Selection Strategy to Generate Aptamer Pairs that Bind to Distinct Sites on Protein Targets

适体 指数富集配体系统进化 化学 核酸 SELEX适体技术 计算生物学 组合化学 热稳定性 靶蛋白 核糖核酸 试剂 生物化学 分子生物学 基因 生物 物理化学
作者
Qiang Gong,Jinpeng Wang,Kareem M. Ahmad,Andrew T. Csordas,Jiehua Zhou,Jeff Nie,Ron Stewart,James A. Thomson,John J. Rossi,H. Tom Soh
出处
期刊:Analytical Chemistry [American Chemical Society]
卷期号:84 (12): 5365-5371 被引量:62
标识
DOI:10.1021/ac300873p
摘要

Many analytical techniques benefit greatly from the use of affinity reagent pairs, wherein each reagent recognizes a discrete binding site on a target. For example, antibody pairs have been widely used to dramatically increase the specificity of enzyme linked immunosorbent assays (ELISA). Nucleic acid-based aptamers offer many advantageous features relative to protein-based affinity reagents, including well-established chemical synthesis, thermostability, and low production cost. However, the generation of suitable aptamer pairs has posed a significant challenge, and few such pairs have been reported to date. To address this important challenge, we present multivalent aptamer isolation systematic evolution of ligands by exponential enrichment (MAI-SELEX), a technique designed for the efficient selection of aptamer pairs. In contrast to conventional selection methods, our method utilizes two selection modules to generate separate aptamer pools that recognize distinct binding sites on a single target. Using MAI-SELEX, we have isolated two groups of 2′-fluoro-modified RNA aptamers that specifically recognize the αV or β3 subunits of integrin αVβ3. These aptamers exhibit low nanomolar affinities for their targets, with minimal cross-reactivity to other closely related integrin homologues. Moreover, we show that these aptamer pairs do not interfere with each other’s binding and effectively detect the target even in complex mixtures such as undiluted serum.
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