Identifying triplex binding rulesin vitroleads to creation of a new synthetic regulatory toolin vivo

Author:

Kaufmann Beate,Willinger Or,Eden Noa,Kermas Lisa,Anavy Leon,Solomon Oz,Atar Orna,Yakhini Zohar,Goldberg Sarah,Amit RoeeORCID

Abstract

SummaryNature provides a rich toolbox of dynamic nucleic acid structures that are widespread in cells and affect multiple biological processes1. Recently, non-canonical structures gained renewed scientific and biotechnological interest2,3. One particularly intriguing form of such structures are triplexes4in which a single-stranded nucleic acid molecule interacts via Hoogsteen bonds with a DNA/RNA double helix5. Despite extensive researchin vitro6–9, the underlying rules for triplex formation remain debated and evidence for triplexesin vivois circumstantial10–12. Here, we demonstrate the development of a deep-sequencing platform termed Triplex-Seq to systematically refine the DNA triplex code and identify high affinity triplex forming oligo (TFO) variants. We identified a preference for short G-rich motifs using an oligo-library with a mix of all four bases. These high-information content motifs formed specific high-affinity triplexes in a pH-independent manner and stability was increased with G-rich double-stranded molecules. We then conjugated one high-affinity and one low-affinity variant to a VP48 peptide and studied these synthetic biomolecules in mammalian cells. Using these peptide-oligo constructs (POCs), we demonstrated possible triplex-induced down-regulation activity in 544 differentially expressed genes. Our results show that deep-sequencing platforms can substantially expand our understanding of triplex binding rules, which in turn has led to the development of a functional non-genetically encoded regulatory tool forin vivoapplications.

Publisher

Cold Spring Harbor Laboratory

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