Статья

Site-Selective Artificial Ribonucleases: Renaissance of Oligonucleotide Conjugates for Irreversible Cleavage of RNA Sequences

Y. Staroseletz, S. Gaponova, O. Patutina, E. Bichenkova, B. Amirloo, T. Heyman, D. Chiglintseva, M. Zenkova,
2021

RNA-targeting therapeutics require highly efficient sequence-specific devices capable of RNA irreversible degradation in vivo. The most developed methods of sequence-specific RNA cleavage, such as siRNA or antisense oligonucleotides (ASO), are currently based on recruitment of either intracellular multi-protein complexes or enzymes, leaving alternative approaches (e.g., ribozymes and DNAzymes) far behind. Recently, site-selective artificial ribonucleases combining the oligonucleotide recognition motifs (or their structural analogues) and catalytically active groups in a single molecular scaffold have been proven to be a great competitor to siRNA and ASO. Using the most efficient catalytic groups, utilising both metal ion-dependent (Cu(II)-2,9-dimethylphenanthroline) and metal ion-free (Tris(2-aminobenzimidazole)) on the one hand and PNA as an RNA recognising oligonucleotide on the other, allowed site-selective artificial RNases to be created with half-lives of 0.5-1 h. Artificial RNases based on the catalytic peptide [(ArgLeu)2Gly]2 were able to take progress a step further by demonstrating an ability to cleave miRNA-21 in tumour cells and provide a significant reduction of tumour growth in mice.

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  • 1. Version of Record от 2021-03-19

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Об авторах
  • Y. Staroseletz
    Laboratory of Nucleic Acids Biochemistry, Institute of Chemical Biology and Fundamental Medicine SB RAS, Lavrentiev’s Ave. 8, 630090 Novosibirsk, Russia;, staroselec@ngs.ru, (Y.S.);, sveta-mira@yandex.ru, (S.G.);, patutina@niboch.nsc.ru, (O.P.);, dashachiglintseva@gmail.com, (D.C.)
  • S. Gaponova
    Laboratory of Nucleic Acids Biochemistry, Institute of Chemical Biology and Fundamental Medicine SB RAS, Lavrentiev’s Ave. 8, 630090 Novosibirsk, Russia;, staroselec@ngs.ru, (Y.S.);, sveta-mira@yandex.ru, (S.G.);, patutina@niboch.nsc.ru, (O.P.);, dashachiglintseva@gmail.com, (D.C.)
  • O. Patutina
    Laboratory of Nucleic Acids Biochemistry, Institute of Chemical Biology and Fundamental Medicine SB RAS, Lavrentiev’s Ave. 8, 630090 Novosibirsk, Russia;, staroselec@ngs.ru, (Y.S.);, sveta-mira@yandex.ru, (S.G.);, patutina@niboch.nsc.ru, (O.P.);, dashachiglintseva@gmail.com, (D.C.)
  • E. Bichenkova
    School of Health Sciences, Faculty of Biology, Medicine and Health, University of Manchester, Oxford Rd., Manchester M13 9PT, UK;, Elena.V.Bichenkova@manchester.ac.uk, (E.B.);, bahareh.amirloo@manchester.ac.uk, (B.A.);, thomas.heyman@manchester.ac.uk, (T.H.)
  • B. Amirloo
    School of Health Sciences, Faculty of Biology, Medicine and Health, University of Manchester, Oxford Rd., Manchester M13 9PT, UK;, Elena.V.Bichenkova@manchester.ac.uk, (E.B.);, bahareh.amirloo@manchester.ac.uk, (B.A.);, thomas.heyman@manchester.ac.uk, (T.H.)
  • T. Heyman
    School of Health Sciences, Faculty of Biology, Medicine and Health, University of Manchester, Oxford Rd., Manchester M13 9PT, UK;, Elena.V.Bichenkova@manchester.ac.uk, (E.B.);, bahareh.amirloo@manchester.ac.uk, (B.A.);, thomas.heyman@manchester.ac.uk, (T.H.)
  • D. Chiglintseva
    Laboratory of Nucleic Acids Biochemistry, Institute of Chemical Biology and Fundamental Medicine SB RAS, Lavrentiev’s Ave. 8, 630090 Novosibirsk, Russia;, staroselec@ngs.ru, (Y.S.);, sveta-mira@yandex.ru, (S.G.);, patutina@niboch.nsc.ru, (O.P.);, dashachiglintseva@gmail.com, (D.C.)
  • M. Zenkova
    Laboratory of Nucleic Acids Biochemistry, Institute of Chemical Biology and Fundamental Medicine SB RAS, Lavrentiev’s Ave. 8, 630090 Novosibirsk, Russia;, staroselec@ngs.ru, (Y.S.);, sveta-mira@yandex.ru, (S.G.);, patutina@niboch.nsc.ru, (O.P.);, dashachiglintseva@gmail.com, (D.C.)
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  • Molecules
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