2007
DOI: 10.1093/nar/gkm143
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RNase T1 mimicking artificial ribonuclease

Abstract: Recently, artificial ribonucleases (aRNases)—conjugates of oligodeoxyribonucleotides and peptide (LR)4-G-amide—were designed and assessed in terms of the activity and specificity of RNA cleavage. The conjugates were shown to cleave RNA at Pyr-A and G–X sequences. Variations of oligonucleotide length and sequence, peptide and linker structure led to the development of conjugates exhibiting G–X cleavage specificity only. The most efficient catalyst is built of nonadeoxyribonucleotide of unique sequence and pepti… Show more

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Cited by 31 publications
(40 citation statements)
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“…This suggests that, in the absence of complementarity, conjugate 5'-luc-h-9/14 behaves as a usual non-specific ribonuclease, which we observed in earlier works [76,77]. This could be attributed to some type of opportunistic cleavage during transient electrostatic interactions or imperfect hydrogen bonding between the ribonuclease and RNA substrate.…”
Section: Ribonuclease Activity Of Control Non-complementary Pocs Agaisupporting
confidence: 54%
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“…This suggests that, in the absence of complementarity, conjugate 5'-luc-h-9/14 behaves as a usual non-specific ribonuclease, which we observed in earlier works [76,77]. This could be attributed to some type of opportunistic cleavage during transient electrostatic interactions or imperfect hydrogen bonding between the ribonuclease and RNA substrate.…”
Section: Ribonuclease Activity Of Control Non-complementary Pocs Agaisupporting
confidence: 54%
“…Our recent data [50,51,76,77] and 5'-h-9/16 POCs, the antisense part of the conjugate was elongated from 14 to 16 nucleotide residues thus leading to shortening of the target single-stranded region of miR-21 within the hybridized complex. It was shown earlier [51] that narrowing of the RNA single-stranded target region upon binding with the conjugate may result in substantial decrease or even complete loss of catalytic activity, presumably due to reduced conformational freedom for the catalytic peptide.…”
Section: Discussionmentioning
confidence: 95%
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“…The reaction products were resolved by electrophoresis in 15% PAA, 8 M urea gels using TBE (10 mM Tris borate (pH 8.3), and 2 mM EDTA) as a running buffer. As nucleotide size markers, an imidazole ladder or a G-ladder produced by partial RNA cleavage by 2 M imidazole or RNase T1, respectively, was used (22,23). For the analysis of the RNA product 5Ј-end, after RNase reaction, RNA products were precipitated by 2% LiClO 4 , washed by acetone, dried, dissolved in Milli-Q water, and phosphorylated with [␥-32 P]ATP and T4 PNK using conditions for forward or phosphate exchange reaction according to the manufacturer's protocol (Fermentas).…”
Section: Methodsmentioning
confidence: 99%