Self-assembling peptides act as versatile templates for gold nanoparticle (AuNP) synthesis. Their organization into discrete nanostructures or hydrogels enables control over AuNP morphology and assembly, offering new opportunities for functional ...
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Hybridization Probes Featuring a Pyrenylpyridine C‐Nucleoside or Its Palladacycle as a Fluorescent Sensor Moiety
Von Wiley-VCH zur Verfügung gestellt
When placed in the middle of a double helix as a nucleobase surrogate, pyren-1-ylpyridine and its palladacyclic derivative show fluorescence emission sensitive to the identity of the canonical nucleobase opposite to it. Emission of the palladacycle is weaker but the base discrimination stronger, possibly because of Pd(II)-mediated base pairing. More emissive metallacycles can find use in genotyping single-nucleotide polymorphisms.
A C-nucleoside analog having pyren-1-ylpyridine as the base moiety has been synthesized and incorporated in the middle of a short oligodeoxynucleotide. A portion of this oligonucleotide is cyclopalladated at the modified residue, and the potential of both the metal-free and the palladacyclic oligonucleotide as hybridization probes for single-nucleotide polymorphism genotyping is assessed by melting studies on relevant duplexes using various techniques. Conventional ultraviolet (UV) melting profiles at 260 nm reveal considerable destabilization of the palladacyclic duplexes relative to their metal-free counterparts. Circular dichroism melting temperatures are higher than their UV counterparts, especially with the palladacyclic duplexes. Cyclopalladation markedly reduces the fluorescence emission of the pyrenylpyridine moiety, but both the metal-free and the palladacyclic oligonucleotide exhibit a qualitatively similar pattern of increased fluorescence on hybridization with a complementary sequence, consistent with the pyrene ring being “pushed out” of the base stack. Emission at low temperature is dependent on the nucleobase paired with the pyrenylpyridine base surrogate with both of the modified oligonucleotides. This discrimination is stronger with the palladacyclic oligonucleotide, possibly owing to Pd(II)-mediated base pairing.
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