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通过镥标记和纳升液相色谱-电感耦合等离子体质谱联用及同位素稀释分析进行绝对肽定量

Absolute peptide quantification by lutetium labeling and nanoHPLC-ICPMS with isotope dilution analysis.

作者信息

Rappel Christina, Schaumlöffel Dirk

机构信息

Laboratoire de Chimie Analytique Bio-Inorganique et Environnement, CNRS UMR 5254, Helioparc, 2 av. Pr. Angot, F-64053 Pau, France.

出版信息

Anal Chem. 2009 Jan 1;81(1):385-93. doi: 10.1021/ac801814a.

DOI:10.1021/ac801814a
PMID:19117464
Abstract

The need of analytical methods for absolute quantitative protein analysis spurred research on new developments in recent years. In this work, a novel approach was developed for accurate absolute peptide quantification based on metal labeling with lutetium diethylenetriamine pentaacetic acid (Lu-DTPA) and nanoflow high-performance liquid chromatography-inductively coupled plasma isotope dilution mass spectrometry (nanoHPLC-ICP-IDMS). In a two-step procedure peptides were derivatized at amino groups with diethylenetriamine pentaacetic anhydride (DTPAA) followed by chelation of lutetium. Electrospray ionization mass spectrometry (ESI MS) of the reaction product demonstrated highly specific peptide labeling. Under optimized nanoHPLC conditions the labeled peptides were baseline-separated, and the excess labeling reagent did not interfere. A 176Lu-labeled spike was continuously added to the column effluent for quantification by ICP-IDMS. The recovery of a Lu-DTPA-labeled standard peptide was close to 100% indicating high labeling efficiency and accurate absolute quantification. The precision of the entire method was 4.9%. The detection limit for Lu-DTPA-tagged peptides was 179 amol demonstrating that lutetium-specific peptide quantification was by 4 orders of magnitude more sensitive than detection by natural sulfur atoms present in cysteine or methionine residues. Furthermore, the application to peptides in insulin tryptic digest allowed the identification of interfering reagents decreasing the labeling efficiency. An additional advantage of this novel approach is the analysis of peptides, which do not naturally feature ICPMS-detectable elements.

摘要

近年来,对蛋白质绝对定量分析方法的需求推动了相关新进展的研究。在这项工作中,开发了一种基于镥二乙烯三胺五乙酸(Lu-DTPA)金属标记和纳流高效液相色谱-电感耦合等离子体质谱同位素稀释质谱法(nanoHPLC-ICP-IDMS)的准确绝对肽定量新方法。在两步法中,肽首先用二乙烯三胺五乙酸酐(DTPAA)在氨基上进行衍生化,然后与镥螯合。反应产物的电喷雾电离质谱(ESI MS)显示了高度特异性的肽标记。在优化的nanoHPLC条件下,标记的肽实现了基线分离,且过量的标记试剂不产生干扰。通过连续向柱流出物中添加176Lu标记的内标进行ICP-IDMS定量。Lu-DTPA标记的标准肽回收率接近100%,表明标记效率高且绝对定量准确。整个方法的精密度为4.9%。Lu-DTPA标记肽的检测限为179 amol,这表明镥特异性肽定量比通过半胱氨酸或甲硫氨酸残基中天然存在的硫原子检测灵敏4个数量级。此外,该方法应用于胰岛素胰蛋白酶消化后的肽分析,可鉴定出降低标记效率的干扰试剂。这种新方法的另一个优点是能够分析天然不含有ICP-MS可检测元素的肽。

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