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有效液相色谱-离子淌度谱-质谱联用分离同分异构脂质物种。

Effective Liquid Chromatography-Trapped Ion Mobility Spectrometry-Mass Spectrometry Separation of Isomeric Lipid Species.

机构信息

Department of Chemistry and Biochemistry , Florida International University , Miami , Florida 33199 , United States.

Department of Chemistry , University of Florida , Gainesville , Florida 32611 , Unites States.

出版信息

Anal Chem. 2019 Apr 16;91(8):5021-5027. doi: 10.1021/acs.analchem.8b04979. Epub 2019 Apr 4.

DOI:10.1021/acs.analchem.8b04979
PMID:30896930
Abstract

Lipids are a major class of molecules that play key roles in different biological processes. Understanding their biological roles and mechanisms remains analytically challenging due to their high isomeric content (e.g., varying acyl chain positions and/or double bond locations/geometries) in eukaryotic cells. In the present work, a combination of liquid chromatography (LC) followed by high resolution trapped ion mobility spectrometry-mass spectrometry (TIMS-MS) was used to investigate common isomeric glycerophosphocholine (PC) and diacylglycerol (DG) lipid species from human plasma. The LC dimension was effective for the separation of isomeric lipid species presenting distinct double bond locations or geometries but was not able to differentiate lipid isomers with distinct acyl chain positions. High resolution TIMS-MS resulted in the identification of lipid isomers that differ in the double bond locations/geometries as well as in the position of the acyl chain with resolving power ( R) up to ∼410 ( R ∼ 320 needed on average). Extremely small structural differences exhibiting collision cross sections (CCS) of less than 1% (down to 0.2%) are sufficient for the discrimination of the isomeric lipid species using TIMS-MS. The same level of performance was maintained in the complex biological mixture for the biologically relevant PC 16:0/18:1 lipid isomers. These results suggest several advantages of using complementary LC-TIMS-MS separations for regular lipidomic analysis, with the main emphasis in the elucidation of isomer-specific lipid biological activities.

摘要

脂质是一类重要的分子,在不同的生物过程中发挥着关键作用。由于真核细胞中脂质具有很高的异构含量(例如,不同的酰基链位置和/或双键位置/几何形状),因此理解它们的生物学作用和机制仍然具有分析挑战性。在本工作中,采用液相色谱(LC)与高分辨囚禁离子淌度质谱联用(TIMS-MS)相结合的方法,从人血浆中研究常见的甘油磷酸胆碱(PC)和二酰基甘油(DG)脂质异构体。LC 维度可有效分离具有不同双键位置或几何形状的异构脂质,但无法区分具有不同酰基链位置的脂质异构体。高分辨 TIMS-MS 可鉴定双键位置/几何形状以及酰基链位置不同的脂质异构体,分辨率( R )高达约 410(平均需要 R ∼ 320)。使用 TIMS-MS 足以区分异构脂质,异构脂质的结构差异极小,其碰撞截面(CCS)小于 1%(低至 0.2%)。在复杂的生物混合物中,对于具有生物学意义的 PC 16:0/18:1 脂质异构体,同样的性能得以保持。这些结果表明,使用互补的 LC-TIMS-MS 分离进行常规脂质组学分析具有多个优势,主要强调阐明异构体特异性脂质的生物学活性。

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