Lu Wenyun, Kwon Yun Kyung, Rabinowitz Joshua D
Department of Chemistry and Lewis-Sigler Institute for Integrative Genomics, Princeton University, Princeton, New Jersey, USA.
J Am Soc Mass Spectrom. 2007 May;18(5):898-909. doi: 10.1016/j.jasms.2007.01.017. Epub 2007 Mar 23.
Folate metabolism, which is responsible for one-carbon transfer reactions in critical cellular processes including thymidine biosynthesis, is among the most important targets of antibiotic and anticancer drugs. Analysis of intracellular folates is complicated by three different types of folate modification: oxidation/reduction, methylation, and polyglutamylation. Here we present a method for quantifying the full diversity of intracellular folates by liquid chromatography-tandem mass spectrometry (LC-MS/MS). The method begins with folate extraction using -75 degrees C methanol:water, with ascorbic acid and ammonium acetate added to prevent folate interconversion. The extract is then separated using hydrophilic interaction chromatography with an amino column, ionized by positive mode electrospray, and analyzed on a triple quadrupole instrument using multiple reaction monitoring. The method has been used to profile the folate pools in Escherichia coli and Saccharomyces cerevisiae, with absolute levels of selected folates in E. coli measured by spiking extracts of cells fed uniformly (13)C-glucose with purified, unlabeled folate standards. An isotope-ratio-based approach has been applied to study the effects of trimethoprim, a clinically important antibiotic that blocks bacterial dihydrofolate reductase. In addition to causing the expected increase in oxidized and decrease in reduced folates, trimethoprim triggered a dramatic and previously unrecognized shift towards shorter polyglutamate chain lengths. This finding highlights the potential for analysis of the full spectrum of cellular folates by MS/MS to unveil novel biological phenomena.
叶酸代谢负责包括胸苷生物合成在内的关键细胞过程中的一碳转移反应,是抗生素和抗癌药物最重要的靶点之一。细胞内叶酸的分析因三种不同类型的叶酸修饰而变得复杂:氧化/还原、甲基化和多聚谷氨酸化。在此,我们提出了一种通过液相色谱-串联质谱(LC-MS/MS)对细胞内叶酸的全部多样性进行定量的方法。该方法首先使用-75℃的甲醇:水进行叶酸提取,并添加抗坏血酸和醋酸铵以防止叶酸相互转化。然后,提取物通过氨基柱进行亲水相互作用色谱分离,通过正模式电喷雾电离,并在三重四极杆仪器上使用多反应监测进行分析。该方法已用于分析大肠杆菌和酿酒酵母中的叶酸池,通过向均匀喂食(13)C-葡萄糖的细胞提取物中加入纯化的未标记叶酸标准品来测量大肠杆菌中选定叶酸的绝对水平。一种基于同位素比率的方法已被应用于研究甲氧苄啶的作用,甲氧苄啶是一种临床上重要的抗生素,可阻断细菌二氢叶酸还原酶。除了导致预期的氧化叶酸增加和还原叶酸减少外,甲氧苄啶还引发了向较短多聚谷氨酸链长度的显著且此前未被认识到的转变。这一发现凸显了通过MS/MS分析细胞叶酸全谱以揭示新生物现象的潜力。