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Direct and simultaneous profiling of epoxyeicosatrienoic acid enantiomers by capillary tandem column chiral-phase liquid chromatography with dual online photodiode array and tandem mass spectrometric detection

机译:毛细管串联串联手性液相色谱双在线光电二极管阵列和串联质谱检测法直接和同时分析环氧二十碳三烯酸对映体

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摘要

Despite first evidence for the cytochrome P450-mediated enantioselective biosynthesis and activity of cis-epoxyeicosatrienoic acids (EETs), as yet little is known about the stereospecifity of EET generation and physiology, because the existing chiral methods are time consuming, labor intensive, and not sensitive enough. We present a method for highly sensitive, direct, and simultaneous chiral analysis of all eight EET enantiomers consisting of (i) solid-phase extraction, (ii) reversed-phase high-performance liquid chromatographic purification followed by (iii) consecutive regio- and enantiomeric separation of the four underivatized EET regioisomers within one chromatographic run employing capillary tandem column chiral-phase liquid chromatography with (iv) reliable dual online photodiode array and gentle electrospray ionization tandem mass spectrometric identification and quantitation of the eluting optical antipodes. This one-step, simple, expeditious, and highly sensitive measurement allows profiling of all eight EET enantiomers at once, thus avoiding substance loss and enabling high sample throughput. Limits of quantification in the low picogram range were achieved by the use of capillary columns with typical high quantitative sensitivity instead of conventional columns with low chromatographic signal intensity employed by previous methods. Application to tissue homogenates demonstrated the suitability of this approach for routine and reliable "enantioprofiling" of free endogenous EETs, i.e., EETs not esterified into cellular membrane phospholipids, typically occurring at very low concentrations. The technique can readily be employed for preparative purification of enantiomers in the microgram range using large-inner-diameter columns.
机译:尽管有关于细胞色素P450介导的对映选择性生物合成和顺式-环氧二十碳三烯酸(EETs)活性的第一个证据,但关于EET产生的立体特异性和生理学知之甚少,因为现有的手性方法费时,费力且不足够敏感。我们提出了一种对所有八种EET对映异构体进行高灵敏度,直接和同时手性分析的方法,该方法包括(i)固相萃取,(ii)反相高效液相色谱纯化,然后(iii)连续进行区域和使用毛细管串联串联手性液相色谱与(iv)可靠的双在线光电二极管阵列和温和的电喷雾电离串联质谱鉴定和定量洗脱的光学对映体,在一个色谱运行中对四种未衍生的EET区域异构体的对映异构体分离。这种一步,简单,快速且高度灵敏的测量方法可以一次分析所有8种EET对映异构体,从而避免了物质损失并实现了高样品通量。通过使用具有典型的高定量灵敏度的毛细管色谱柱代替以前方法使用的具有低色谱信号强度的常规色谱柱,可以实现低皮克级定量限。应用于组织匀浆证明了该方法适用于游离内源性EET的常规和可靠的“对映体图”,即未酯化为细胞膜磷脂的EET,通常以非常低的浓度存在。使用大内径色谱柱,该技术可轻松用于微克级对映体的制备纯化。

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