4.7 Article

Macrolide Biosensor Optimization through Cellular Substrate Sequestration

Journal

ACS SYNTHETIC BIOLOGY
Volume 10, Issue 2, Pages 258-264

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/acssynbio.0c00572

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Funding

  1. National Institutes of Health [R01GM117138]
  2. National Science Foundation [MCB-1936774]
  3. Welch Foundation [C-1729]

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This study successfully improved the sensitivity of biosensors for erythromycin by trapping the target molecule within cells, allowing for detection at very low concentrations. The strategy also shows potential for use with a range of macrolide substrates, indicating promise for drug development and metabolic engineering applications. Future studies could further extend this strategy to enhance the sensitivity of other biosensors.
Developing and optimizing small-molecule biosensors is a central goal of synthetic biology. Here we incorporate additional cellular components to improve biosensor sensitivity by preventing target molecules from diffusing out of cells. We demonstrate that trapping erythromycin within Escherichia coli through phosphorylation increases the sensitivity of its biosensor (MphR) by approximately 10-fold. When combined with prior engineering efforts, our optimized biosensor can detect erythromycin concentrations as low as 13 nM. We show that this strategy works with a range of macrolide substrates, enabling the potential usage of our optimized system for drug development and metabolic engineering. This strategy can be extended in future studies to improve the sensitivity of other biosensors. Our findings further suggest that many naturally evolved genes involved in resistance to multiple classes of antibiotics may increase intracellular drug concentrations to modulate their own expression, acting as a form of regulatory feedback.

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