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FRET‐MC: A fluorescence melting competition assay for studying G4 structures in vitro

费斯特共振能量转移 G-四倍体 化学 序列(生物学) 熔化温度 荧光 单分子微动 竞赛(生物学) 生物物理学 计算生物学 纳米技术 生物化学 DNA 生物 物理 量子力学 复合材料 材料科学 生态学
作者
Yu Luo,Anton Granzhan,Daniela Verga,Jean‐Louis Mergny
出处
期刊:Biopolymers [Wiley]
卷期号:112 (4) 被引量:27
标识
DOI:10.1002/bip.23415
摘要

G-quadruplexes (G4) play crucial roles in biology, analytical chemistry and nanotechnology. The stability of G4 structures is impacted by the number of G-quartets, the length and positions of loops, flanking motifs, as well as additional structural elements such as bulges, capping base pairs, or triads. Algorithms such as G4Hunter or Quadparser may predict if a given sequence is G4-prone by calculating a quadruplex propensity score; however, experimental validation is still required. We previously demonstrated that this validation is not always straightforward, and that a combination of techniques is often required to unambiguously establish whether a sequence forms a G-quadruplex or not. In this article, we adapted the well-known FRET-melting assay to characterize G4 in batch, where the sequence to be tested is added, as an unlabeled competitor, to a system composed of a dual-labeled probe (F21T) and a specific quadruplex ligand. PhenDC3 was preferred over TMPyP4 because of its better selectivity for G-quadruplexes. In this so-called FRET-MC (melting competition) assay, G4-forming competitors lead to a marked decrease of the ligand-induced stabilization effect (∆Tm ), while non-specific competitors (e.g., single- or double-stranded sequences) have little effect. Sixty-five known sequences with different typical secondary structures were used to validate the assay, which was subsequently employed to assess eight novel sequences that were not previously characterized.
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