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建立常规液相色谱-质谱法检测血液中酒精生物标志物磷酰乙醇(PEth)的方法。

Method development for routine liquid chromatography-mass spectrometry measurement of the alcohol biomarker phosphatidylethanol (PEth) in blood.

机构信息

Alcohol Laboratory, Department of Laboratory Medicine, Karolinska Institutet, Stockholm, Sweden.

出版信息

Clin Chim Acta. 2011 Jul 15;412(15-16):1428-35. doi: 10.1016/j.cca.2011.04.022. Epub 2011 Apr 19.

Abstract

BACKGROUND

Phosphatidylethanol (PEth) is a group of phospholipids formed from ethanol and phosphatidylcholine by action of phospholipase D. Measurement of PEth in whole blood samples is employed as an alcohol biomarker. This work aimed to further develop an LC-MS method for PEth to make it practical for routine laboratory use.

METHODS

Blood samples were obtained from blood donors and from the clinical samples pool. A whole blood total lipid extract was separated on a C4 column, followed by ESI-MS detection of the deprotonated molecules in SIM mode or ESI-MS/MS detection of the major product ions (fatty acid fragments) by SRM.

RESULTS

Initial results indicated that individual calibration curves are required for MS quantitation of some PEth forms, and that deuterated analogs are preferable over phosphatidylpropanol as the internal standard. PEth-16:0/18:1 was the single most sensitive molecular form as alcohol biomarker, being detected in every of 211 blood specimens containing 0.1-20 μmol/L total PEth at reporting limits in the range 0.1-1.0 μmol/L. PEth-16:0/18:1 and 16:0/18:2, accounting for about 36% and 26%, respectively, of the total amount, correlated well with total PEth (R(2)=0.922-0.940), but the correlation was better for the sum of both forms (R(2)=0.994). Based on analysis of specimens from 200 blood donors, 95% reference intervals (CLSI C28-A3) were estimated to be <0.70 μmol/L for total PEth, <0.20 μmol/L for PEth-16:0/18:1, and <0.18 μmol/L for PEth-16:0/18:2.

CONCLUSIONS

The LC-ESI-MS(/MS) method allowed for simultaneous qualitative and quantitative measurements of PEth forms in whole blood samples. Related to the routine application of blood PEth as alcohol biomarker, reference intervals were suggested for total PEth and the major molecular forms PEth-16:0/18:1 and 16:0/18:2.

摘要

背景

磷脂酰乙醇(PEth)是由乙醇和磷脂酰胆碱在磷脂酶 D 的作用下形成的一组磷脂。全血样本中 PEth 的测量被用作酒精生物标志物。本工作旨在进一步开发 LC-MS 方法来测定 PEth,使其适用于常规实验室使用。

方法

从献血者和临床样本库中采集血样。全血总脂质提取物在 C4 柱上分离,然后以 SIM 模式对去质子化分子进行 ESI-MS 检测,或通过 SRM 对主要产物离子(脂肪酸片段)进行 ESI-MS/MS 检测。

结果

初步结果表明,对于某些 PEth 形式的 MS 定量需要单独的校准曲线,并且氘代类似物比磷脂丙醇作为内标更可取。PEth-16:0/18:1 是作为酒精生物标志物最敏感的单一分子形式,在报告限为 0.1-1.0 μmol/L 的范围内,在包含 0.1-20 μmol/L 总 PEth 的 211 个血样中均能检测到。PEth-16:0/18:1 和 16:0/18:2 分别占总量的约 36%和 26%,与总 PEth 相关性良好(R²=0.922-0.940),但两种形式之和的相关性更好(R²=0.994)。基于 200 名献血者标本的分析,总 PEth 的 95%参考区间(CLSI C28-A3)估计为<0.70 μmol/L,PEth-16:0/18:1 为<0.20 μmol/L,PEth-16:0/18:2 为<0.18 μmol/L。

结论

LC-ESI-MS(/MS) 方法允许同时对全血样本中的 PEth 形式进行定性和定量测量。与血液 PEth 作为酒精生物标志物的常规应用相关,建议为总 PEth 以及主要分子形式 PEth-16:0/18:1 和 16:0/18:2 建立参考区间。

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