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首页> 外文期刊>Protein Science: A Publication of the Protein Society >An automated in vitro protein folding screen applied to a human dynactin subunit.
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An automated in vitro protein folding screen applied to a human dynactin subunit.

机译:自动体外蛋白质折叠筛选应用于人dynactin亚基。

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摘要

The preparation of proteins for structural and functional analysis using the Escherichia coli expression system is often hampered by the formation of insoluble intracellular protein aggregates (inclusion bodies). Transferring those proteins into their native states by in vitro protein folding requires screening for the best buffer conditions and suitable additives. However, it is difficult to assess the success of such a screen if no biological assay is available. We established a fully automated folding screen and a system to detect folded protein that is based on analytical hydrophobic interaction chromatography and tryptophan fluorescence spectroscopy. The system was evaluated with two model enzymes (carbonic anhydrase II and malate dehydrogenase), and was successfully applied to the folding of the p22 subunit of human dynactin, which is expressed in inclusion bodies in E. coli. The described screen allows for high-throughput folding analysis of inclusion body proteins for structural and functional analyses.
机译:使用大肠埃希氏菌表达系统进行结构和功能分析所需的蛋白质制备,常常会因形成不溶性细胞内蛋白质聚集体(包涵体)而受到阻碍。通过体外蛋白质折叠将这些蛋白质转移至天然状态需要筛选最佳缓冲条件和合适的添加剂。但是,如果没有生物学检测方法,则很难评估这种筛选的成功率。我们建立了一个全自动折叠屏风和检测折叠蛋白的系统,该系统基于分析性疏水相互作用色谱和色氨酸荧光光谱法。该系统用两种模型酶(碳酸酐酶II和苹果酸脱氢酶)进行了评估,并成功应用于人Dynactin的p22亚基的折叠,该折叠在大肠杆菌的包涵体中表达。所描述的屏幕可对包含体蛋白进行高通量折叠分析,以进行结构和功能分析。

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