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Enhancement of Alpha 1-antitrypsin Production in Pichia pastoris by Designing and Optimizing Medium Using Elemental Analysis

机译:通过元素分析设计和优化培养基提高巴斯德毕赤酵母中α1-抗胰蛋白酶的产量

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摘要

>Background: Human alpha 1-antitrypsin (AAT) is a monomeric glycosylated protein; it is the potent inhibitor of a whole range of serine proteases and protects tissues against their destructive effects. The human plasma-derived AAT, which is currently used to augment the AAT level in patients, is limited due to high cost and source limitation. Recombinant production of AAT can be considered as a potential alternative. >Objectives: This study aims to develop and optimize a new chemically defi ned medium based on an elemental analysis of the yeast Pichia pastoris for an effi cient culture of the recombinant yeast-producing secretory AAT. >Materials and Methods: An elemental analysis of Carbon (C), Hydrogen (H), Nitrogen (N), Sulfur (S); CHNS in its abbreviated form, and metallic elements was performed to determine the exact molecular constituent of the P. pastoris. The medium components were selected according to the obtained formula; they were optimized by the response surface methodology (RSM). The grown yeast cell was measured at the end of 18 h glycerol batch culture. The amounts of AAT production and elastase inhibitory capacity (EIC) were measured at the end of three days’ methanol feeding. >Results: The optimized medium compositions consist of glycerol (40 g.L-1), KH2PO4 (24.78 g.L-1), NaCl, (0.88 g.L-1),MgSO4.7H2O (1.95 g.L-1), (NH4)2SO4(22.76 g.L-1), and trace elements (20 mL.L-1). The presented quadratic models showthat KH2PO4and (NH4)2SO4, are the most abundant ones in the P. pastoris biomass and have the greatest effect on the cellgrowth, EIC, and AAT protein production responses.>Conclusions: According to the results of this study, it can be concluded that the characterizing cell composition formulacould be considered as an appropriate method to design culture media in order to improve cell growth and productivity.Compared to the common P. pastoris chemically defi ned media, FM22 and BSM, production of AAT protein increased by1.5 and 1.4 times, respectively, in this new medium.
机译:>背景:人α1-抗胰蛋白酶(AAT)是一种单体糖基化蛋白;它是各种丝氨酸蛋白酶的有效抑制剂,可保护组织免遭破坏。由于高成本和来源的限制,目前用于提高患者AAT水平的人血浆来源的AAT受到限制。重组生产AAT可以被视为潜在的替代方法。 >目标:本研究旨在基于酵母毕赤酵母的元素分析,开发和优化一种新的化学定义培养基,以有效培养重组产生酵母的分泌型AAT。 >材料和方法:碳(C),氢(H),氮(N),硫(S)的元素分析; CHNS的缩写形式和金属元素用于确定巴斯德毕赤酵母的确切分子组成。根据获得的公式选择培养基成分;通过响应面方法(RSM)对它们进行了优化。在18 h甘油分批培养结束时测量生长的酵母细胞。在喂食甲醇三天后测量了AAT的产生量和弹性蛋白酶抑制能力(EIC)。 >结果:优化的培养基组成包括:甘油(40 gL -1 ),KH2PO4(24.78 gL -1 ),氯化钠(0.88 gL -1 ),硫酸镁.7小时O(1.95 g.L -1 ),(NH4)2SO4(22.76 g.L -1 )和微量元素(20 mL.L -1 )。呈现的二次模型显示那KH2PO4和(NH4)2SO4是巴斯德毕赤酵母生物量中含量最高的物质,对细胞的影响最大生长,EIC和AAT蛋白质生产反应。>结论:根据这项研究的结果,可以得出结论,表征细胞组成的公式可以被认为是设计培养基以改善细胞生长和生产力的合适方法。与常见的巴斯德毕赤酵母化学定义培养基FM22和BSM相比,AAT蛋白的产量增加了在这种新媒体中,播放次数分别为1.5和1.4倍。

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