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利用去阻遏技术实现毕赤酵母的甲醇独立表达

Methanol Independent Expression by Pichia Pastoris Employing De-repression Technologies.

作者信息

Fischer Jasmin Elgin, Hatzl Anna-Maria, Weninger Astrid, Schmid Christian, Glieder Anton

机构信息

bisy e.U.

Institute of Molecular Biotechnology, Technical University of Graz.

出版信息

J Vis Exp. 2019 Jan 23(143). doi: 10.3791/58589.

DOI:10.3791/58589
PMID:30735181
Abstract

Methanol is a well-established carbon source and inducer for efficient protein production employing Pichia pastoris (P. pastoris) as a host on micro-, lab and industrial scale. However, due to its toxicity and flammability, there is a desire to avoid methanol while maintaining the high productivity of P. pastoris. Small scale bioreactor cultivations (0.5-5 L working volume) are commonly used to evaluate a strain and its protein production characteristics since microscale cultivation in deep well plates can be hardly controlled or relies on expensive equipment. Furthermore, traditional protocols for the cultivation and induction of P. pastoris were established for constitutive expression or methanol induction and so far, no reliable protocols were described to screen P. pastoris expression strains with derepressible promoters in (controlled and monitored) parallel cultivations. To simplify such initial cultivations to characterize and compare new protein production strains, we established a simple shake flask cultivation system for methanol free expression that simulates bioreactor conditions including a constant slow glycerol feed and online monitoring, thereby coming closer to the real conditions in bioreactors compared to mostly applied small scale batch cultivations. To drive recombinant protein expression in P. pastoris, the carbon source repressed promoters PDC and PDF were applied. Polymer discs with embedded carbon source, releasing a constant amount of glycerol, assured a feed rate delivering the necessary energy for maintaining the promoters active while keeping the biomass generation low.

摘要

甲醇是一种成熟的碳源和诱导剂,可用于在微型、实验室和工业规模上以巴斯德毕赤酵母(P. pastoris)作为宿主高效生产蛋白质。然而,由于其毒性和易燃性,人们希望在保持巴斯德毕赤酵母高生产力的同时避免使用甲醇。小规模生物反应器培养(工作体积为0.5 - 5升)通常用于评估菌株及其蛋白质生产特性,因为在深孔板中的微型培养很难控制或依赖昂贵的设备。此外,巴斯德毕赤酵母培养和诱导的传统方案是为组成型表达或甲醇诱导而建立的,到目前为止,尚未有可靠的方案描述在(受控和监测的)平行培养中筛选具有可去阻遏启动子的巴斯德毕赤酵母表达菌株。为了简化此类用于表征和比较新蛋白质生产菌株的初始培养,我们建立了一种用于无甲醇表达的简单摇瓶培养系统,该系统模拟生物反应器条件,包括恒定缓慢的甘油进料和在线监测,因此与大多数应用的小规模分批培养相比,更接近生物反应器中的实际条件。为了驱动巴斯德毕赤酵母中的重组蛋白表达,应用了碳源阻遏启动子PDC和PDF。带有嵌入式碳源的聚合物圆盘可释放恒定数量的甘油,确保进料速率能提供维持启动子活性所需的能量,同时保持低生物量生成。

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