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Editor's Pick Experimental Therapeutics

Optimization of a Noncanonical Anti-infective: Interrogation of the Target Binding Pocket for a Small-Molecule Inhibitor of Escherichia coli Polysaccharide Capsule Expression

Mehreen Arshad, Grace A. Beggs, Richard G. Brennan, Patrick C. Seed
Mehreen Arshad
aDepartment of Pediatrics, Duke University School of Medicine, Durham, North Carolina, USA
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Grace A. Beggs
bDepartment of Biochemistry, Duke University School of Medicine, Durham, North Carolina, USA
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Richard G. Brennan
bDepartment of Biochemistry, Duke University School of Medicine, Durham, North Carolina, USA
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Patrick C. Seed
aDepartment of Pediatrics, Duke University School of Medicine, Durham, North Carolina, USA
cDepartment of Molecular Genetics and Microbiology, Duke University School of Medicine, Durham, North Carolina, USA
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DOI: 10.1128/AAC.01208-20
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ABSTRACT

We previously identified a small-molecule inhibitor of capsule biogenesis (designated DU011) and identified its target as MprA, a MarR family transcriptional repressor of multidrug efflux pumps. Unlike other proposed MprA ligands, such as salicylate and 2,4-dinitrophenol (DNP), DU011 does not alter Escherichia coli antibiotic resistance and has significantly enhanced inhibition of capsule expression. We hypothesized that the potency and the unique action of DU011 are due to novel interactions with the MprA binding pocket and the conformation assumed by MprA upon binding DU011 relative to other ligands. To understand the dynamics of MprA-DU011 interaction, we performed hydrogen-deuterium exchange mass spectrometry (HDX-MS); this suggested that four peptide regions undergo conformational changes upon binding DU011. We conducted isothermal calorimetric titration (ITC) to quantitatively characterize MprA binding to DU011 and canonical ligands and observed a distinct two-site binding isotherm associated with the binding reaction of MprA to DU011; however, salicylate and DNP showed a one-site binding isotherm with lower affinity. To elucidate the binding pocket(s) of MprA, we selected single point mutants of MprA that included mutated residues predicted to be within the putative binding pocket (Q51A, F58A, and E65D) as well as on or near the DNA-binding domain (L81A, S83T, and T86A). Our ITC studies suggest that two of the tested MprA mutants had lower affinity for DU011: Q51A and F58A. In addition to elucidating the MprA binding pocket for DU011, we studied the binding of these mutants to salicylate and DNP to reveal the binding pockets of these canonical ligands.

FOOTNOTES

    • Received 15 June 2020.
    • Returned for modification 10 July 2020.
    • Accepted 13 October 2020.
    • Accepted manuscript posted online 19 October 2020.
  • Supplemental material is available online only.

  • Copyright © 2020 American Society for Microbiology.

All Rights Reserved.

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Optimization of a Noncanonical Anti-infective: Interrogation of the Target Binding Pocket for a Small-Molecule Inhibitor of Escherichia coli Polysaccharide Capsule Expression
Mehreen Arshad, Grace A. Beggs, Richard G. Brennan, Patrick C. Seed
Antimicrobial Agents and Chemotherapy Dec 2020, 65 (1) e01208-20; DOI: 10.1128/AAC.01208-20

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Optimization of a Noncanonical Anti-infective: Interrogation of the Target Binding Pocket for a Small-Molecule Inhibitor of Escherichia coli Polysaccharide Capsule Expression
Mehreen Arshad, Grace A. Beggs, Richard G. Brennan, Patrick C. Seed
Antimicrobial Agents and Chemotherapy Dec 2020, 65 (1) e01208-20; DOI: 10.1128/AAC.01208-20
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KEYWORDS

Escherichia coli
MarR family
isothermal titration calorimetry
small-molecule inhibitor

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