A suppressor tRNA-mediated feedforward loop eliminates leaky gene expression in bacteria

Author:

Ho Joanne M L1ORCID,Miller Corwin A1,Parks Sydney E1,Mattia Jacob R1,Bennett Matthew R12ORCID

Affiliation:

1. Department of Biosciences, Rice University MS-140, 6100 Main St., Houston, TX 77005, USA

2. Department of Bioengineering, Rice University MS-140, 6100 Main St. Houston, TX 77005, USA

Abstract

Abstract Ligand-inducible genetic systems are the mainstay of synthetic biology, allowing gene expression to be controlled by the presence of a small molecule. However, ‘leaky’ gene expression in the absence of inducer remains a persistent problem. We developed a leak dampener tool that drastically reduces the leak of inducible genetic systems while retaining signal in Escherichia coli. Our system relies on a coherent feedforward loop featuring a suppressor tRNA that enables conditional readthrough of silent non-sense mutations in a regulated gene, and this approach can be applied to any ligand-inducible transcription factor. We demonstrate proof-of-principle of our system with the lactate biosensor LldR and the arabinose biosensor AraC, which displayed a 70-fold and 630-fold change in output after induction of a fluorescence reporter, respectively, without any background subtraction. Application of the tool to an arabinose-inducible mutagenesis plasmid led to a 540-fold change in its output after induction, with leak decreasing to the level of background mutagenesis. This study provides a modular tool for reducing leak and improving the fold-induction within genetic circuits, demonstrated here using two types of biosensors relevant to cancer detection and genetic engineering.

Funder

National Sciences Foundation

National Institutes of Health

Robert A. Welch Foundation

Publisher

Oxford University Press (OUP)

Subject

Genetics

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