Pyrene-nucleobase conjugates: synthesis, oligonucleotide binding and confocal bioimaging studies

Fluorescent pyrene-linker-nucleobase (nucleobase = thymine, adenine) conjugates with carbonyl and hydroxy functionalities in the linker were synthesized and characterized. X-ray single-crystal structure analysis performed for the pyrene-C(O)CH CH -thymine ( ) conjugate reveals dimers of molecules st...

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Veröffentlicht in:Beilstein journal of organic chemistry 2017-11, Vol.13 (1), p.2521-2534
Hauptverfasser: Jabłoński, Artur, Fritz, Yannic, Wagenknecht, Hans-Achim, Czerwieniec, Rafał, Bernaś, Tytus, Trzybiński, Damian, Woźniak, Krzysztof, Kowalski, Konrad
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Sprache:eng
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Zusammenfassung:Fluorescent pyrene-linker-nucleobase (nucleobase = thymine, adenine) conjugates with carbonyl and hydroxy functionalities in the linker were synthesized and characterized. X-ray single-crystal structure analysis performed for the pyrene-C(O)CH CH -thymine ( ) conjugate reveals dimers of molecules stabilized by hydrogen bonds between the thymine moieties. The photochemical characterization showed structure-dependent fluorescence properties of the investigated compounds. The conjugates bearing a carbonyl function represent weak emitters as compared to compounds with a hydroxy function in the linker. The self-assembly properties of pyrene nucleobases were investigated in respect to their binding to single and double strand oligonucleotides in water and in buffer solution. In respect to the complementary oligothymidine T template in water, compounds and both show a self-assembling behavior according to canonical base-base pairing. However, in buffer solution, derivative was much more effective than in binding to the T template. Furthermore the adenine derivative binds to the double-stranded (dA) -T template with a self-assembly ratio of 112%. Such a high value of a self-assembly ratio can be rationalized by a triple-helix-like binding, intercalation, or a mixture of both. Remarkably, compound also shows dual staining pattern in living HeLa cells. Confocal microscopy confirmed that predominantly stains mitochondria but it also accumulates in the nucleoli of the cells.
ISSN:1860-5397
2195-951X
1860-5397
DOI:10.3762/bjoc.13.249