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Superior protein titers in half the fermentation time: Promoter and process engineering for the glucose‐regulated GTH1 promoter of Pichia pastoris

机译:在一半发酵时间内即可获得优异的蛋白滴度:巴斯德毕赤酵母葡萄糖调节的GTH1启动子的启动子和工艺工程

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摘要

Protein production in Pichia pastoris is often based on the methanol‐inducible P AOX1 promoter which drives the expression of the target gene. The use of methanol has major drawbacks, so there is a demand for alternative promoters with good induction properties such as the glucose‐regulated P GTH1 promoter which we reported recently. To further increase its potential, we investigated its regulation in more details by the screening of promoter variants harboring deletions and mutations. Thereby we could identify the main regulatory region and important putative transcription factor binding sites of P GTH1. Concluding from that, yeast metabolic regulators, monomeric Gal4‐class motifs, carbon source‐responsive elements, and yeast GC‐box proteins likely contribute to the regulation of the promoter. We engineered a P GTH1 variant with greatly enhanced induction properties compared with that of the wild‐type promoter. Based on that, a model‐based bioprocess design for high volumetric productivity in a limited time was developed for the P GTH1 variant, to employ a glucose fed‐batch strategy that clearly outperformed a classical methanol fed‐batch of a P AOX1 strain in terms of titer and process performance.
机译:巴斯德毕赤酵母中的蛋白质生产通常基于甲醇诱导的P AOX1启动子,该启动子驱动靶基因的表达。甲醇的使用具有主要缺点,因此需要具有良好诱导特性的替代启动子,例如我们最近报道的葡萄糖调节的PGTH1启动子。为了进一步增加其潜力,我们通过筛选具有缺失和突变的启动子变体来更详细地研究其调控。因此,我们可以确定P GTH1的主要调控区和重要的假定转录因子结合位点。最后,酵母代谢调节剂,单体Gal4类基序,碳源响应元件和酵母GC-box蛋白可能有助于启动子的调控。我们设计了一个P GTH1变异体,与野生型启动子相比,其诱导特性大大增强。在此基础上,针对P GTH1变体开发了基于模型的生物工艺设计,以在有限的时间内实现高产量,采用了葡萄糖补料分批策略,该策略明显优于P AOX1菌株的经典甲醇补料分批。效价和工艺性能。

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