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在毕赤酵母高密度生物反应器研究中,氮源补充可以改善产物质量和数量:以易蛋白水解的链激酶为例。

Nitrogen supplementation ameliorates product quality and quantity during high cell density bioreactor studies of Pichia pastoris: A case study with proteolysis prone streptokinase.

机构信息

Department of Microbiology, University of Delhi South Campus, New Delhi 110021, India.

Department of Microbiology, University of Delhi South Campus, New Delhi 110021, India.

出版信息

Int J Biol Macromol. 2021 Jun 1;180:760-770. doi: 10.1016/j.ijbiomac.2021.03.021. Epub 2021 Mar 11.

DOI:10.1016/j.ijbiomac.2021.03.021
PMID:33716129
Abstract

Streptokinase is a well-established cost-effective therapeutic molecule for thrombo-embolic complications. In the current study, a tag-free variant of streptokinase with a native N-terminus (N-rSK) was developed using the Pichia expression system. A three-copy clone was screened that secreted 1062 mg/L of N-rSK in the complex medium at shake flask level. The biologically active (67,552.61 IU/mg) N-rSK recovered by anion exchange chromatography was predicted to contain 15.43% α-helices, 26.43% β-sheets. The fermentation run in a complex medium yielded a poor quality product due to excessive N-rSK degradation. Therefore, modified basal salt medium was also employed during fermentation operations to reduce the proteolytic processing of the recombinant product. The concomitant feeding of 1 g/L/h soya flour hydrolysate with methanol during the protein synthesis phase reduced the proteolysis and yielded 2.29 g/L of N-rSK. The fermentation medium was also supplemented with urea during growth and induction phases. The combined feeding approach of nitrogen-rich soya flour hydrolysate and urea during bioreactor operations showed significant improvement in protein stability and resulted in a 4-fold increase in N-rSK concentration to a level of 4.03 g/L over shake flask. Under optimized conditions, the volumetric productivity and specific product yield were 52.33 mg/L/h and 33.24 mg/g DCW, respectively.

摘要

链激酶是一种成熟的、具有成本效益的治疗血栓栓塞并发症的治疗分子。在本研究中,使用毕赤酵母表达系统开发了一种带有天然 N 端(N-rSK)的无标签链激酶变体。筛选出一个三拷贝克隆,在摇瓶水平的复杂培养基中分泌 1062mg/L 的 N-rSK。通过阴离子交换色谱回收的具有生物活性(67552.61IU/mg)的 N-rSK 预计含有 15.43%的α-螺旋和 26.43%的β-折叠。由于过量的 N-rSK 降解,复杂培养基中的发酵生产出的产品质量较差。因此,在发酵过程中还使用了改良的基础盐培养基,以减少重组产物的蛋白水解加工。在蛋白质合成阶段,同时以 1g/L/h 的速度补料添加豆粕水解物和甲醇,可以减少蛋白水解,并产生 2.29g/L 的 N-rSK。在生长和诱导阶段,发酵培养基中还添加了尿素。在生物反应器操作中,富氮豆粕水解物和尿素的联合补料方法显著提高了蛋白质稳定性,使 N-rSK 浓度提高了 4 倍,达到 4.03g/L,超过摇瓶水平。在优化条件下,比生产率和比产物得率分别为 52.33mg/L/h 和 33.24mg/gDCW。

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