Mapping the interactions of selected antibiotics and their Cu2+ complexes with the antigenomic delta ribozyme

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Abstract

The interactions of selected antibiotics with the trans-acting antigenomic delta ribozyme were mapped. Ribozyme with two oligonucleotide substrates was used, one uncleavable with deoxycytidine at the cleavage site, mimicking the initial state of ribozyme, and the other with an all-RNA substrate mimicking, after cleavage, the product state. Mapping was performed with a set of RNA structural probing methods: Pb2+ -induced cleavage, nuclease digestion, and the selective 2′-hydroxyl acylation analyzed by primer extension (SHAPE) approach. The experimental results combined with molecular modeling revealed different binding sites for neomycin B, amikacin and actinomycin D inside the ribozyme structure. Neomycin B, an aminoglycoside antibiotic, which strongly inhibited the catalytic properties of delta ribozyme, was bound to the pocket formed by the P1 stem, the P1.1 pseudoknot, and the J4/2 junction. Amikacin showed less effective binding to the ribozyme catalytic core, resulting in weak inhibition. Complexes of these aminoglycosides with Cu2+ ions were bound to the same ribozyme regions, but more effectively, showing lower Kd values. On the other hand, the Cu 2+ complex of the cyclopeptide antibiotic actinonomycin D was preferentially intercalated into the P2 and the P4 double-stranded region, and was three times more potent in ribozyme inhibition than the free antibiotic. In addition, some differences in SHAPE reactivities between the ribozyme forms containing all-RNA and deoxycytidine-modified substrates in the J4/2 region were detected, pointing to different ribozyme conformations before and after the cleavage event. © 2013 The Authors Journal compilation © 2013 FEBS.

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Wrzesinski, J., Błaszczyk, L., Wrońska, M., Kasprowicz, A., Stokowa-Sołtys, K., Nagaj, J., … Ciesiołka, J. (2013). Mapping the interactions of selected antibiotics and their Cu2+ complexes with the antigenomic delta ribozyme. FEBS Journal, 280(11), 2652–2664. https://doi.org/10.1111/febs.12257

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