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使用 [U-C]棕榈酸分析鞘脂类生物合成的串联质谱法时需要考虑的因素。

Factors to consider in using [U-C]palmitate for analysis of sphingolipid biosynthesis by tandem mass spectrometry.

机构信息

Newborn Screening and Molecular Biology Branch, Centers for Disease Control and Prevention, Atlanta, GA, USA.

出版信息

J Lipid Res. 2011 Aug;52(8):1583-94. doi: 10.1194/jlr.D015586. Epub 2011 May 17.

Abstract

This study describes the use of a stable-isotope labeled precursor ([U-¹³C]palmitate) to analyze de novo sphingolipid biosynthesis by tandem mass spectrometry. It also describes factors to consider in interpreting the data, including the isotope's location (¹³C appears in three isotopomers and isotopologues: [M + 16] for the sphingoid base or N-acyl fatty acid, and [M + 32] for both); the isotopic enrichment of palmitoyl-CoA; and its elongation, desaturation, and incorporation into N-acyl-sphingolipids. For HEK293 cells incubated with 0.1 mM [U-¹³C]palmitic acid, ∼60% of the total palmitoyl-CoA was ¹³C-labeled by 3 h (which was near isotopic equilibrium); with this correction, the rates of de novo biosynthesis of C16:0-ceramide, C16:0-monohexosylceramide, and C16:0-sphingomyelins were 62 ± 3, 13 ± 2, and 60 ± 11 pmol/h per mg protein, respectively, which are consistent with an estimated rate of appearance of C16:0-ceramide using exponential growth modeling (119 ± 11 pmol/h per mg protein). Including estimates for the very long-chain fatty acyl-CoAs, the overall rate of sphingolipid biosynthesis can be estimated to be at least ∼1.6-fold higher. Thus, consideration of these factors gives a more accurate picture of de novo sphingolipid biosynthesis than has been possible to-date, while acknowledging that there are inherent limitations to such approximations.

摘要

本研究采用稳定同位素标记前体 ([U-¹³C]棕榈酸),通过串联质谱分析从头合成鞘脂的生物合成。还描述了在解释数据时需要考虑的因素,包括同位素的位置 (¹³C 出现在三种同位素异形体和同位素标记物中:[M + 16] 是鞘氨醇碱基或 N-酰基脂肪酸,[M + 32] 是两者);棕榈酰-CoA 的同位素丰度;以及其延伸、去饱和和掺入 N-酰基鞘脂。对于用 0.1 mM [U-¹³C]棕榈酸孵育的 HEK293 细胞,约 60%的总棕榈酰-CoA 在 3 小时内被 ¹³C 标记(接近同位素平衡);通过这种校正,C16:0-神经酰胺、C16:0-单己糖神经酰胺和 C16:0-神经鞘磷脂的从头生物合成速率分别为 62 ± 3、13 ± 2 和 60 ± 11 pmol/h/mg 蛋白,这与使用指数增长模型估计的 C16:0-神经酰胺出现率一致(119 ± 11 pmol/h/mg 蛋白)。包括非常长链脂肪酸酰基-CoA 的估计值,鞘脂生物合成的总速率至少可以估计为约 1.6 倍。因此,考虑这些因素可以更准确地描述从头合成鞘脂的生物合成,而不是迄今为止可能的情况,同时承认这种近似存在固有局限性。

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