开发一种平行定量蛋白质组学方法,用于检测环氧化酶和脂氧合酶,同时定量分析氧化脂类,从而全面研究花生四烯酸级联反应。

Development of a quantitative proteomics approach for cyclooxygenases and lipoxygenases in parallel to quantitative oxylipin analysis allowing the comprehensive investigation of the arachidonic acid cascade.

机构信息

Chair of Food Chemistry, Faculty of Mathematics and Natural Sciences, University of Wuppertal, Gaußstr. 20, 42119, Wuppertal, Germany.

出版信息

Anal Bioanal Chem. 2023 Feb;415(5):913-933. doi: 10.1007/s00216-022-04489-3. Epub 2023 Jan 23.

Abstract

Oxylipins derived from the cyclooxygenase (COX) and lipoxygenase (LOX) pathways of the arachidonic acid (ARA) cascade are essential for the regulation of the inflammatory response and many other physiological functions. Comprehensive analytical methods comprised of oxylipin and protein abundance analysis are required to fully understand mechanisms leading to changes within these pathways. Here, we describe the development of a quantitative multi-omics approach combining liquid chromatography tandem mass spectrometry-based targeted oxylipin metabolomics and proteomics. As the first targeted proteomics method to cover these pathways, it enables the quantitative analysis of all human COX (COX-1 and COX-2) and relevant LOX pathway enzymes (5-LOX, 12-LOX, 15-LOX, 15-LOX-2, and FLAP) in parallel to the analysis of 239 oxylipins with our targeted oxylipin metabolomics method from a single sample. The detailed comparison between MRM and classical MRM-based detection in proteomics showed increased selectivity for MRM, while MRM performed better in terms of sensitivity (LLOQ, 16-122 pM vs. 75-840 pM for the same peptides), linear range (up to 1.5-7.4 μM vs. 4-368 nM), and multiplexing capacities. Thus, the MRM mode was more favorable for this pathway analysis. With this sensitive multi-omics approach, we comprehensively characterized oxylipin and protein patterns in the human monocytic cell line THP-1 and differently polarized primary macrophages. Finally, the quantification of changes in protein and oxylipin levels induced by lipopolysaccharide stimulation and pharmaceutical treatment demonstrates its usefulness to study molecular modes of action involved in the modulation of the ARA cascade.

摘要

花生四烯酸 (ARA) 级联中环氧化酶 (COX) 和脂氧合酶 (LOX) 途径衍生的氧化脂类对于调节炎症反应和许多其他生理功能至关重要。需要综合的氧化脂和蛋白质丰度分析方法来充分了解导致这些途径变化的机制。在这里,我们描述了一种定量多组学方法的开发,该方法结合了基于液相色谱串联质谱的靶向氧化脂代谢组学和蛋白质组学。作为第一个涵盖这些途径的靶向蛋白质组学方法,它能够同时定量分析所有人类 COX(COX-1 和 COX-2)和相关 LOX 途径酶(5-LOX、12-LOX、15-LOX、15-LOX-2 和 FLAP)以及我们的靶向氧化脂代谢组学方法从单个样本中分析 239 种氧化脂。MRM 和经典基于 MRM 的蛋白质组学检测之间的详细比较表明,MRM 具有更高的选择性,而 MRM 在灵敏度(LLOQ,16-122 pM 与相同肽段的 75-840 pM 相比)、线性范围(高达 1.5-7.4 μM 与 4-368 nM 相比)和多重化能力方面表现更好。因此,MRM 模式更有利于这种途径分析。使用这种灵敏的多组学方法,我们全面描述了人单核细胞系 THP-1 和不同极化的原代巨噬细胞中的氧化脂和蛋白质图谱。最后,定量分析脂多糖刺激和药物处理引起的蛋白质和氧化脂水平的变化,证明了它在研究参与 ARA 级联调节的分子作用模式方面的有用性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f7ea/9883352/20df1d327719/216_2022_4489_Fig1_HTML.jpg

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