氏度时,大多数EET和DHET区域异构体悬浮在碱性介质中仍保持完整。然而,在这些相同条件下,5,6-EET迅速分解为内酯,并缓慢转化为5,6-DHET。接受CE时,EET和DHET区域异构体被基线拆分(R大于或等于1.3);在194 nm处很容易检测到10 pg的EET或DHET区域异构体。此外,UV光谱具有区域专一性,与HPLC中获得的光谱相同,只是在235 nm处发生了另外的弱吸收。高灵敏度,高分辨率和不同的紫外光谱共同实现了对从鼠肝分离的磷脂中EET的鉴定和定量。因此,CE成功地用于类二十烷酸的痕量分析。 [参考:30]

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