Harnessing intrinsic fluorescence for typing of secondary structures of DNA

Author:

Zuffo Michela12ORCID,Gandolfini Aurélie12,Heddi Brahim3ORCID,Granzhan Anton12ORCID

Affiliation:

1. CNRS UMR9187, INSERM U1196, Institut Curie, PSL Research University, F-91405 Orsay, France

2. CNRS UMR9187, INSERM U1196, Université Paris-Saclay, F-91405 Orsay, France

3. Laboratoire de Biologie et de Pharmacologie Appliquée, CNRS UMR8113, École Normale Supérieure Paris-Saclay, F-94235 Cachan, France

Abstract

Abstract High-throughput investigation of structural diversity of nucleic acids is hampered by the lack of suitable label-free methods, combining fast and cheap experimental workflow with high information content. Here, we explore the use of intrinsic fluorescence emitted by nucleic acids for this scope. After a preliminary assessment of suitability of this phenomenon for tracking conformational changes of DNA, we examined steady-state emission spectra of an 89-membered set of oligonucleotides with reported conformation (G-quadruplexes (G4s), i-motifs, single- and double-strands) by means of multivariate analysis. Principal component analysis of emission spectra resulted in successful clustering of oligonucleotides into three corresponding conformational groups, without discrimination between single- and double-stranded structures. Linear discriminant analysis was exploited for the assessment of novel sequences, allowing the evaluation of their G4-forming propensity. Our method does not require any labeling agent or dye, avoiding the related bias, and can be utilized to screen novel sequences of interest in a high-throughput and cost-effective manner. In addition, we observed that left-handed (Z-) G4 structures were systematically more fluorescent than most other G4 structures, almost reaching the quantum yield of 5′-d[(G3T)3G3]-3′ (G3T, the most fluorescent G4 structure reported to date).

Funder

French National Research Agency

Institut Curie

Publisher

Oxford University Press (OUP)

Subject

Genetics

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