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dUTP 及其在内部结合于 DNA 的荧光团的光谱和光物理性质,用于优化生物体系中的信号检测。

Spectroscopic and photophysical properties of dUTP and internally DNA bound fluorophores for optimized signal detection in biological formats.

机构信息

BAM Federal Institute for Materials Research and Testing, Berlin, Germany.

出版信息

Photochem Photobiol. 2012 Jul-Aug;88(4):867-75. doi: 10.1111/j.1751-1097.2012.01119.x. Epub 2012 Mar 28.

DOI:10.1111/j.1751-1097.2012.01119.x
PMID:22360746
Abstract

Efficient signal generation in DNA-based assays requires understanding of the influence of fluorophore's interactions on the spectroscopic properties. The resulting changes in fluorescence intensity, quantum yield, emission anisotropy, and fluorescence lifetime provide straightforward tools for the study of molecular dynamics and interaction between labels and nucleic acids. Searching for bright fluorescent reporters for rolling circle amplification (RCA) as efficient signal enhancement strategy for biological formats, we investigated the spectroscopic properties of seven dyes: cyanines, rhodamines, and BODIPYs. They spectrally resemble Cy3, the most frequently used fluorophore in biodetection formats, and are measured in six samples (free dye, dye-dUTP, internally labeled ssDNA and dsDNA-single- and triple-labeled) using steady-state and time-resolved fluorometry. Special emphasis was dedicated to characterizing the nature of the interaction of these fluorophores differing in dye class, charge, and rigidity. Our results suggest dye charge and structure as main factors governing the dye's interactions, with DY-555 and Cy3B presenting the best candidates for our envisaged signal amplification strategy. This label comparison underlines the importance of a proper understanding of structure-property relations and dye-biomolecule interactions for reporter choice and presents a road map towards the design and interpretation of experiments using these labels on DNA of known sequence.

摘要

高效的基于 DNA 的分析需要理解荧光团相互作用对光谱性质的影响。荧光强度、量子产率、发射各向异性和荧光寿命的变化为研究分子动力学和标记物与核酸之间的相互作用提供了直接的工具。为了寻找用于滚环扩增(RCA)的明亮荧光报告物作为生物格式的有效信号增强策略,我们研究了七种染料的光谱性质:菁染料、罗丹明和 BODIPY。它们在光谱上类似于 Cy3,这是生物检测格式中最常用的荧光团,并使用稳态和时间分辨荧光法在六种样品(游离染料、染料-dUTP、内部标记的单链 DNA 和双链 DNA-单标记和三标记)中进行测量。特别强调了表征这些荧光团在染料类别、电荷和刚性方面不同的相互作用性质。我们的结果表明,染料电荷和结构是控制染料相互作用的主要因素,DY-555 和 Cy3B 是我们预期信号放大策略的最佳候选者。这种标记物比较强调了正确理解结构-性质关系和染料-生物分子相互作用对于报告物选择的重要性,并为使用这些标记物在已知序列的 DNA 上进行实验的设计和解释提供了路线图。

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