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- W2030601151 abstract "Many genomics assays use profluorescent oligonucleotide probes that are covalently labeled at the 5‘ end with a fluorophore and at the 3‘ end with a quencher. It is generally accepted that quenching in such probes without a stem structure occurs through Förster resonance energy transfer (FRET or FET) and that the fluorophore and quencher should be chosen to maximize their spectral overlap. We have studied two dual-labeled probes with two different fluorophores, the same sequence and quencher, and with no stem structure: 5‘Cy3.5−β-actin−3‘BHQ1 and 5‘FAM−β-actin−3‘BHQ1. Analysis of their absorption spectra, relative fluorescence quantum yields, and fluorescence lifetimes shows that static quenching occurs in both of these dual-labeled probes and that it is the dominant quenching mechanism in the Cy3.5−BHQ1 probe. Absorption spectra are consistent with the formation of an excitonic dimer, an intramolecular heterodimer between the Cy3.5 fluorophore and the BHQ1 quencher." @default.
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- W2030601151 date "2002-05-21" @default.
- W2030601151 modified "2023-10-18" @default.
- W2030601151 title "Intramolecular Dimers: A New Strategy to Fluorescence Quenching in Dual-Labeled Oligonucleotide Probes" @default.
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- W2030601151 doi "https://doi.org/10.1021/ja025678o" @default.
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