Department of Chemistry and Biochemistry, Saint Louis University, 3501 Laclede Avenue, St. Louis, Missouri 63103, United States.
Edward A. Doisy Department of Biochemistry and Molecular Biology and Center for Cardiovascular Research, Saint Louis University School of Medicine, St. Louis, Missouri 63104, United States.
J Am Soc Mass Spectrom. 2024 Jul 3;35(7):1403-1412. doi: 10.1021/jasms.3c00447. Epub 2024 Jun 13.
Multiplexing of phosphatidylcholine analysis is hindered by a lack of appropriate derivatization. Presented here is a tagging scheme that uses a quaternary amine tag and targets the hydroxy group of the phosphate, which switches the net charge from neutral to +2. Quantitative yields were achieved from >99% reaction completion derived by dimethoxymethyl morpholinium (DMTMM) activation. Fragmentation of phosphatidylcholines (PCs) and lysophosphatidylcholines (LPCs) releases two trimethylamines and the acyl chains through neutral loss and generates a unique double cyclization constant mass reporter. Selective incorporation of isotopes onto the tag produces a six-plex set of isobaric reagents. For equivalent six-plex-labeled samples, <14% RSD was achieved, followed by a dynamic range of 1:10 without signal compression. Quantification of PCs/LPCs in human hepatic cancer cells was conducted as six-plex using data-dependent analysis tandem MS. We report a six-plex qualitative and quantitative isobaric tagging strategy expanding the limits of analyzing PCs/LPCs.
多相膦脂酸分析受到缺乏适当衍生化的阻碍。本文提出了一种标记方案,该方案使用季铵标签并针对磷酸酯的羟基,这将净电荷从中性变为+2。通过二甲氧基甲基吗啉鎓(DMTMM)激活,实现了定量收率> 99%的反应完成。膦脂酸(PC)和溶血膦脂酸(LPC)的断裂通过中性损失释放两个三甲胺和酰基链,并产生独特的双环化恒定质量报告。将同位素选择性掺入标签中可产生六重同位素质谱试剂。对于等效的六重标记样品,实现了<14%的 RSD,随后在没有信号压缩的情况下动态范围为 1:10。使用基于数据的分析串联质谱法对人肝癌细胞中的 PC/LPC 进行了六重定量分析。我们报告了一种六重定性和定量的等压标记策略,扩展了分析 PC/LPC 的限制。
