Kerwin J L, Tuininga A R, Ericsson L H
Department of Botany, University of Washington, Seattle 98195.
J Lipid Res. 1994 Jun;35(6):1102-14.
This paper describes the use of positive and negative ion electrospray mass spectrometry (MS) and MS/MS (tandem mass spectrometry) to identify glycerophospholipid and ceramide headgroups and their alkyl, alkenyl and acyl constituents. Molecular ion adducts were the primary products formed by positive ionization, occurring as [M+H]+, [M+Na]+, [M+K]+, [M+formate]+, or [M+acetate]+, depending upon the class of glycerophospholipid and the presence or absence of these ionization-promoting species. Similar (negatively charged) ions corresponding to the loss of the groups listed above were formed in negative ion MS. Positive ion electrospray MS/MS provides information on the nature of the headgroup, with the formation of an ion corresponding to the headgroup itself, or the loss of the headgroup from the molecular ion H+ or Na+ adduct. Acyl constituents are identified during negative ion MS/MS from the formation of their RCOO- ions. The nature of alkyl or alkenyl substituents in glycerophosphoethanolamine (PE) molecular species can be identified from residual ions following the loss of ethanolamine plus loss of the acyl moiety in the sn-2 position, and cyclization of a phosphate oxygen with C-2 of glycerol. In glycerophosphoinositol (PI) species, it appears that an RCO- ion is formed during negative ion MS/MS, possibly to steric interference from the bulky phosphoinositol headgroup that prevents cyclization (and subsequent stabilization) of the ion described for PE species. Positive and negative ion electrospray MS spectra for molecular species of commercial preparations of PE, PI, phosphatidylserine (PS), glycerophosphocholine (PC) and sphingomyelin (SM) produced similar profiles. For phospholipids occurring as Na+ adducts, concentrations above ca. 1 ng/microliter produced significant quantities of both [M+H]+ and [M+Na]+ ions for those molecular species present in the largest quantities, complicating interpretation of the spectra. Complete profiles of molecular species were obtained from as little as 10 picograms of material. Major components of PE were identified from 0.1 picogram total lipid. Using single ion monitoring of the Na+ adduct of beta-acetyl-gamma-O-hexadecyl L-alpha-phosphatidylcholine, 10 femtograms of material was detected. A mixture of 1 nanogram each of PE, PI, PS, and PC was readily resolved into individual molecular species, with little apparent loss of resolution or preferential ionization. Electrospray MS did not provide information on the position (sn-1 or sn-2) of fatty acids, and was not capable of differentiating in all instances between alkyl-acyl and alkenyl-acyl substituents without prior separation of these lipid subclasses.(ABSTRACT TRUNCATED AT 400 WORDS)
本文描述了使用正离子和负离子电喷雾质谱(MS)以及串联质谱(MS/MS)来鉴定甘油磷脂和神经酰胺的头部基团及其烷基、烯基和酰基成分。分子离子加合物是正离子化形成的主要产物,根据甘油磷脂的类别以及这些促进电离的物质的存在与否,以[M+H]+、[M+Na]+、[M+K]+、[M+甲酸根]+或[M+乙酸根]+的形式出现。在负离子质谱中形成了与上述基团丢失相对应的类似(带负电荷)离子。正离子电喷雾MS/MS提供了有关头部基团性质的信息,形成了与头部基团本身相对应的离子,或者分子离子H+或Na+加合物中头部基团的丢失。在负离子MS/MS过程中,通过其RCOO-离子的形成来鉴定酰基成分。甘油磷酰乙醇胺(PE)分子物种中烷基或烯基取代基的性质可以从乙醇胺丢失加上sn-2位酰基部分丢失后的残余离子以及磷酸氧与甘油C-2的环化来鉴定。在甘油磷酰肌醇(PI)物种中,在负离子MS/MS过程中似乎形成了一个RCO-离子,这可能是由于庞大的磷酸肌醇头部基团的空间干扰,阻止了PE物种中所述离子的环化(以及随后的稳定)。PE、PI、磷脂酰丝氨酸(PS)、甘油磷酰胆碱(PC)和鞘磷脂(SM)商业制剂分子物种的正离子和负离子电喷雾质谱图产生了相似的图谱。对于以Na+加合物形式存在的磷脂,浓度高于约1 ng/微升时,对于含量最多的那些分子物种会产生大量的[M+H]+和[M+Na]+离子,使光谱的解释变得复杂。从低至10皮克的材料中获得了分子物种的完整图谱。从0.1皮克总脂质中鉴定出了PE的主要成分。使用β-乙酰基-γ-O-十六烷基-L-α-磷脂酰胆碱的Na+加合物的单离子监测,检测到了10飞克的材料。将1纳克的PE、PI、PS和PC的混合物很容易解析为各个分子物种,几乎没有明显的分辨率损失或优先电离。电喷雾质谱没有提供有关脂肪酸位置(sn-1或sn-2)的信息,并且在没有事先分离这些脂质亚类的情况下,并非在所有情况下都能够区分烷基-酰基和烯基-酰基取代基。(摘要截断于400字)
