Effect of DNA Glycosylases OGG1 and Neil1 on Oxidized G-Rich Motif in the <i>KRAS</i> Promoter

The promoter of the <i>Kirsten ras</i> (<i>KRAS</i>) proto-oncogene contains, upstream of the transcription start site, a quadruplex-forming motif called 32R with regulatory functions. As guanine under oxidative stress can be oxidized to 8-oxoguanine (8OG), we investigated th...

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Main Authors: Annalisa Ferino, Luigi E. Xodo
Format: Article
Language:English
Published: MDPI AG 2021-01-01
Series:International Journal of Molecular Sciences
Subjects:
Online Access:https://www.mdpi.com/1422-0067/22/3/1137
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spelling doaj-6a4bf286ad0b4acb8117d234125e3eea2021-01-25T00:02:09ZengMDPI AGInternational Journal of Molecular Sciences1661-65961422-00672021-01-01221137113710.3390/ijms22031137Effect of DNA Glycosylases OGG1 and Neil1 on Oxidized G-Rich Motif in the <i>KRAS</i> PromoterAnnalisa Ferino0Luigi E. Xodo1Laboratory of Biochemistry, Department of Medicine, P.le Kolbe 4, 33100 Udine, ItalyLaboratory of Biochemistry, Department of Medicine, P.le Kolbe 4, 33100 Udine, ItalyThe promoter of the <i>Kirsten ras</i> (<i>KRAS</i>) proto-oncogene contains, upstream of the transcription start site, a quadruplex-forming motif called 32R with regulatory functions. As guanine under oxidative stress can be oxidized to 8-oxoguanine (8OG), we investigated the capacity of glycosylases 8-oxoguanine glycosylase (OGG1) and endonuclease VIII-like 1 (Neil1) to excise 8OG from 32R, either in duplex or G-quadruplex (G4) conformation. We found that OGG1 efficiently excised 8OG from oxidized 32R in duplex but not in G4 conformation. By contrast, glycosylase Neil1 showed more activity on the G4 than the duplex conformation. We also found that the excising activity of Neil1 on folded 32R depended on G4 topology. Our data suggest that Neil1, besides being involved in base excision repair pathway (BER), could play a role on <i>KRAS</i> transcription.https://www.mdpi.com/1422-0067/22/3/1137G4 DNAOGG1Neil18-oxoguanine<i>KRAS</i>
collection DOAJ
language English
format Article
sources DOAJ
author Annalisa Ferino
Luigi E. Xodo
spellingShingle Annalisa Ferino
Luigi E. Xodo
Effect of DNA Glycosylases OGG1 and Neil1 on Oxidized G-Rich Motif in the <i>KRAS</i> Promoter
International Journal of Molecular Sciences
G4 DNA
OGG1
Neil1
8-oxoguanine
<i>KRAS</i>
author_facet Annalisa Ferino
Luigi E. Xodo
author_sort Annalisa Ferino
title Effect of DNA Glycosylases OGG1 and Neil1 on Oxidized G-Rich Motif in the <i>KRAS</i> Promoter
title_short Effect of DNA Glycosylases OGG1 and Neil1 on Oxidized G-Rich Motif in the <i>KRAS</i> Promoter
title_full Effect of DNA Glycosylases OGG1 and Neil1 on Oxidized G-Rich Motif in the <i>KRAS</i> Promoter
title_fullStr Effect of DNA Glycosylases OGG1 and Neil1 on Oxidized G-Rich Motif in the <i>KRAS</i> Promoter
title_full_unstemmed Effect of DNA Glycosylases OGG1 and Neil1 on Oxidized G-Rich Motif in the <i>KRAS</i> Promoter
title_sort effect of dna glycosylases ogg1 and neil1 on oxidized g-rich motif in the <i>kras</i> promoter
publisher MDPI AG
series International Journal of Molecular Sciences
issn 1661-6596
1422-0067
publishDate 2021-01-01
description The promoter of the <i>Kirsten ras</i> (<i>KRAS</i>) proto-oncogene contains, upstream of the transcription start site, a quadruplex-forming motif called 32R with regulatory functions. As guanine under oxidative stress can be oxidized to 8-oxoguanine (8OG), we investigated the capacity of glycosylases 8-oxoguanine glycosylase (OGG1) and endonuclease VIII-like 1 (Neil1) to excise 8OG from 32R, either in duplex or G-quadruplex (G4) conformation. We found that OGG1 efficiently excised 8OG from oxidized 32R in duplex but not in G4 conformation. By contrast, glycosylase Neil1 showed more activity on the G4 than the duplex conformation. We also found that the excising activity of Neil1 on folded 32R depended on G4 topology. Our data suggest that Neil1, besides being involved in base excision repair pathway (BER), could play a role on <i>KRAS</i> transcription.
topic G4 DNA
OGG1
Neil1
8-oxoguanine
<i>KRAS</i>
url https://www.mdpi.com/1422-0067/22/3/1137
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