Induction without methanol: novel regulated promoters enable high-level expression in Pichia pastoris

毕赤酵母 发起人 生物 异源的 基因表达 基因 异源表达 分子生物学 表达式向量 报告基因 基因表达调控 重组DNA 生物化学
作者
Roland Prielhofer,Michael Maurer,Joachim Klein,Jana Wenger,Christoph Kiziak,Brigitte Gasser,Diethard Mattanovich
出处
期刊:Microbial Cell Factories [BioMed Central]
卷期号:12 (1) 被引量:127
标识
DOI:10.1186/1475-2859-12-5
摘要

Abstract Background Inducible high-level expression is favoured for recombinant protein production in Pichia pastoris . Therefore, novel regulated promoters are desired, ideally repressing heterologous gene expression during initial growth and enabling it in the production phase. In a typical large scale fed-batch culture repression is desired during the batch phase where cells grow on a surplus of e.g. glycerol, while heterologous gene expression should be active in the feed phase under carbon (e.g. glucose) limitation. Results DNA microarray analysis of P. pastoris wild type cells growing in glycerol-based batch and glucose-based fed batch was used for the identification of genes with both, strong repression on glycerol and high-level expression in the feed phase. Six novel glucose-limit inducible promoters were successfully applied to express the intracellular reporter eGFP. The highest expression levels together with strong repression in pre-culture were achieved with the novel promoters P G1 and P G6 . Human serum albumin (HSA) was used to characterize the promoters with an industrially relevant secreted protein. A P G1 clone with two gene copies reached about 230% of the biomass specific HSA titer in glucose-based fed batch fermentation compared to a P GAP clone with identical gene copy number, while P G6 only achieved 39%. Two clones each carrying eleven gene copies, expressing HSA under control of P G1 and P G6 respectively were generated by post-transformational vector amplification. They produced about 1.0 and 0.7 g L -1 HSA respectively in equal fed batch processes. The suitability in production processes was also verified with HyHEL antibody Fab fragment for P G1 and with porcine carboxypeptidase B for P G6 . Moreover, the molecular function of the gene under the control of P G1 was determined to encode a high-affinity glucose transporter and named GTH1 . Conclusions A set of novel regulated promoters, enabling induction without methanol, was successfully identified by using DNA microarrays and shown to be suitable for high level expression of recombinant proteins in glucose-based protein production processes.

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