Establishment of an In Bacterio Assay for the Assessment of Carbon Storage Regulator A (CsrA) Inhibitors

Author:

Wu Yingwen12ORCID,Zoller Ben G. E.1ORCID,Kamal Mohamed Ashraf Mostafa34,Hotop Sven‐Kevin5ORCID,Lehr Claus‐Michael34ORCID,Brönstrup Mark5ORCID,Dersch Petra6ORCID,Empting Martin142ORCID

Affiliation:

1. Department of Antiviral & Antivirulence Drugs (AVID) Helmholtz Institute for Pharmaceutical Research Saarland (HIPS) Saarland University 66123 Saarbrücken Germany

2. Cluster of Excellence RESIST (EXC 2155) Hanover Medical School Carl-Neuberg-Straße 1 30625 Hanover Germany

3. Department of Drug Delivery (DDEL) Helmholtz Institute for Pharmaceutical Research Saarland (HIPS) Saarland University 66123 Saarbrücken Germany

4. Department of Pharmacy Saarland University 66123 Saarbrücken Germany

5. Department of Chemical Biology Helmholtz Centre for Infection Research German Center for Infection Research (DZIF) 38124 Braunschweig Germany

6. Institute of Infectiology Center for Molecular Biology of Inflammation (ZMBE) University of Münster 48149 Münster Germany

Abstract

AbstractPolymicrobial infections involving various combinations of microorganisms, such as Escherichia, Pseudomonas, or Yersinia, can lead to acute and chronic diseases in for example the gastrointestinal and respiratory tracts. Our aim is to modulate microbial communities by targeting the posttranscriptional regulator system called carbon storage regulator A (CsrA) (or also repressor of secondary metabolites (RsmA)). In previous studies, we identified easily accessible CsrA binding scaffolds and macrocyclic CsrA binding peptides through biophysical screening and phage display technology. However, due to the lack of an appropriate in bacterio assay to evaluate the cellular effects of these inhibitor hits, the focus of the present study is to establish an in bacterio assay capable of probing and quantifying the impact on CsrA‐regulated cellular mechanisms. We have successfully developed an assay based on a luciferase reporter gene assay, which in combination with a qPCR expression gene assay, allows for the monitoring of expression levels of different downstream targets of CsrA. The chaperone protein CesT was used as a suitable positive control for the assay, and in time‐dependent experiments, we observed a CesT‐mediated increase in bioluminescence over time. By this means, the cellular on‐target effects of non‐bactericidal/non‐bacteriostatic virulence modulating compounds targeting CsrA/RsmA can be evaluated.

Publisher

Wiley

Subject

Organic Chemistry,Molecular Biology,Molecular Medicine,Biochemistry

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