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利用理论蛋白质同位素分布通过质谱法解析小质量差异的翻译后修饰。

Using theoretical protein isotopic distributions to parse small-mass-difference post-translational modifications via mass spectrometry.

机构信息

Department of Biochemistry and Biophysics, Oregon State University, Corvallis, OR 97331, USA.

出版信息

J Am Soc Mass Spectrom. 2013 Jan;24(1):115-24. doi: 10.1007/s13361-012-0500-1. Epub 2012 Dec 18.

Abstract

Small-mass-difference modifications to proteins are obscured in mass spectrometry by the natural abundance of stable isotopes such as (13)C that broaden the isotopic distribution of an intact protein. Using a ZipTip (Millipore, Billerica, MA, USA) to remove salt from proteins in preparation for high-resolution mass spectrometry, the theoretical isotopic distribution intensities calculated from the protein's empirical formula could be fit to experimentally acquired data and used to differentiate between multiple low-mass modifications to proteins. We could readily distinguish copper from zinc bound to a single-metal superoxide dismutase (SOD1) species; copper and zinc only differ by an average mass of 1.8 Da and have overlapping stable isotope patterns. In addition, proteins could be directly modified while bound to the ZipTip. For example, washing 11 mM S-methyl methanethiosulfonate over the ZipTip allowed the number of free cysteines on proteins to be detected as S-methyl adducts. Alternatively, washing with the sulfhydryl oxidant diamide could quickly reestablish disulfide bridges. Using these methods, we could resolve the relative contributions of copper and zinc binding, as well as disulfide reduction to intact SOD1 protein present from <100 μg of the lumbar spinal cord of a transgenic, SOD1 overexpressing mouse. Although techniques like ICP-MS can measure total metal in solution, this is the first method able to assess the metal-binding and sulfhydryl reduction of SOD1 at the individual subunit level and is applicable to many other proteins.

摘要

蛋白质中的小质量差异修饰会被(13)C 等稳定同位素的天然丰度所掩盖,这些同位素会使完整蛋白质的同位素分布变宽。在进行高分辨率质谱分析之前,使用 ZipTip(Millipore,马萨诸塞州比勒里卡,美国)去除蛋白质中的盐,可以将从蛋白质经验公式计算出的理论同位素分布强度拟合到实验获得的数据上,并用于区分蛋白质的多种低质量修饰。我们可以轻松区分与单金属超氧化物歧化酶(SOD1)结合的铜和锌;铜和锌仅相差 1.8 Da 的平均质量,且具有重叠的稳定同位素模式。此外,蛋白质可以在与 ZipTip 结合的同时直接进行修饰。例如,用 11 mM 的 S-甲基甲硫氨酸亚砜在 ZipTip 上洗涤,可以检测到蛋白质上自由半胱氨酸的数量作为 S-甲基加合物。或者,用巯基氧化剂二酰胺洗涤可以快速重新建立二硫键。使用这些方法,我们可以确定铜和锌结合以及二硫键还原对完整 SOD1 蛋白的相对贡献,这些蛋白来自转基因、SOD1 过表达小鼠的 <100 μg 腰椎脊髓。尽管 ICP-MS 等技术可以测量溶液中的总金属,但这是第一种能够在单个亚基水平上评估 SOD1 的金属结合和巯基还原的方法,并且适用于许多其他蛋白质。

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