Abstract
BackgroundThe classic AOX1 replacement approach is still one of the most often used techniques for expression of recombinant proteins in the methylotrophic yeast Pichia pastoris. Although this approach is largely successful, it frequently delivers clones with unpredicted production characteristics and a work-intense screening process is required to find the strain with desired productivity.ResultsIn this project 845 P. pastoris clones, transformed with a GFP expression cassette, were analyzed for their methanol-utilization (Mut)-phenotypes, GFP gene expression levels and gene copy numbers. Several groups of strains with irregular features were identified. Such features include GFP expression that is markedly higher or lower than expected based on gene copy number as well as strains that grew under selective conditions but where the GFP gene cassette and its expression could not be detected. From these classes of strains 31 characteristic clones were selected and their genomes sequenced. By correlating the assembled genome data with the experimental phenotypes novel insights were obtained. These comprise a clear connection between productivity and cassette-to-cassette orientation in the genome, the occurrence of false-positive clones due to a secondary recombination event, and lower total productivity due to the presence of untransformed cells within the isolates were discovered. To cope with some of these problems, the original vector was optimized by replacing the AOX1 terminator, preventing the occurrence of false-positive clones due to the secondary recombination event.ConclusionsStandard methods for transformation of P. pastoris led to a multitude of unintended and sometimes detrimental integration events, lowering total productivity. By documenting the connections between productivity and integration event we obtained a deeper understanding of the genetics of mutation in P. pastoris. These findings and the derived improved mutagenesis and transformation procedures and tools will help other scientists working on recombinant protein production in P. pastoris and similar non-conventional yeasts.Electronic supplementary materialThe online version of this article (doi:10.1186/s12934-016-0486-7) contains supplementary material, which is available to authorized users.
Highlights
The classic AOX1 replacement approach is still one of the most often used techniques for expression of recombinant proteins in the methylotrophic yeast Pichia pastoris
Characterization and grouping of pAHBgl‐GFP P. pastoris clones In total, 845 P. pastoris clones transformed with the GFP expression cassette were characterized for their Mutphenotypes, GFP gene expressions and gene copy numbers (GCN)
The intent of the transformation strategy used in our study was to replace the native AOX1 gene with a single copy of the GFP expression cassette
Summary
The classic AOX1 replacement approach is still one of the most often used techniques for expression of recombinant proteins in the methylotrophic yeast Pichia pastoris. This approach is largely successful, it fre‐ quently delivers clones with unpredicted production characteristics and a work-intense screening process is required to find the strain with desired productivity. The most common approach for heterologous protein expression in P. pastoris is the insertion of the target gene into the genome under the control of the AOX1 (alcohol oxidase 1) promoter (pAOX1). This approach offers tight regulation and a very strong, methanol-inducible expression [6]. Much progress has been made in understanding the regulation of pAOX1 as well as creating novel synthetic variants with improved characteristics, underlining that the importance of the promoter still holds [12,13,14,15,16,17]
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