Customizing amino acid metabolism of Pichia pastoris for recombinant protein production

Author:

Rußmayer Hannes12,Buchetics Markus12,Mattanovich Matthias134,Neubauer Stefan25,Steiger Matthias12,Graf Alexandra B.26,Koellensperger Gunda25,Hann Stephan25,Sauer Michael12,Gasser Brigitte12,Mattanovich Diethard12

Affiliation:

1. Department of Biotechnology Institute of Microbiology and Microbial Biotechnology University of Natural Resources and Life Sciences Vienna Austria

2. Austrian Centre of Industrial Biotechnology Vienna Austria

3. Novo Nordisk Foundation Centre for Biosustainability, Technical University of Denmark Lyngby Denmark

4. Novo Nordisk Foundation Centre for Basic Metabolic Research, Copenhagen University Copenhagen Denmark

5. Department of Chemistry Institute of Analytical Chemistry University of Natural Resources and Life Sciences Vienna Austria

6. School of Bioengineering University of Applied Sciences FH Campus Vienna Vienna Austria

Abstract

AbstractAmino acids are the building blocks of proteins. In this respect, a reciprocal effect of recombinant protein production on amino acid biosynthesis as well as the impact of the availability of free amino acids on protein production can be anticipated. In this study, the impact of engineering the amino acid metabolism on the production of recombinant proteins was investigated in the yeast Pichia pastoris (syn Komagataella phaffii). Based on comprehensive systems‐level analyses of the metabolomes and transcriptomes of different P. pastoris strains secreting antibody fragments, cell engineering targets were selected. Our working hypothesis that increasing intracellular amino acid levels could help unburden cellular metabolism and improve recombinant protein production was examined by constitutive overexpression of genes related to amino acid metabolism. In addition to 12 genes involved in specific amino acid biosynthetic pathways, the transcription factor GCN4 responsible for regulation of amino acid biosynthetic genes was overexpressed. The production of the used model protein, a secreted carboxylesterase (CES) from Sphingopyxis macrogoltabida, was increased by overexpression of pathway genes for alanine and for aromatic amino acids, and most pronounced, when overexpressing the regulator GCN4. The analysis of intracellular amino acid levels of selected clones indicated a direct linkage of improved recombinant protein production to the increased availability of intracellular amino acids. Finally, fed batch cultures showed that overexpression of GCN4 increased CES titers 2.6‐fold, while the positive effect of other amino acid synthesis genes could not be transferred from screening to bioreactor cultures.

Funder

Österreichische Forschungsförderungsgesellschaft

Publisher

Wiley

Subject

Molecular Medicine,Applied Microbiology and Biotechnology,General Medicine

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