4.4 Article

Optochemical Control of Bacterial Gene Expression: Novel Photocaged Compounds for Different Promoter Systems

Journal

CHEMBIOCHEM
Volume 23, Issue 1, Pages -

Publisher

WILEY-V C H VERLAG GMBH
DOI: 10.1002/cbic.202100467

Keywords

caged compounds; gene expression; optogenetics; photochemistry; synthetic biology

Funding

  1. Bioeconomy Science Center
  2. Ministry of Culture and Science of the German federal state of North Rhine-Westphalia MKW [313/323-400-00213]
  3. Projekt DEAL

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Research on the use of photocaged compounds for controlling gene expression in bacteria synthesized six photocaged carbohydrates, successfully applied in E. coli. The study found that carbonate and carbamate bonds were convenient for linkage, and also discussed challenges and potential solutions during both photocaged inducer synthesis and application.
Photocaged compounds are applied for implementing precise, optochemical control of gene expression in bacteria. To broaden the scope of UV-light-responsive inducer molecules, six photocaged carbohydrates were synthesized and photochemically characterized, with the absorption exhibiting a red-shift. Their differing linkage through ether, carbonate, and carbamate bonds revealed that carbonate and carbamate bonds are convenient. Subsequently, those compounds were successfully applied in vivo for controlling gene expression in E. coli via blue light illumination. Furthermore, benzoate-based expression systems were subjected to light control by establishing a novel photocaged salicylic acid derivative. Besides its synthesis and in vitro characterization, we demonstrate the challenging choice of a suitable promoter system for light-controlled gene expression in E. coli. We illustrate various bottlenecks during both photocaged inducer synthesis and in vivo application and possibilities to overcome them. These findings pave the way towards novel caged inducer-dependent systems for wavelength-selective gene expression.

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