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白蛋白-Cys34加合物的抗体富集与质谱分析。

Antibody enrichment and mass spectrometry of albumin-Cys34 adducts.

作者信息

Chung Ming-Kei, Grigoryan Hasmik, Iavarone Anthony T, Rappaport Stephen M

机构信息

Center for Exposure Biology, School of Public Health, University of California , Berkeley, California 94720, United States.

出版信息

Chem Res Toxicol. 2014 Mar 17;27(3):400-7. doi: 10.1021/tx400337k. Epub 2013 Dec 24.

DOI:10.1021/tx400337k
PMID:24328277
Abstract

Untargeted analyses of tryptic peptides of human serum albumin (HSA) have been used to investigate unknown exposures to reactive electrophiles (adductomics). To reduce the complexity of the analytical matrix and thereby enhance identification of adducts by liquid chromatography-high-resolution mass spectrometry (LC-HRMS), a polyclonal anti-T3 antibody was designed to capture Cys34 adducts in tryptic digests of HSA (T3 is the third largest tryptic peptide). Epitopes were selected from sequences at both C- and N-termini based on the three-dimensional structure of the T3 peptide to minimize the influence of modified Cys34 residues. The assay was simplified by attaching magnetic beads to the anti-T3 antibody. When applied to commercial HSA and to plasma samples from healthy humans and analyzed by LC-HRMS, antibody treatment greatly reduced the background of non-T3 peptides in the sample matrix. Although other lipophilic HSA peptides were still present, presumably due to nonspecific binding to the antibody-magnetic-bead surfaces, their concentrations in antibody-treated samples were reduced about 6-fold compared to the same samples that had not been treated with the antibody. Analysis of antibody-enriched HSA digests from human plasma samples revealed 10 modified T3 peptides of which 8 were identified from accurate masses. Identified peptides included Cys34 oxidation and cysteinylation products and modifications representing losses of water and Lys and transpeptidation of Arg.

摘要

人血清白蛋白(HSA)胰蛋白酶解肽段的非靶向分析已被用于研究对活性亲电试剂的未知暴露情况(加合物组学)。为了降低分析基质的复杂性,从而通过液相色谱-高分辨率质谱(LC-HRMS)增强加合物的鉴定,设计了一种多克隆抗T3抗体来捕获HSA胰蛋白酶解物中的Cys34加合物(T3是第三大胰蛋白酶肽段)。基于T3肽段的三维结构,从C端和N端序列中选择表位,以尽量减少修饰的Cys34残基的影响。通过将磁珠连接到抗T3抗体上简化了检测方法。当应用于市售HSA以及健康人的血浆样本并通过LC-HRMS分析时,抗体处理大大降低了样本基质中非T3肽段的背景。尽管其他亲脂性HSA肽段仍然存在,推测是由于与抗体-磁珠表面的非特异性结合,但与未用抗体处理的相同样本相比,其在抗体处理样本中的浓度降低了约6倍。对来自人血浆样本的抗体富集HSA酶解物的分析揭示了10种修饰的T3肽段,其中8种通过精确质量得以鉴定。鉴定出的肽段包括Cys34氧化和半胱氨酸化产物以及代表水、赖氨酸损失和精氨酸转肽作用的修饰。

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