Valentina Arciuolo , Simona Marzano , Rossella Buono, Nicola Grasso, Anna Di Porzio, Antonio Randazzo, Bruno Pagano, Jussara Amato
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引用次数: 0
摘要
g -四plex (G4s)是参与关键细胞过程的非规范DNA/RNA结构,它们与蛋白质的相互作用正成为治疗靶点。然而,鉴定结合G4s并可能调节这些相互作用的配体的策略仍然有限。在这里,我们描述了一种基于荧光的检测方法,用于快速定量评估结合G4s并可能干扰蛋白质识别的小分子。该方法采用从保守的g4结合蛋白基序衍生的荧光团标记肽,以及用荧光受体标记的g4形成序列。通过荧光增加检测配体诱导的肽位移。对一组已知的G4配体进行了测试,结果与结合亲和力相关。双链DNA竞争分析进一步评估了配体的选择性。该方法提供了一种可扩展的工具,用于筛选具有与G4识别基序竞争能力的G4配体,支持药物发现工作。
Screening of G-quadruplex DNA ligands by fluorescence detection of peptide displacement
G-quadruplexes (G4s) are noncanonical DNA/RNA structures involved in key cellular processes, and their interactions with proteins are emerging as therapeutic targets. However, strategies to identify ligands that bind G4s and potentially modulate these interactions remain limited. Here, we describe a fluorescence-based assay for rapid, quantitative evaluation of small molecules that bind G4s and potentially interfere with protein recognition. The method employs a fluorophore-labeled peptide derived from a conserved G4-binding protein motif, and a G4-forming sequence labeled with a fluorescence acceptor. Ligand-induced peptide displacement is detected via fluorescence increase. A panel of known G4 ligands was tested, and results correlated with binding affinities. A duplex DNA competition assay further assessed ligand selectivity. This method provides a scalable tool for screening G4 ligands with ability to compete with G4-recognition motifs, supporting drug discovery efforts.
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