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首页> 外文期刊>Journal of Biotechnology >A novel flow cytometry-based method for analysis of expression levels in Escherichia coli, giving information about precipitated and soluble protein
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A novel flow cytometry-based method for analysis of expression levels in Escherichia coli, giving information about precipitated and soluble protein

机译:一种基于流式细胞术的新型方法,用于分析大肠杆菌中的表达水平,提供有关沉淀和可溶性蛋白的信息

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摘要

A high throughput method for screening of protein expression is described. By using a flow cytometer, levels of both soluble and precipitated protein can simultaneously be assessed in vivo. Protein fragments were fused to the N-terminus of enhanced GFP and the cell samples were analysed using a flow cytometer. Data concerning whole cell fluorescence and light scattering was collected. The whole cell fluorescence is probing intracellular concentrations of soluble fusion proteins. Concurrently, forward scattered light gives data about inclusion body formation, valuable information in process optimisation. To evaluate the method, the cells were disrupted, separated into soluble and non-soluble fractions and analysed by gel electrophoresis. A clear correlation between fluorescence and soluble target protein was shown. Interestingly, the distribution of the cells regarding forward scatter (standard deviation) correlates with the amount of inclusion bodies formed. Finally, the newly developed method was used to evaluate two different purification tags, His(6) and Z(basic), and their effect on the expression pattern.
机译:描述了用于筛选蛋白质表达的高通量方法。通过使用流式细胞仪,可同时在体内评估可溶性和沉淀蛋白的水平。将蛋白质片段融合到增强的GFP的N端,并使用流式细胞仪分析细胞样品。收集有关全细胞荧光和光散射的数据。整个细胞的荧光正在探测可溶性融合蛋白的细胞内浓度。同时,前向散射光会提供有关包涵体形成的数据,以及过程优化中的宝贵信息。为了评估该方法,将细胞破碎,分为可溶性和非可溶性级分,并通过凝胶电泳进行分析。显示了荧光和可溶性靶蛋白之间的明显相关性。有趣的是,关于正向散射的细胞分布(标准偏差)与所形成的包涵体的数量相关。最后,新开发的方法用于评估两个不同的纯化标签,His(6)和Z(碱性),以及它们对表达模式的影响。

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