<HashMap><database>biostudies-literature</database><scores/><additional><submitter>Conlon SG</submitter><funding>Division of Chemistry</funding><funding>University of California Institute for Mexico and the United States</funding><funding>NIEHS NIH HHS</funding><funding>Achievement Rewards for College Scientists Foundation</funding><funding>National Cancer Institute</funding><funding>NCI NIH HHS</funding><funding>Consejo Nacional de Ciencia y Tecnolog?a</funding><funding>University of California, Davis</funding><pagination>291-301</pagination><full_dataset_link>https://www.ebi.ac.uk/biostudies/studies/S-EPMC10906249</full_dataset_link><repository>biostudies-literature</repository><omics_type>Unknown</omics_type><volume>10(2)</volume><pubmed_abstract>The base excision repair glycosylase MUTYH prevents mutations associated with the oxidatively damaged base, 8-oxo-7,8-dihydroguanine (OG), by removing &lt;i>undamaged&lt;/i> misincorporated adenines from OG:A mispairs. Defects in OG:A repair in individuals with inherited MUTYH variants are correlated with the colorectal cancer predisposition syndrome known as &lt;i>MUTYH&lt;/i>-associated polyposis (MAP). Herein, we reveal key structural features of OG required for efficient repair by human MUTYH using structure-activity relationships (SAR). We developed a GFP-based plasmid reporter assay to define SAR with synthetically generated OG analogs in human cell lines. Cellular repair results were compared with kinetic parameters measured by adenine glycosylase assays &lt;i>in vitro&lt;/i>. Our results show substrates lacking the 2-amino group of OG, such as 8OI:A (8OI = 8-oxoinosine), are not repaired in cells, despite being excellent substrates in &lt;i>in vitro&lt;/i> adenine glycosylase assays, new evidence that the search and detection steps are critical factors in cellular MUTYH repair functionality. Surprisingly, modification of the O8/N7H of OG, which is the distinguishing feature of OG relative to G, was tolerated in both MUTYH-mediated cellular repair and &lt;i>in vitro&lt;/i> adenine glycosylase activity. The lack of sensitivity to alterations at the O8/N7H in the SAR of MUTYH substrates is distinct from previous work with bacterial MutY, indicating that the human enzyme is much less stringent in its lesion verification. Our results imply that the human protein relies almost exclusively on detection of the unique major groove position of the 2-amino group of OG within OG&lt;sub>&lt;i>syn&lt;/i>&lt;/sub>:A&lt;sub>&lt;i>anti&lt;/i>&lt;/sub> mispairs to select contextually incorrect adenines for excision and thereby thwart mutagenesis. These results predict that MUTYH variants that exhibit deficiencies in OG:A detection will be severely compromised in a cellular setting. Moreover, the reliance of MUTYH on the interaction with the OG 2-amino group suggests that disrupting this interaction with small molecules may provide a strategy to develop potent and selective MUTYH inhibitors.</pubmed_abstract><journal>ACS central science</journal><pubmed_title>Cellular Repair of Synthetic Analogs of Oxidative DNA Damage Reveals a Key Structure-Activity Relationship of the Cancer-Associated MUTYH DNA Repair Glycosylase.</pubmed_title><pmcid>PMC10906249</pmcid><funding_grant_id>R29 CA067985</funding_grant_id><funding_grant_id>R01 CA067985</funding_grant_id><funding_grant_id>T32 ES007059</funding_grant_id><funding_grant_id>P30 CA093373</funding_grant_id><funding_grant_id>CA067985</funding_grant_id><funding_grant_id>1903855</funding_grant_id><pubmed_authors>Trasvina-Arenas CH</pubmed_authors><pubmed_authors>David SS</pubmed_authors><pubmed_authors>Conlon SG</pubmed_authors><pubmed_authors>Raetz AG</pubmed_authors><pubmed_authors>Khuu C</pubmed_authors><pubmed_authors>Xia T</pubmed_authors><pubmed_authors>Hamm ML</pubmed_authors></additional><is_claimable>false</is_claimable><name>Cellular Repair of Synthetic Analogs of Oxidative DNA Damage Reveals a Key Structure-Activity Relationship of the Cancer-Associated MUTYH DNA Repair Glycosylase.</name><description>The base excision repair glycosylase MUTYH prevents mutations associated with the oxidatively damaged base, 8-oxo-7,8-dihydroguanine (OG), by removing &lt;i>undamaged&lt;/i> misincorporated adenines from OG:A mispairs. Defects in OG:A repair in individuals with inherited MUTYH variants are correlated with the colorectal cancer predisposition syndrome known as &lt;i>MUTYH&lt;/i>-associated polyposis (MAP). Herein, we reveal key structural features of OG required for efficient repair by human MUTYH using structure-activity relationships (SAR). We developed a GFP-based plasmid reporter assay to define SAR with synthetically generated OG analogs in human cell lines. Cellular repair results were compared with kinetic parameters measured by adenine glycosylase assays &lt;i>in vitro&lt;/i>. Our results show substrates lacking the 2-amino group of OG, such as 8OI:A (8OI = 8-oxoinosine), are not repaired in cells, despite being excellent substrates in &lt;i>in vitro&lt;/i> adenine glycosylase assays, new evidence that the search and detection steps are critical factors in cellular MUTYH repair functionality. Surprisingly, modification of the O8/N7H of OG, which is the distinguishing feature of OG relative to G, was tolerated in both MUTYH-mediated cellular repair and &lt;i>in vitro&lt;/i> adenine glycosylase activity. The lack of sensitivity to alterations at the O8/N7H in the SAR of MUTYH substrates is distinct from previous work with bacterial MutY, indicating that the human enzyme is much less stringent in its lesion verification. Our results imply that the human protein relies almost exclusively on detection of the unique major groove position of the 2-amino group of OG within OG&lt;sub>&lt;i>syn&lt;/i>&lt;/sub>:A&lt;sub>&lt;i>anti&lt;/i>&lt;/sub> mispairs to select contextually incorrect adenines for excision and thereby thwart mutagenesis. These results predict that MUTYH variants that exhibit deficiencies in OG:A detection will be severely compromised in a cellular setting. Moreover, the reliance of MUTYH on the interaction with the OG 2-amino group suggests that disrupting this interaction with small molecules may provide a strategy to develop potent and selective MUTYH inhibitors.</description><dates><release>2024-01-01T00:00:00Z</release><publication>2024 Feb</publication><modification>2026-04-08T19:52:49.235Z</modification><creation>2025-04-06T17:15:19.499Z</creation></dates><accession>S-EPMC10906249</accession><cross_references><pubmed>38435525</pubmed><doi>10.1021/acscentsci.3c00784</doi></cross_references></HashMap>