首页> 外文期刊>The Journal of toxicological sciences >A convenient method to assess chemical modification of protein thiols by electrophilic metals.
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A convenient method to assess chemical modification of protein thiols by electrophilic metals.

机译:评估亲电金属对蛋白质硫醇的化学修饰的便捷方法。

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摘要

Although covalent modification of protein thiols by electrophilic metals is implicated in disruption of protein functions associated with toxicity, there are limited methods available to detect such modifications. In the present study, we established a convenient method to assess modification of protein thiols by electrophiles, referred to as a biotin-PEAC?-maleimide (BPM)-labeling assay. In this assay, protein S-modification by electrophiles can be estimated by a decrease in protein modification by BPM, a thiol reactive probe. Using methylmercury (MeHg) as a model electrophilic metal, thiol modification of cellular proteins was detected by the BPM-labeling assay in SH-SY5Y cell lysates and primary mouse hepatocytes. The sensitivity and reliability of the assay was confirmed by atomic absorption spectrometry with recombinant Keap1 as a model thiol protein. This assay was applied to not only MeHg but also to other metals such as cadmium and lead. We also established a BPM-precipitation assay with avidin-agarose beads to separate BPM-modified cellular proteins followed by detection with the individual antibodies. This assay was available for detecting MeHg-induced S-modification of cellular Keap1 in SH-SY5Y cells. Taken together, we have developed reliable simple methods to estimate protein S-modification by electrophilic metals.
机译:尽管亲电金属对蛋白质硫醇的共价修饰涉及与毒性相关的蛋白质功能的破坏,但检测这种修饰的方法有限。在本研究中,我们建立了一种方便的方法来评估亲电试剂对蛋白质硫醇的修饰,称为生物素-PEACβ-马来酰亚胺(BPM)标记测定法。在该测定中,亲电体对蛋白质S的修饰可通过BPM(一种硫醇反应性探针)对蛋白质的修饰减少来估算。使用甲基汞(MeHg)作为模型亲电子金属,通过BPM标记测定法在SH-SY5Y细胞裂解液和原代小鼠肝细胞中检测到细胞蛋白的巯基修饰。用重组Keap1作为模型硫醇蛋白的原子吸收光谱法证实了该测定方法的灵敏度和可靠性。该测定法不仅适用于MeHg,还适用于其他金属,例如镉和铅。我们还用抗生物素蛋白-琼脂糖珠建立了BPM沉淀测定法,以分离BPM修饰的细胞蛋白,然后用单个抗体进行检测。该测定法可用于检测MeHg诱导的SH-SY5Y细胞中Keap1细胞的S-修饰。综上所述,我们已经开发出可靠的简单方法来估计亲电金属对蛋白质S的修饰。

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