Issue 6, 2014

A simple “add and measure” FRET-based telomeric tandem repeat sequence detection and telomerase assay method

Abstract

A simple and sensitive method for measuring telomeric tandem repeat DNA and telomerase activity based on fluorescence resonance energy transfer (FRET) with a FAM-modified 12-mer ODN probe as a donor (fluorophore) and ethidium bromide (EB) as an acceptor (quencher) is proposed. When telomeric DNA and the FAM-modified probe form a duplex, EB intercalates between base-pairs, resulting in fluorescence quenching of FAM through FRET from FAM to EB. This method can be used to estimate the amount of telomeric DNAs in a sample solution as the molar concentration of the telomeric DNA unit [5′-(TTA GGG TTA GGG)-3′]. A linear fluorescence quenching ratio was obtained in 5–1000 pM of telomeric DNA units by adjusting the amount of FAM-modified probe. A PCR-free telomerase activity assay using this FRET-based method could be applied to ≥400 HeLa cells per μL. This assay represents a novel technique for initial screenings of cancer diagnosis and is a facile method for quantifying telomeric DNA or other tandem repeat sequences.

Graphical abstract: A simple “add and measure” FRET-based telomeric tandem repeat sequence detection and telomerase assay method

Supplementary files

Article information

Article type
Paper
Submitted
21 Oct 2013
Accepted
03 Dec 2013
First published
20 Dec 2013

Org. Biomol. Chem., 2014,12, 936-941

A simple “add and measure” FRET-based telomeric tandem repeat sequence detection and telomerase assay method

K. Kawamura, H. Yaku, D. Miyoshi and T. Murashima, Org. Biomol. Chem., 2014, 12, 936 DOI: 10.1039/C3OB42092B

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