
High affinity nucleic acid analogues such as gammaPNA (γPNA) are capable of invading stable secondary and tertiary structures in DNA and RNA targets but are susceptible to off-target binding to mismatch-containing sequences. We introduced a hairpin secondary structure into a γPNA oligomer to enhance hybridization selectivity compared with a hairpin-free analogue. The hairpin structure features a five base PNA mask that covers the proximal five bases of the γPNA probe, leaving an additional five γPNA bases available as a toehold for target hybridization. Surface plasmon resonance experiments demonstrated that the hairpin probe exhibited slower on-rates and faster off-rates (i.e., lower affinity) compared with the linear probe but improved single mismatch discrimination by up to a factor of five, due primarily to slower on-rates for mismatch vs. perfect match targets. The ability to discriminate against single mismatches was also determined in a cell-free mRNA translation assay using a luciferase reporter gene, where the hairpin probe was two-fold more selective than the linear probe. These results validate the hairpin design and present a generalizable approach to improving hybridization selectivity.
Peptide Nucleic Acids, antisense, selectivity, Organic chemistry, Nucleic Acid Hybridization, DNA, Surface Plasmon Resonance, Article, QD241-441, γPNA, Nucleic Acid Conformation, RNA, γpna, hybridization
Peptide Nucleic Acids, antisense, selectivity, Organic chemistry, Nucleic Acid Hybridization, DNA, Surface Plasmon Resonance, Article, QD241-441, γPNA, Nucleic Acid Conformation, RNA, γpna, hybridization
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