The Generation of Multicopy Recombinant Strains
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The extremely high levels of alcohol oxidase produced from the native AOX1 gene in Pichia pastoris (5–30% of cell protein on induction) suggested that single-copy AOX1 -promoter expression vectors would be sufficient for efficient foreign gene expression. Therefore, the first strategy adopted for generating recombinant strains was to replace the AOX1 gene with a single copy of the foreign gene expression cassette (transplacement), since this type of transformant is the most stable. Some of the earliest studies supported this strategy, e.g., expression of β-galactosidase or hepatitis B surface antigen was efficient and was not improved by increasing vector copy number (1 ,2 ).