Toxic protein expression in Escherichia coli using a rhamnose-based tightly regulated and tunable promoter system

Author:

Giacalone Matthew J.1,Gentile Angela M.2,Lovitt Brian T.2,Berkley Neil L.2,Gunderson Carl W.1,Surber Mark W.2

Affiliation:

1. San Diego State University, San Diego

2. Mpex Pharmaceuticals, San Diego, CA, USA

Abstract

The refinement of tightly regulated prokaryotic expression systems that permit functional expression of toxic recombinant proteins is a continually evolving process. Unfortunately, the current best promoter options are either tightly repressed and produce little protein, or produce substantial protein but lack the necessary repression to avoid mutations stimulated by leaky expression in the absence ofinducer. In this report, we present three novel prokaryotic expression constructs that are tightly regulated by L-rhamnose and D-glucose. These expression vectors utilize the Escherichia coli rhaT promoter and corresponding regulatory genes to provide titratable, high-level protein yield without compromising clone integrity. Together, these components may enable the stable cloning and functional expression of otherwise toxic proteins.

Publisher

Future Science Ltd

Subject

General Biochemistry, Genetics and Molecular Biology,Biotechnology

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