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用于提高毕赤酵母中异源蛋白产量的甘油醛-3-磷酸脱氢酶启动子的转录工程。

Transcriptional engineering of the glyceraldehyde-3-phosphate dehydrogenase promoter for improved heterologous protein production in Pichia pastoris.

作者信息

Ata Özge, Prielhofer Roland, Gasser Brigitte, Mattanovich Diethard, Çalık Pınar

机构信息

Department of Biotechnology, Graduate School of Natural and Applied Sciences, Middle East Technical University, Ankara 06800, Turkey.

Department of Biotechnology, University of Natural Resources and Life Sciences, Vienna, Austria.

出版信息

Biotechnol Bioeng. 2017 Oct;114(10):2319-2327. doi: 10.1002/bit.26363. Epub 2017 Jul 27.

DOI:10.1002/bit.26363
PMID:28650069
Abstract

The constitutive glyceraldehyde-3-phosphate dehydrogenase promoter (P ), which is one of the benchmark promoters of Pichia pastoris, was analyzed in terms of putative transcription factor binding sites. We constructed a synthetic library with distinct regulatory properties through deletion and duplication of these putative transcription factor binding sites and selected transcription factor (TF) genes were overexpressed or deleted to understand their roles on heterologous protein production. Using enhanced green fluorescent protein, an expression strength in a range between 0.35- and 3.10-fold of the wild-type P was obtained. Another model protein, recombinant human growth hormone was produced under control of selected promoter variants and 1.6- to 2.4-fold higher product titers were reached compared to wild-type P . In addition, a GAL4-like TF was found to be a crucial factor for the regulation of P , and its overexpression enhanced the heterologous protein production considerably (up to 2.2-fold compared to the parental strain). The synthetic P library generated enabled us to investigate the different putative transcription factors which are responsible for the regulation of P under different growth conditions, ergo recombinant protein production under P . Biotechnol. Bioeng. 2017;114: 2319-2327. © 2017 Wiley Periodicals, Inc.

摘要

组成型磷酸甘油醛脱氢酶启动子(P)是巴斯德毕赤酵母的基准启动子之一,对其假定的转录因子结合位点进行了分析。我们通过删除和复制这些假定的转录因子结合位点构建了一个具有不同调控特性的合成文库,并对选定的转录因子(TF)基因进行过表达或缺失操作,以了解它们在异源蛋白生产中的作用。使用增强型绿色荧光蛋白,获得了野生型P强度0.35至3.10倍范围内的表达强度。在选定的启动子变体控制下生产另一种模型蛋白重组人生长激素,与野生型P相比,产品滴度提高了1.6至2.4倍。此外,发现一种类似GAL4的TF是P调控的关键因素,其过表达显著提高了异源蛋白产量(与亲本菌株相比提高了2.2倍)。生成的合成P文库使我们能够研究在不同生长条件下负责P调控的不同假定转录因子,从而研究在P控制下的重组蛋白生产。《生物技术与生物工程》2017年;114: 2319 - 2327。© 2017威利期刊公司

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