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LC/MS/MS method for analysis of E2 series prostaglandins and isoprostanes

机译:LC / MS / MS方法分析E2系列前列腺素和异前列腺素

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摘要

15-series prostaglandins (PGE2s) and isoprostanes (isoPGE2s) are robust biomarkers of oxidative stress, possess potent biological activity, and may be derived through cyclooxygenase or free radical pathways. Thus, their quantification is critical in understanding many biological processes where PG, isoPG, or oxidative stress are involved. LC/MS/MS methods allow a highly selective, sensitive, simultaneous analysis for prostanoids without derivatization. However, the LC/MS/MS methods currently used do not allow for simultaneous separation of the major brain PGE2/D2 and isoPGE2 without derivatization and multiple HPLC separations. The developed LC/MS/MS method allows for the major brain PGE2/PGD2/isoPGE2 such as PGE2, entPGE2, 8-isoPGE2, 11β-PGE2, PGD2, and 15(R)-PGD2 to be separated and quantified without derivatization. The method was validated by analyzing free and esterified isoPGE2 in mouse brains fixed with head-focused microwave irradiation before or after global ischemia. Using the developed method, we report for the first time the esterified isoPGE2 levels in brain tissue under basal conditions and upon global ischemia and demonstrate a nonreleasable pool of esterified isoPG upon ischemia. In addition, we demonstrated that PGE2s found esterified in the sn-2 position in phospholipids are derived from a free radical nonenzymatic pathway under basal conditions. Our method for brain PG analysis provides a high level of selectivity to detect changes in brain PG and isoPG mass under both basal and pathological conditions.
机译:15系列前列腺素(PGE2s)和异前列腺素(isoPGE2s)是氧化应激的强大生物标志物,具有强大的生物活性,可通过环氧合酶或自由基途径衍生。因此,它们的定量对于理解涉及PG,isoPG或氧化应激的许多生物过程至关重要。 LC / MS / MS方法可对前列腺素进行高度选择性,灵敏的同时分析,而无需衍生化。但是,当前使用的LC / MS / MS方法无法同时分离主要的大脑PGE2 / D2和isoPGE2,而无需衍生化和多次HPLC分离。先进的LC / MS / MS方法可对主要的大脑PGE2 / PGD2 / isoPGE2(例如PGE2,entPGE2、8-isoPGE2、11β-PGE2,PGD2和15(R)-PGD2)进行分离和定量而无需衍生化。该方法通过分析全脑缺血之前或之后用头聚焦微波辐射固定的小鼠大脑中游离和酯化的isoPGE2进行了验证。使用开发的方法,我们首次报告了在基础条件下和局部缺血时脑组织中酯化的isoPGE2水平,并证明了缺血后不可释放的酯化isoPG池。此外,我们证明在碱性条件下,磷脂中sn-2位置被酯化的PGE2来源于自由基的非酶途径。我们的脑PG分析方法可提供高水平的选择性,以检测基础和病理条件下脑PG和isoPG量的变化。

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