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首页> 外文期刊>Journal of Biochemical and Biophysical Methods >Construction of a high sensitive Escherichia coli alkaline phosphatase reporter system for screening affinity peptides.
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Construction of a high sensitive Escherichia coli alkaline phosphatase reporter system for screening affinity peptides.

机译:用于筛选亲和力肽的高灵敏度大肠杆菌碱性磷酸酶报告系统的构建。

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摘要

An enzyme-linker-peptide fusion protein reporter system was constructed for sensitive analysis of affinity of peptide ligands to their receptor. An E. coli alkaline phosphatase (EAP) mutant enzyme with high catalytic activity was selected as the reporter protein. Interaction of affinity peptide and streptavidin was applied as demonstration of the method. Three affinity peptides, strep-tag I (SI), strep-tag II (SII) and streptavidin binding peptide (SBP) were genetically fused to the C-terminal of EAP respectively, with an insertion of a flexible linker peptide in between. The enzyme activity of the EAP fusions showed no obvious change. After expression and purification, the EAP-affinity peptide fusions were applied to the streptavidin modified surface. Binding of the fusions to the surface through interaction of affinity peptides to streptavidin was indicated by color generated from conversion of the substrate by EAP. The relative affinity and specificity of each affinity peptides to the immobilized streptavidin were then evaluated with high sensitivity and broad detection range. This method may be used for effective high-throughput screening of high affinity peptide from the peptide pool.
机译:构建了酶联蛋白-肽融合蛋白报告系统,用于灵敏地分析肽配体对其受体的亲和力。选择具有高催化活性的大肠杆菌碱性磷酸酶(EAP)突变酶作为报告蛋白。应用亲和肽和链霉亲和素的相互作用作为该方法的证明。将三种亲和力肽,strep-tag I(SI),strep-tag II(SII)和链霉亲和素结合肽(SBP)分别遗传融合到EAP的C端,并在两者之间插入一个柔性接头肽。 EAP融合体的酶活性没有明显变化。表达和纯化后,将EAP亲和肽融合物应用于链霉亲和素修饰的表面。通过亲和肽与链霉亲和素的相互作用,将融合物与表面结合,由EAP转化底物所产生的颜色表示。然后以高灵敏度和宽检测范围评估了每种亲和肽对固定化链霉亲和素的相对亲和力和特异性。该方法可用于从肽库中有效地高通量筛选高亲和力肽。

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