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Cleavage of RNA in hybrid duplexes by theE. coli ribonuclease H: II. Substrate properties of oligonucleotides containing nonnucleotide linkers |
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| Authors: | P E Vorobjev I A Pyshnaya D V Pyshnyi M N Repkova A G Venyaminova M A Zenkova E M Ivanova C Scalfi-Happ H Seliger G M Bonora V F Zarytova |
| Institution: | (1) Novosibirsk Institute of Bioorganic Chemistry, Siberian Division, Russian Academy of Sciences, pr. Akademika Lavrent’eva 8, 630090 Novosibirsk, Russia;(2) Section of Polymers, University of Ulm, D-89069 Ulm, Germany;(3) Department of Chemical Sciences, University of Trieste, 1-42127 Trieste, Italy |
| Abstract: | The 20-mer bridged oligodeoxynucleotides containing short oligomers joined by the hexamethylenediol and hexaethylene glycol linkers were shown to form complementary DNA/DNA and RNA/DNA complexes whose thermostability depends on the length and number of the nonnucleotide linkers. Hybrid complexes of the bridged oligonucleotides proved to be substrates for theE. coli ribonuclease H. The presence of one-three nonnucleotide linkers in a 20-mer decreased the hydrolysis efficacy only 1.2–1.4-fold. It is the composition of the RNA cleavage products that was influenced the most significantly by the nonnucleotide linkers. RNase H simultaneously hydrolyzed the RNA 3′-ends of each hybrid duplex involving a bridged oligonucleotide. The presence of an inverted 3′-3′-phosphodiester bond at the 3′-end of the oligodeoxyribonucleotide only slightly affected the RNase H activity. For the previous report, see 1]. |
| Keywords: | antisense oligonucleotides bridged oligonucleotides nonnucleotide insert ribonuclease H phosphodiester bond inversion thermostability of complementary complexes |
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