Engineered transcription activator-like effector dimer proteins confer DNA loop-dependent gene repression comparable to Lac repressor

Author:

Becker Nicole A1,Peters Justin P2,Lewis Elizabeth1,Daby Camden L1,Clark Karl13,Maher L James1ORCID

Affiliation:

1. Department of Biochemistry and Molecular Biology, Mayo Clinic College of Medicine and Science , Rochester , MN 55905 , USA

2. Department of Chemistry and Biochemistry, University of Northern Iowa , Cedar Falls , IA 50614 , USA

3. Department of Animal Science, Texas A&M University, College Station , TX 77843 , USA

Abstract

Abstract Natural prokaryotic gene repression systems often exploit DNA looping to increase the local concentration of gene repressor proteins at a regulated promoter via contributions from repressor proteins bound at distant sites. Using principles from the Escherichia coli lac operon we design analogous repression systems based on target sequence-programmable Transcription Activator-Like Effector dimer (TALED) proteins. Such engineered switches may be valuable for synthetic biology and therapeutic applications. Previous TALEDs with inducible non-covalent dimerization showed detectable, but limited, DNA loop-based repression due to the repressor protein dimerization equilibrium. Here, we show robust DNA loop-dependent bacterial promoter repression by covalent TALEDs and verify that DNA looping dramatically enhances promoter repression in E. coli. We characterize repression using a thermodynamic model that quantitates this favorable contribution of DNA looping. This analysis unequivocally and quantitatively demonstrates that optimized TALED proteins can drive loop-dependent promoter repression in E. coli comparable to the natural LacI repressor system. This work elucidates key design principles that set the stage for wide application of TALED-dependent DNA loop-based repression of target genes.

Funder

Mayo Foundation

NIH

Mayo Clinic College of Medicine and Science

Publisher

Oxford University Press (OUP)

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