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蛋白质棕榈酰化位点的标记与定量

Labeling and quantifying sites of protein palmitoylation.

作者信息

Drisdel Renaldo C, Green William N

机构信息

University of Chicago, Chicago, IL, USA.

出版信息

Biotechniques. 2004 Feb;36(2):276-85. doi: 10.2144/04362RR02.

Abstract

As a reversible posttranslational modification, protein palmitoylation has the potential to regulate the trafficking and function of a variety of proteins. However, the extent, function, and dynamic nature of palmitoylation are poorly resolved because of limitations in assay methods. Here, we introduce methods where hydroxylamine-mediated cleavage of the palmitoyl-thioester bond generates a free sulfhydryl, which can then be specifically labeled with sulfhydryl-reactive reagents. This methodology is more sensitive and allows for quantitative estimates of palmitoylation. Unlike other techniques used to assay posttranslational modifications, the techniques we have developed can label all sites of modification with a variety of probes, radiolabeled or nonradioactive, and can be used to assay the palmitoylation of proteins expressed in vivo in brain or other tissues.

摘要

作为一种可逆的翻译后修饰,蛋白质棕榈酰化有潜力调节多种蛋白质的运输和功能。然而,由于检测方法的局限性,棕榈酰化的程度、功能和动态性质仍未得到很好的解析。在此,我们介绍了一些方法,其中羟胺介导的棕榈酰硫酯键裂解会产生一个游离巯基,然后可以用巯基反应试剂对其进行特异性标记。这种方法更灵敏,能够对棕榈酰化进行定量评估。与用于检测翻译后修饰的其他技术不同,我们开发的技术可以用各种放射性或非放射性探针标记所有修饰位点,并且可用于检测在脑或其他组织中体内表达的蛋白质的棕榈酰化。

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