Dynamics of Methylated Cytosine Flipping by UHRF1

DNA methylation patterns, which are critical for gene expression, are replicated by DNA methyltransferase 1 (DNMT1) and ubiquitin-like containing PHD and RING finger domains 1 (UHRF1) proteins. This replication is initiated by the recognition of hemimethylated CpG sites and further flipping of methy...

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Veröffentlicht in:	Journal of the American Chemical Society 2017-02, Vol.139 (6), p.2520-2528
Hauptverfasser:	Kilin, Vasyl, Gavvala, Krishna, Barthes, Nicolas P. F, Michel, Benoît Y, Shin, Dongwon, Boudier, Christian, Mauffret, Olivier, Yashchuk, Valeriy, Mousli, Marc, Ruff, Marc, Granger, Florence, Eiler, Sylvia, Bronner, Christian, Tor, Yitzhak, Burger, Alain, Mély, Yves
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Schlagworte:	CCAAT-Enhancer-Binding Proteins - chemistry CCAAT-Enhancer-Binding Proteins - metabolism Cytosine - chemistry Cytosine - metabolism DNA - chemistry DNA - metabolism DNA Methylation DNA Replication Fluorescence Humans Kinetics Life Sciences Molecular Structure Thermodynamics Ubiquitin-Protein Ligases
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creator	Kilin, Vasyl Gavvala, Krishna Barthes, Nicolas P. F Michel, Benoît Y Shin, Dongwon Boudier, Christian Mauffret, Olivier Yashchuk, Valeriy Mousli, Marc Ruff, Marc Granger, Florence Eiler, Sylvia Bronner, Christian Tor, Yitzhak Burger, Alain Mély, Yves
description	DNA methylation patterns, which are critical for gene expression, are replicated by DNA methyltransferase 1 (DNMT1) and ubiquitin-like containing PHD and RING finger domains 1 (UHRF1) proteins. This replication is initiated by the recognition of hemimethylated CpG sites and further flipping of methylated cytosines (mC) by the Set and Ring Associated (SRA) domain of UHRF1. Although crystallography has shed light on the mechanism of mC flipping by SRA, tools are required to monitor in real time how SRA reads DNA and flips the modified nucleobase. To accomplish this aim, we have utilized two distinct fluorescent nucleobase surrogates, 2-thienyl-3-hydroxychromone nucleoside (3HCnt) and thienoguanosine (thG), incorporated at different positions into hemimethylated (HM) and nonmethylated (NM) DNA duplexes. Large fluorescence changes were associated with mC flipping in HM duplexes, showing the outstanding sensitivity of both nucleobase surrogates to the small structural changes accompanying base flipping. Importantly, the nucleobase surrogates marginally affected the structure of the duplex and its affinity for SRA at positions where they were responsive to base flipping, illustrating their promise as nonperturbing probes for monitoring such events. Stopped-flow studies using these two distinct tools revealed the fast kinetics of SRA binding and sliding to NM duplexes, consistent with its reader role. In contrast, the kinetics of mC flipping was found to be much slower in HM duplexes, substantially increasing the lifetime of CpG-bound UHRF1, and thus the probability of recruiting DNMT1 to faithfully duplicate the DNA methylation profile. The fluorescence-based approach using these two different fluorescent nucleoside surrogates advances the mechanistic understanding of the UHRF1/DNMT1 tandem and the development of assays for the identification of base flipping inhibitors.
doi_str_mv	10.1021/jacs.7b00154
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Although crystallography has shed light on the mechanism of mC flipping by SRA, tools are required to monitor in real time how SRA reads DNA and flips the modified nucleobase. To accomplish this aim, we have utilized two distinct fluorescent nucleobase surrogates, 2-thienyl-3-hydroxychromone nucleoside (3HCnt) and thienoguanosine (thG), incorporated at different positions into hemimethylated (HM) and nonmethylated (NM) DNA duplexes. Large fluorescence changes were associated with mC flipping in HM duplexes, showing the outstanding sensitivity of both nucleobase surrogates to the small structural changes accompanying base flipping. Importantly, the nucleobase surrogates marginally affected the structure of the duplex and its affinity for SRA at positions where they were responsive to base flipping, illustrating their promise as nonperturbing probes for monitoring such events. Stopped-flow studies using these two distinct tools revealed the fast kinetics of SRA binding and sliding to NM duplexes, consistent with its reader role. In contrast, the kinetics of mC flipping was found to be much slower in HM duplexes, substantially increasing the lifetime of CpG-bound UHRF1, and thus the probability of recruiting DNMT1 to faithfully duplicate the DNA methylation profile. 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F</creatorcontrib><creatorcontrib>Michel, Benoît Y</creatorcontrib><creatorcontrib>Shin, Dongwon</creatorcontrib><creatorcontrib>Boudier, Christian</creatorcontrib><creatorcontrib>Mauffret, Olivier</creatorcontrib><creatorcontrib>Yashchuk, Valeriy</creatorcontrib><creatorcontrib>Mousli, Marc</creatorcontrib><creatorcontrib>Ruff, Marc</creatorcontrib><creatorcontrib>Granger, Florence</creatorcontrib><creatorcontrib>Eiler, Sylvia</creatorcontrib><creatorcontrib>Bronner, Christian</creatorcontrib><creatorcontrib>Tor, Yitzhak</creatorcontrib><creatorcontrib>Burger, Alain</creatorcontrib><creatorcontrib>Mély, Yves</creatorcontrib><title>Dynamics of Methylated Cytosine Flipping by UHRF1</title><title>Journal of the American Chemical Society</title><addtitle>J. Am. Chem. Soc</addtitle><description>DNA methylation patterns, which are critical for gene expression, are replicated by DNA methyltransferase 1 (DNMT1) and ubiquitin-like containing PHD and RING finger domains 1 (UHRF1) proteins. 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This replication is initiated by the recognition of hemimethylated CpG sites and further flipping of methylated cytosines (mC) by the Set and Ring Associated (SRA) domain of UHRF1. Although crystallography has shed light on the mechanism of mC flipping by SRA, tools are required to monitor in real time how SRA reads DNA and flips the modified nucleobase. To accomplish this aim, we have utilized two distinct fluorescent nucleobase surrogates, 2-thienyl-3-hydroxychromone nucleoside (3HCnt) and thienoguanosine (thG), incorporated at different positions into hemimethylated (HM) and nonmethylated (NM) DNA duplexes. Large fluorescence changes were associated with mC flipping in HM duplexes, showing the outstanding sensitivity of both nucleobase surrogates to the small structural changes accompanying base flipping. Importantly, the nucleobase surrogates marginally affected the structure of the duplex and its affinity for SRA at positions where they were responsive to base flipping, illustrating their promise as nonperturbing probes for monitoring such events. Stopped-flow studies using these two distinct tools revealed the fast kinetics of SRA binding and sliding to NM duplexes, consistent with its reader role. In contrast, the kinetics of mC flipping was found to be much slower in HM duplexes, substantially increasing the lifetime of CpG-bound UHRF1, and thus the probability of recruiting DNMT1 to faithfully duplicate the DNA methylation profile. 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subjects	CCAAT-Enhancer-Binding Proteins - chemistry CCAAT-Enhancer-Binding Proteins - metabolism Cytosine - chemistry Cytosine - metabolism DNA - chemistry DNA - metabolism DNA Methylation DNA Replication Fluorescence Humans Kinetics Life Sciences Molecular Structure Thermodynamics Ubiquitin-Protein Ligases
title	Dynamics of Methylated Cytosine Flipping by UHRF1
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