Systematic sequence engineering enhances the induction strength of the glucose-regulated GTH1 promoter of Komagataella phaffii

Author:

Flores-Villegas Mirelle12,Rebnegger Corinna123,Kowarz Viktoria12,Prielhofer Roland2,Mattanovich Diethard123,Gasser Brigitte123ORCID

Affiliation:

1. CD-Laboratory for Growth-decoupled Protein Production in Yeast at Department of Biotechnology, University of Natural Resources and Life Sciences (BOKU) , Vienna , Austria

2. University of Natural Resources and Life Sciences Vienna (BOKU), Department of Biotechnology, Institute of Microbiology and Microbial Biotechnology , Muthgasse 18, 1190  Vienna , Austria

3. ACIB GmbH , Muthgasse 11, 1190  Vienna , Austria

Abstract

Abstract The promoter of the high-affinity glucose transporter Gth1 (PGTH1) is tightly repressed on glucose and glycerol surplus, and strongly induced in glucose-limitation, thus enabling regulated methanol-free production processes in the yeast production host Komagataella phaffii. To further improve this promoter, an intertwined approach of nucleotide diversification through random and rational engineering was pursued. Random mutagenesis and fluorescence activated cell sorting of PGTH1 yielded five variants with enhanced induction strength. Reverse engineering of individual point mutations found in the improved variants identified two single point mutations with synergistic action. Sequential deletions revealed the key promoter segments for induction and repression properties, respectively. Combination of the single point mutations and the amplification of key promoter segments led to a library of novel promoter variants with up to 3-fold higher activity. Unexpectedly, the effect of gaining or losing a certain transcription factor binding site (TFBS) was highly dependent on its context within the promoter. Finally, the applicability of the novel promoter variants for biotechnological production was proven for the secretion of different recombinant model proteins in fed batch cultivation, where they clearly outperformed their ancestors. In addition to advancing the toolbox for recombinant protein production and metabolic engineering of K. phaffii, we discovered single nucleotide positions and correspondingly affected TFBS that distinguish between glycerol- and glucose-mediated repression of the native promoter.

Funder

Austrian Federal Ministry of Labour and Economy

Christian Doppler Research Association

Austrian Federal Ministry for Climate Action, Environment, Energy, Mobility, Innovation and Technology (BMK);

Styrian Business Promotion Agency

Standortagentur Tirol

Austrian Research Promotion Agency

Publisher

Oxford University Press (OUP)

Subject

Genetics

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