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利用大肠杆菌无细胞体系生产稳定同位素标记蛋白的经济方法。

An economical method for producing stable-isotope labeled proteins by the E. coli cell-free system.

机构信息

RIKEN Systems and Structural Biology Center, 1-7-22 Suehiro-cho, Tsurumi, Yokohama, 230-0045, Japan.

出版信息

J Biomol NMR. 2010 Dec;48(4):193-201. doi: 10.1007/s10858-010-9455-3. Epub 2010 Nov 4.

Abstract

Improvement of the cell-free protein synthesis system (CF) over the past decade have made it one of the most powerful protein production methods. The CF approach is especially useful for stable-isotope (SI) labeling of proteins for NMR analysis. However, it is less popular than expected, partly because the SI-labeled amino acids used for SI labeling by the CF are too expensive. In the present study, we developed a simple and inexpensive method for producing an SI-labeled protein using Escherichia coli cell extract-based CF. This method takes advantage of endogenous metabolic conversions to generate SI-labeled asparagine, glutamine, cysteine, and tryptophan, which are much more expensive than the other 16 kinds of SI-labeled amino acids, from inexpensive sources, such as SI-labeled algal amino acid mixture, SI-labeled indole, and sodium sulfide, during the CF reaction. As compared with the conventional method employing 20 kinds of SI-labeled amino acids, highly enriched uniform SI-labeling with similar labeling efficiency was achieved at a greatly reduced cost with the newly developed method. Therefore, our method solves the cost problem of the SI labeling of proteins using the CF.

摘要

在过去的十年中,无细胞蛋白合成系统 (CF) 的改进使其成为最强大的蛋白质生产方法之一。CF 方法特别适用于用于 NMR 分析的蛋白质的稳定同位素 (SI) 标记。然而,它并没有像预期的那样受欢迎,部分原因是 CF 用于 SI 标记的 SI 标记氨基酸过于昂贵。在本研究中,我们开发了一种使用基于大肠杆菌细胞提取物的 CF 生产 SI 标记蛋白的简单且廉价的方法。该方法利用内源性代谢转化,从廉价来源(如 SI 标记的藻类氨基酸混合物、SI 标记的吲哚和硫化钠)在 CF 反应过程中生成比其他 16 种 SI 标记氨基酸昂贵得多的 SI 标记天冬酰胺、谷氨酰胺、半胱氨酸和色氨酸。与使用 20 种 SI 标记氨基酸的传统方法相比,新开发的方法以大大降低的成本实现了具有相似标记效率的高度富集的均匀 SI 标记。因此,我们的方法解决了 CF 中蛋白质 SI 标记的成本问题。

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