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重组大豆曲霉碱性蛋白酶在毕赤酵母中的高效表达、纯化及酶学特性分析

High-level expression, purification, and enzymatic characterization of a recombinant Aspergillus sojae alkaline protease in Pichia pastoris.

作者信息

Ke Ye, Yuan XiaoMei, Li JiaSheng, Zhou Wei, Huang XiaoHui, Wang Tao

机构信息

School of Life Sciences, Shaoguan University, Shaoguan, Guangdong, 512005, People's Republic of China.

出版信息

Protein Expr Purif. 2018 Aug;148:24-29. doi: 10.1016/j.pep.2018.03.009. Epub 2018 Mar 26.

DOI:10.1016/j.pep.2018.03.009
PMID:29596989
Abstract

An alkaline protease (Ap) was cloned from Aspergillus sojae GIM3.33 via RT-PCR technique. A truncated Ap without the signal peptide was successfully expressed in the Pichia pastoris KM71 strain. The following describes the optimal process conditions for the recombinant engineering of a strain expressing a recombinant Ap (rAp) in a triangular flask: inoculum concentration OD value 20.0 in 40 mL working volume (in 500 mL flasks), methanol addition (1.0%; volume ratio), 0.02% biotin solution (60 μL), and YNB primary concentration (13.0 g/L). Under these conditions, the protease activity of rAp in the fermentation broth reached 400.4 ± 40.5 U/mL after induction for three days. The rAp was isolated and purified, and its enzymatic characteristics were tested. Its optimal pH was 10.0, and it remained stable in a pH range of 7.0-10.0. Its optimal temperature was 45 °C and it retained >50% activity at 40 °C for 60 min. The rAp activity was significantly inhibited by PMSF, Zn and Fe and the rAp had a broad substrate specificity for natural proteins and synthetic peptide substrates, and preferred substrates at P1 position with large hydrophobic side-chain groups. Compared to Papain (8.7%) and Alcalase (12.2%), the degree of hydrolysis of rAp to soy protein isolate was 16.5%; therefore, rAp was a good candidate for the processing of food industry byproducts.

摘要

通过RT-PCR技术从酱油曲霉GIM3.33中克隆了一种碱性蛋白酶(Ap)。在毕赤酵母KM71菌株中成功表达了一种不含信号肽的截短型Ap。以下描述了在三角瓶中表达重组Ap(rAp)的重组工程菌株的最佳工艺条件:接种物浓度OD值为20.0(工作体积40 mL,置于500 mL烧瓶中),甲醇添加量(1.0%;体积比),0.02%生物素溶液(60 μL),以及YNB初始浓度(13.0 g/L)。在这些条件下,诱导三天后发酵液中rAp的蛋白酶活性达到400.4±40.5 U/mL。对rAp进行了分离纯化,并测试了其酶学特性。其最适pH为10.0,在pH 7.0 - 10.0范围内保持稳定。其最适温度为45℃,在40℃下60分钟内活性保留>50%。PMSF、Zn和Fe对rAp活性有显著抑制作用,rAp对天然蛋白质和合成肽底物具有广泛的底物特异性,且对P1位带有大疏水侧链基团的底物更偏好。与木瓜蛋白酶(8.7%)和碱性蛋白酶(12.2%)相比,rAp对大豆分离蛋白的水解度为16.5%;因此,rAp是食品工业副产品加工的良好候选酶。

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