Please use this identifier to cite or link to this item: https://doi.org/10.3389/fbioe.2023.1191162
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dc.titleEngineering Escherichia coli for diagnosis and management of hyperuricemia
dc.contributor.authorGencer, Gozde
dc.contributor.authorMancuso, Christopher
dc.contributor.authorChua, Koon Jiew
dc.contributor.authorLing, Hua
dc.contributor.authorCostello, Cait M
dc.contributor.authorChang, Matthew Wook
dc.contributor.authorMarch, John C
dc.date.accessioned2023-06-16T01:05:35Z
dc.date.available2023-06-16T01:05:35Z
dc.date.issued2023-05-23
dc.identifier.citationGencer, Gozde, Mancuso, Christopher, Chua, Koon Jiew, Ling, Hua, Costello, Cait M, Chang, Matthew Wook, March, John C (2023-05-23). Engineering Escherichia coli for diagnosis and management of hyperuricemia. Frontiers in Bioengineering and Biotechnology 11. ScholarBank@NUS Repository. https://doi.org/10.3389/fbioe.2023.1191162
dc.identifier.issn2296-4185
dc.identifier.urihttps://scholarbank.nus.edu.sg/handle/10635/242057
dc.description.abstract<jats:p>Uric acid disequilibrium is implicated in chronic hyperuricemia-related diseases. Long-term monitoring and lowering of serum uric acid levels may be crucial for diagnosis and effective management of these conditions. However, current strategies are not sufficient for accurate diagnosis and successful long-term management of hyperuricemia. Moreover, drug-based therapeutics can cause side effects in patients. The intestinal tract plays an important role in maintaining healthy serum acid levels. Hence, we investigated the engineered human commensal <jats:italic>Escherichia coli</jats:italic> as a novel method for diagnosis and long-term management of hyperuricemia. To monitor changes in uric acid concentration in the intestinal lumen, we developed a bioreporter using the uric acid responsive synthetic promoter, <jats:italic>pucpro</jats:italic>, and uric acid binding <jats:italic>Bacillus subtilis</jats:italic> PucR protein. Results demonstrated that the bioreporter module in commensal <jats:italic>E. coli</jats:italic> can detect changes in uric acid concentration in a dose-dependent manner. To eliminate the excess uric acid, we designed a uric acid degradation module, which overexpresses an <jats:italic>E. coli</jats:italic> uric acid transporter and a <jats:italic>B. subtilis</jats:italic> urate oxidase. Strains engineered with this module degraded all the uric acid (250 µM) found in the environment within 24 h, which is significantly lower (<jats:italic>p</jats:italic> &lt; 0.001) compared to wild type <jats:italic>E. coli</jats:italic>. Finally, we designed an <jats:italic>in vitro</jats:italic> model using human intestinal cell line, Caco-2, which provided a versatile tool to study the uric acid transport and degradation in an environment mimicking the human intestinal tract. Results showed that engineered commensal <jats:italic>E. coli</jats:italic> reduced (<jats:italic>p</jats:italic> &lt; 0.01) the apical uric acid concentration by 40.35% compared to wild type <jats:italic>E. coli</jats:italic>. This study shows that reprogramming <jats:italic>E. coli</jats:italic> holds promise as a valid alternative synthetic biology therapy to monitor and maintain healthy serum uric acid levels.</jats:p>
dc.publisherFrontiers Media SA
dc.sourceElements
dc.typeArticle
dc.date.updated2023-06-15T10:04:11Z
dc.contributor.departmentBIOCHEMISTRY
dc.description.doi10.3389/fbioe.2023.1191162
dc.description.sourcetitleFrontiers in Bioengineering and Biotechnology
dc.description.volume11
dc.published.stateUnpublished
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