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半胱氨酸加合物在人血清白蛋白中的富集。

Enrichment of cysteinyl adducts of human serum albumin.

机构信息

Gillings School of Global Public Health, University of North Carolina, Chapel Hill, NC 27599, USA.

出版信息

Anal Biochem. 2010 May 1;400(1):61-8. doi: 10.1016/j.ab.2010.01.006. Epub 2010 Jan 13.

Abstract

We report a method to enrich cysteinyl adducts of human serum albumin (HSA), representing biomarkers of exposure to systemic electrophiles. Because the major site of HSA adduction is the single free sulfhydryl group at Cys34, we used thiol-affinity resins to remove mercaptalbumin (i.e., unadducted HSA) from the cysteinyl adducts. Electrospray ionization mass spectrometry was used to detect mercaptalbumin and HSA-Cys34 modifications before and after enrichment of HSA. Differences in adduct content were detected across samples of freshly isolated, archived, and commercial HSA. Cysteinylated and glycosylated adducts were present in all samples, with abundances decreasing in the following order: commercial HSA>archived HSA>fresh HSA. After enrichment of HSA, mercaptalbumin was no longer observed in mass spectra. The ratios of HSA adducts post-/preenrichment, quantified via the Bradford assay and gel electrophoresis, were 0.029 mg adducts/mg HSA in fresh HSA and 0.323 mg adducts/mg HSA in archived HSA. The apparent elevation of adduct levels in archived samples could be due to differences in specimen preparation and storage rather than to differences in circulating HSA adducts. We conclude that thiol-affinity resins can efficiently remove mercaptalbumin from HSA samples prior to characterization and quantitation of protein adducts of reactive systemic electrophiles.

摘要

我们报告了一种富集人血清白蛋白(HSA)中半胱氨酸加合物的方法,这些加合物可作为全身亲电试剂暴露的生物标志物。由于 HSA 加合的主要部位是 Cys34 上的单个游离巯基,因此我们使用巯基亲和树脂从半胱氨酸加合物中去除巯基白蛋白(即未加合的 HSA)。电喷雾电离质谱法用于检测巯基白蛋白和 HSA-Cys34 修饰物在 HSA 富集前后的变化。新鲜分离、存档和商业 HSA 样本中的加合物含量存在差异。所有样品中均存在半胱氨酸化和糖基化加合物,其丰度按以下顺序降低:商业 HSA>存档 HSA>新鲜 HSA。HSA 富集后,质谱中不再观察到巯基白蛋白。通过 Bradford 测定法和凝胶电泳定量的 HSA 加合物的后/前富集比在新鲜 HSA 中为 0.029 mg 加合物/mg HSA,在存档 HSA 中为 0.323 mg 加合物/mg HSA。存档样品中加合物水平的明显升高可能是由于标本制备和储存的差异,而不是循环 HSA 加合物的差异。我们得出结论,巯基亲和树脂可在对反应性全身亲电试剂的蛋白质加合物进行表征和定量之前,有效地从 HSA 样品中去除巯基白蛋白。

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