Engineering protein translocation pathway to improve recombinant proteins in Pichia pastoris

IF 3.6 Q2 BIOTECHNOLOGY & APPLIED MICROBIOLOGY Current Research in Biotechnology Pub Date : 2024-01-01 DOI:10.1016/j.crbiot.2024.100182
Shengyan Wang , Huijia Dai , Qingling Tang , Yujing Yu , Yaying Xie , Tao Wang , Yide Huang
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Abstract

Pichia pastoris is one of the most commonly used hosts for producing heterologous proteins, whereas production levels vary depending on the protein of interest and are also regulated by regulatory factors. We conducted RNA-seq by expressing the reporter EGFP and observed significant upregulation of certain subunits (Sec61p, Sbh1p, Sss1p, Sec66p and Sec72p) of the Sec complex in the high-expression recombinant GS115 stains. The overexpression of these genes may increase the expression levels of heterogeneous proteins. In this study, the endogenous promoters of the Sec complex subunits Sbh1p, Sss1p, Sec66p and Sec72p were isolated and verified their activity using the Lac-Z reporter gene. Sss1, Sbh1, Sec66 and Sec72 were overexpressed under the control of their own promoters in Pichia pastoris, respectively. The overexpression of Sss1, Sbh1, Sec66 and Sec72 in cells was confirmed by fluorescent microscope and Western blot analysis. The α-amylase was employed to evaluate the effect of overexpression of the Sec subunits on the heterologous protein expression. The results demonstrated that the α-amylase activity increased by 16%, 58%, 16% and 17% in the strains overexpressing Sss1, Sbh1, Sec66 and Sec72, respectively. Engineering the protein translocation pathway can be an alternative to enhance heterogeneous proteins in Pichia pastoris expression system.

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改造蛋白质转运途径,改进 Pichia pastoris 的重组蛋白质
Pichia pastoris 是生产异源蛋白最常用的宿主之一,但其生产水平因相关蛋白的不同而异,而且还受调控因子的调控。我们通过表达报告基因 EGFP 进行了 RNA-seq,在高表达重组 GS115 染色体中观察到 Sec 复合物的某些亚基(Sec61p、Sbh1p、Sss1p、Sec66p 和 Sec72p)显著上调。这些基因的过度表达可能会增加异质蛋白的表达水平。本研究分离了 Sec 复合物亚基 Sbh1p、Sss1p、Sec66p 和 Sec72p 的内源启动子,并使用 Lac-Z 报告基因验证了它们的活性。Sss1、Sbh1、Sec66 和 Sec72 分别在各自启动子的控制下在 Pichia pastoris 中过表达。荧光显微镜和 Western 印迹分析证实了 Sss1、Sbh1、Sec66 和 Sec72 在细胞中的过表达。利用α-淀粉酶来评估过表达Sec亚基对异源蛋白表达的影响。结果表明,在过表达Sss1、Sbh1、Sec66和Sec72的菌株中,α-淀粉酶活性分别提高了16%、58%、16%和17%。在Pichia pastoris表达系统中,蛋白质转运途径工程化是提高异质蛋白的一种替代方法。
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来源期刊
Current Research in Biotechnology
Current Research in Biotechnology Biochemistry, Genetics and Molecular Biology-Biotechnology
CiteScore
6.70
自引率
3.60%
发文量
50
审稿时长
38 days
期刊介绍: Current Research in Biotechnology (CRBIOT) is a new primary research, gold open access journal from Elsevier. CRBIOT publishes original papers, reviews, and short communications (including viewpoints and perspectives) resulting from research in biotechnology and biotech-associated disciplines. Current Research in Biotechnology is a peer-reviewed gold open access (OA) journal and upon acceptance all articles are permanently and freely available. It is a companion to the highly regarded review journal Current Opinion in Biotechnology (2018 CiteScore 8.450) and is part of the Current Opinion and Research (CO+RE) suite of journals. All CO+RE journals leverage the Current Opinion legacy-of editorial excellence, high-impact, and global reach-to ensure they are a widely read resource that is integral to scientists' workflow.
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