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A simple luciferase assay for signal transduction activity detection of epidermal growth factor displayed on phage.

机译:一种简单的荧光素酶测定法,用于检测噬菌体上显示的表皮生长因子的信号转导活性。

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摘要

Studies on receptor-ligand interactions are important for the design of agonists or antagonists of natural ligands. We developed a luciferase reporter assay to screen epidermal growth factor receptor (EGFR) binding molecules rapidly for their ability to stimulate or inhibit signal transduction. Human EGF displayed on fd filamentous phage presented an activity similar to soluble EGF when tested for binding to the EGFR, for induction of cell cycle progression or in the luciferase assay. Two libraries of human EGF variants displayed on phage were constructed in which the aspartic acid residue at position 46 or the arginine residue at position 41 were randomised. EGF mutants displayed on phage were screened in parallel for binding to the EGFR using an ELISA assay and for transducing activity using the luciferase assay. Regarding the 46 position, most of the mutants retained the ability to bind the EGFR and their transducing activity corresponded perfectly with their binding. For the more crucial 41 position, only the wild-type EGF was able to bind the EGFR. Our approach allowed a simple determination of crucial positions and paved the way for identification of agonists with altered transduction activity.
机译:受体-配体相互作用的研究对于天然配体的激动剂或拮抗剂的设计很重要。我们开发了荧光素酶报告基因检测法,以快速筛选表皮生长因子受体(EGFR)结合分子的刺激或抑制信号转导能力。当测试与EGFR的结合,诱导细胞周期进程或在萤光素酶测定中,显示在fd丝状噬菌体上的人EGF表现出与可溶性EGF相似的活性。构建了两个在噬菌体上展示的人EGF变体文库,其中第46位的天冬氨酸残基或第41位的精氨酸残基是随机的。平行筛选展示在噬菌体上的EGF突变体,以使用ELISA测定法与EGFR结合,并使用荧光素酶测定法筛选其转导活性。关于46位,大多数突变体保留了结合EGFR的能力,并且其转导活性与其结合完全一致。对于更为关键的41位,只有野生型EGF能够结合EGFR。我们的方法允许简单地确定关键位置,并为识别具有改变的转导活性的激动剂铺平了道路。

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