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Improved Production of Active Streptomyces griseus Trypsin with a Novel Auto-Catalyzed Strategy

机译:用新型的自动催化策略改善活性链霉菌胰蛋白酶的生产

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N-terminal sequences play crucial roles in regulating expression, translation, activation and enzymatic properties of proteins. To reduce cell toxicity of intracellular trypsin and increase secretory expression, we developed a novel auto-catalyzed strategy to produce recombinant trypsin by engineering the N-terminus of mature Streptomyces griseus trypsin (SGT). The engineered N-terminal peptide of SGT was composed of the thioredoxin, glycine-serine linker, His6-tag and the partial bovine trypsinogen pro-peptide (DDDDK). Furthermore, we constructed a variant TLEI with insertion of the artificial peptide at N-terminus and site-directed mutagenesis of the autolysis residue R145. In fed-batch fermentation, the production of extracellular trypsin activity was significantly improved to 47.4?±?1.2?U·ml(-1) (amidase activity, 8532?±?142.2?U·ml(-1) BAEE activity) with a productivity of 0.49?U·ml(-1)·h(-1), which was 329% greater than that of parent strain Pichia pastoris GS115-SGT. This work has significant potential to be scaled-up for microbial production of SGT. In addition, the N-terminal peptide engineering strategy can be extended to improve heterologous expression of other toxic enzymes.
机译:N-末端序列在调节蛋白质的表达,翻译,激活和酶学性质中起重要作用。为了降低细胞内胰蛋白酶的细胞毒性并增加分泌物表达,我们开发了一种新的自动催化策略,通过工程制备重组胰蛋白酶,其成熟的胰蛋白酶Griseus胰蛋白酶(SGT)的N-末端。 SGT的工程化N-末端肽由硫辛蛋白,甘氨酸 - 丝氨酸接头,His6标签和部分牛胰蛋白酶原培养物(DDDDK)组成。此外,我们构建了一种变型TLEI,其在N-末端插入人工肽和自分解残余物R145的定点诱变。在喂养批量发酵中,细胞外胰蛋白酶活性的产生显着改善至47.4?±1.2?ml(-1)(酰胺酶活性,8532〜αα142.2≤ml(-1)Baee活动)生产率为0.49?u·ml(-1)·h(-1),其比亲本菌株Pichia Pastoris GS115-SGT大329%。这项工作具有显着的潜力,可扩大用于SGT的微生物生产。此外,可以扩展N-末端肽工程策略以改善其他有毒酶的异源表达。

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