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Monitoring Protein Refolding Induced by Disulfide Formation Using Capillary lsoelectric Focusing- Electrospray Ionization Mass Spectrometry

机译:使用毛细管等电聚焦-电喷雾电离质谱法监测由二硫键形成引起的蛋白质折叠

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Rapid growth in the biotechnology industry has led to a dramatic increase in attention to the protein folding problem. Understanding protein-folding pathways is essential to the production of biopharmaceuticals since commercial production of recombinant proteins often requires a protein-refolding process for recovery of high yields. Protein folding coupled to the formation of disulfide bonds presents one of the simplest approaches to studying folding intermediates. On-line capillary isoelectric focusing-electrospray ionization mass spectrometry (CIEF-ESIMS) is demonstrated for kinetic studies of disulfide bond-induced protein refolding. Refolding intermediates of bovine pancreatic ribonuclease A, a model system for this study, are blocked at different stages by alkylating free thiols with iodoacetate. The alkylation reaction results in the introduction of charge (-1) and mass (59) differences for each alkylation site, providing the means for predictable separation and direct identification of refolding intermediates using CIEF-ESIMS. Besides the observation of refolding intermediates containing different numbers of disulfide bonds and even mixed disulfides, the two.dimensional resolving power of CIEF-ESIMS allows the determination of conformational heterogeneity among groups of refolding intermediates.
机译:生物技术产业的快速发展导致人们对蛋白质折叠问题的关注急剧增加。了解蛋白质折叠途径对于生物药物的生产至关重要,因为重组蛋白质的商业化生产通常需要蛋白质折叠过程才能回收高产。蛋白质折叠与二硫键的形成偶联是研究折叠中间体的最简单方法之一。在线毛细管等电聚焦-电喷雾电离质谱(CIEF-ESIMS)已被证明可用于二硫键诱导的蛋白质复性的动力学研究。牛胰核糖核酸酶A(本研究的模型系统)的重折叠中间体在不同阶段通过用碘乙酸烷基化游离硫醇而被封闭。烷基化反应导致每个烷基化位点引入电荷(-1)和质量(59)差异,从而提供了使用CIEF-ESIMS进行可预测的分离和直接识别重折叠中间体的方法。除了观察包含不同数量的二硫键甚至混合的二硫键的重折叠中间体外,CIEF-ESIMS的二维分辨能力还可以确定重折叠中间体组之间的构象异质性。

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