A Single-Chain Antibody/Epitope System for Functional Analysis of Protein−Protein Interactions

表位 融合蛋白 蛋白质-蛋白质相互作用 计算生物学 细胞生物学 血浆蛋白结合 信号转导衔接蛋白 相互作用体 SH3域 突变 噬菌体展示 线性表位 化学 靶蛋白 表位定位 生物 抗体 信号转导 生物化学 受体酪氨酸激酶 遗传学 突变 重组DNA 基因
作者
Kôsaku Fujiwara,Kari Poikonen,Lourdes M. Alemán,Minna Valtavaara,Kalle Saksela,Bruce J. Mayer
出处
期刊:Biochemistry [American Chemical Society]
卷期号:41 (42): 12729-12738 被引量:18
标识
DOI:10.1021/bi0263309
摘要

Protein-protein interactions play a critical role in cellular processes such as signal transduction. Although many methods for identifying the binding partners of a protein of interest are available, it is currently difficult or impossible to assess the functional consequences of a specific interaction in vivo. To address this issue, we propose to modify proteins by addition of an artificial protein binding interface, thereby forcing them to interact in the cell in a pairwise fashion and allowing the functional consequences to be determined. For this purpose, we have developed an artificial binding interface consisting of a anti-Myc single-chain antibody (ScFv) and its peptide epitope. We found that the binding of an ScFv derived from anti-Myc monoclonal antibody 9E10 was relatively weak in vivo, so we selected an improved clone, 3DX, by in vitro mutagenesis and phage display. 3DX bound well to its epitope in a yeast two-hybrid system, and GST-fused 3DX also bound to several Myc-tagged proteins in mammalian cells. In vivo binding was relatively insensitive to the position of the ScFv in a fusion protein, but was improved by including multiple tandem copies of the Myc epitope in the binding partner. To test the system, we successfully replaced the SH3 domain-mediated interaction between the Abl tyrosine kinase and adaptor proteins Crk and Nck with an engineered interaction between 3DX and multiple Myc tags. We expect that this approach, which we term a functional interaction trap, will be a powerful proteomic tool for investigating protein-protein interactions.
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