2018
DOI: 10.1021/acs.biochem.8b00277
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Reactivity and Specificity of RNase T1, RNase A, and RNase H toward Oligonucleotides of RNA Containing 8-Oxo-7,8-dihydroguanosine

Abstract: Understanding how oxidatively damaged RNA interacts with ribonucleases is important because of its proposed role in the development and progression of disease. Thus, understanding structural aspects of RNA containing lesions generated under oxidative stress, as well as its interactions with other biopolymers, is fundamental. We explored the reactivity of RNase A, RNase T, and RNase H toward oligonucleotides of RNA containing 8-oxo-7,8-dihydroguanosine (8oxoG). This is the first example that addresses this rela… Show more

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Cited by 13 publications
(11 citation statements)
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“…It can be assumed that the expected H-bonding interactions between 8-oxopurines, in its syn-conformation, and A play a role in this behavior (Fig 8C). This is also in agreement with 8-oxoG exhibiting H-bonding interactions as Uridine, arising from a conformational change around the glycosidic bond, in other enzymatic contexts [53]. Interestingly, the corresponding 8-oxoI analogue also allowed for incorporation of dC and dA, with higher efficiency in the presence of dATP (app.…”
Section: Plos Onesupporting
confidence: 81%
“…It can be assumed that the expected H-bonding interactions between 8-oxopurines, in its syn-conformation, and A play a role in this behavior (Fig 8C). This is also in agreement with 8-oxoG exhibiting H-bonding interactions as Uridine, arising from a conformational change around the glycosidic bond, in other enzymatic contexts [53]. Interestingly, the corresponding 8-oxoI analogue also allowed for incorporation of dC and dA, with higher efficiency in the presence of dATP (app.…”
Section: Plos Onesupporting
confidence: 81%
“…(Figure 1—figure supplement 3) For RNAse of embryos prior to probe hybridization: RNA-FISH to AAGAG was performed on embryos pre-treated with RNaseIII (which cleaves dsRNA; Nicholson, 2014), RNaseH (which cleaves the RNA strand in RNA/DNA hybrids), RNase I (which non-specifically cleaves ssRNA and dsRNA), and RNaseA (which cleaves adjacent to pyrimidines, preferentially in ssRNA, and specifically not between purines such as 5’-AGAAGGGAGAAG [Herbert et al, 2018; Kelemen et al, 2000]). Reaction conditions were as follows: Samples were treated in 50 μl final volume with either RNAseIII: 1X RNAseIII buffer, 1.5 μl Shortcut RNaseIII (New England Biolabs, cat.…”
Section: Methodsmentioning
confidence: 99%
“…To understand the impact of the modification on the structure, all strands were radiolabeled and treated with RNase A, which cleaves single‐stranded RNAs at both pyrimidine and 8‐oxoG sites into fragments containing 5′‐OH and 3′‐phosphate ends . The results were then compared with those obtained with canonical strand 1 .…”
Section: Resultsmentioning
confidence: 99%