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用于高效分泌和纯化来自莱茵衣藻的人类生长因子的工程融合蛋白

Engineered Fusion Proteins for Efficient Protein Secretion and Purification of a Human Growth Factor from the Green Microalga Chlamydomonas reinhardtii.

作者信息

Baier Thomas, Kros Dana, Feiner Rebecca C, Lauersen Kyle J, Müller Kristian M, Kruse Olaf

机构信息

Bielefeld University, Faculty of Biology , Center for Biotechnology (CeBiTec) , Universitätsstrasse 27 , 33615 Bielefeld , Germany.

Bielefeld University, Faculty of Technology , Cellular and Molecular Biotechnology , Universitätsstrasse 25 , 33615 Bielefeld , Germany.

出版信息

ACS Synth Biol. 2018 Nov 16;7(11):2547-2557. doi: 10.1021/acssynbio.8b00226. Epub 2018 Oct 22.

DOI:10.1021/acssynbio.8b00226
PMID:30296377
Abstract

Light-driven recombinant protein (RP) production in eukaryotic microalgae offers a sustainable alternative to other established cell-culture systems. RP production via secretion into the culture medium enables simple product separation from the cells adding a layer of process value in addition to the algal biomass, which can be separately harvested. For the model microalga Chlamydomonas reinhardtii, a broad range of molecular tools have been established to enable heterologous gene expression; however, low RP production levels and unreliable purification from secretion concepts have been reported. Domesticated C. reinhardtii strains used for genetic engineering are often cell-wall deficient. These strains nevertheless secrete cell-wall components such as insoluble (hydroxy)proline-rich glycoproteins into the culture media, which hinder downstream purification processes. Here, we attempted to overcome limitations in secretion titers and improve protein purification by combining fusion partners that enhance RP secretion and enable alternative aqueous two-phase (ATPS) RP extraction from the culture medium. Protein fusions were strategically designed to contain a stably folded peptide, which enhanced secretion capacities and gave insights into (some) regulatory mechanisms responsible for this process in the algal host. The elevated protein titers mediated by this fusion were then successfully applied in combination with a fungal hydrophobin tag, which enabled protein purification from the complex microalgal extracellular environment by ATPS, to yield functional recombinant human epidermal growth factor (hEGF) from the algal host.

摘要

在真核微藻中利用光驱动生产重组蛋白(RP)为其他成熟的细胞培养系统提供了一种可持续的替代方案。通过分泌到培养基中来生产RP,除了可以单独收获的藻类生物质外,还能使产品从细胞中简单分离,从而增加了一层工艺价值。对于模式微藻莱茵衣藻,已经建立了广泛的分子工具来实现异源基因表达;然而,已有报道称其RP生产水平较低,且从分泌概念中进行纯化的可靠性较差。用于基因工程的驯化莱茵衣藻菌株通常缺乏细胞壁。这些菌株仍然会将细胞壁成分,如不溶性的富含(羟基)脯氨酸的糖蛋白分泌到培养基中,这会阻碍下游的纯化过程。在这里,我们试图通过结合能够增强RP分泌并实现从培养基中进行替代水相两相(ATPS)RP提取的融合伙伴,来克服分泌滴度的限制并改善蛋白质纯化。蛋白质融合体经过精心设计,包含一个稳定折叠的肽段,该肽段增强了分泌能力,并深入了解了藻类宿主中负责此过程的(一些)调控机制。然后,由这种融合介导的提高的蛋白质滴度与真菌疏水蛋白标签成功结合应用,该标签能够通过ATPS从复杂的微藻细胞外环境中纯化蛋白质,从而从藻类宿主中产生功能性重组人表皮生长因子(hEGF)。

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