Systematic engineering of plant cytochrome P450 system identifies a comprehensive strategy for expression of highly functional P450 enzymes inEscherichia coli

Author:

Poborsky MichalORCID,Crocoll ChristophORCID,Motawie Mohammed SaddikORCID,Halkier Barbara AnnORCID

Abstract

AbstractCytochrome P450s catalyse diverse and unique chemical reactions, which makes them invaluable enzymes in nature and industry. Metabolic engineers leverage these unique catalytic properties when refactoring plant biosynthetic pathways into microbial cell factories. However, due to their hydrophobic anchor, microbial expression of membrane-bound cytochrome P450s is challenging. An arsenal of protein engineering strategies was developed to improve their expression inEscherichia coli, but extensive screening is often necessary to tailor the engineering approach to an individual enzyme. Here, we propose a universal strategy that allows the expression of highly active cytochrome P450s inE. coliby systematically evaluating six common N-terminal modifications and their effect onin vivoactivity of enzymes from the CYP79 and CYP83 families. We identified transmembrane domain truncation as the only strategy that had a significantly positive effect on all seven tested enzymes, increasing product titres between 2- to 170-fold. When comparing the changes in protein titre and product generation, we show that higher expression does not always translate to higherin vivoactivity, thus making protein titre an unreliable screening target. Our results demonstrate that transmembrane domain truncation improvesin vivoactivity across a broad range of cytochrome P450s with diverse N-terminal sequences and could be applied as the modification-of-choice to avoid the time-consuming screening process and accelerate the future design ofE. colicell factories.

Publisher

Cold Spring Harbor Laboratory

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