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高通量定量分析周质腔重组蛋白的方法。

Approaches for high-throughput quantification of periplasmic recombinant proteins.

机构信息

School of Chemical Engineering and Institute of Microbiology and Infection, The University of Birmingham, Edgbaston, Birmingham B15 2TT, UK.

School of Chemical Engineering and Institute of Microbiology and Infection, The University of Birmingham, Edgbaston, Birmingham B15 2TT, UK.

出版信息

N Biotechnol. 2023 Nov 25;77:149-160. doi: 10.1016/j.nbt.2023.09.003. Epub 2023 Sep 12.

Abstract

The Gram-negative periplasm is a convenient location for the accumulation of many recombinant proteins including biopharmaceutical products. It is the site of disulphide bond formation, required by some proteins (such as antibody fragments) for correct folding and function. It also permits simpler protein release and downstream processing than cytoplasmic accumulation. As such, targeting of recombinant proteins to the E. coli periplasm is a key strategy in biologic manufacture. However, expression and translocation of each recombinant protein requires optimisation including selection of the best signal peptide and growth and production conditions. Traditional methods require separation and analysis of protein compositions of periplasmic and cytoplasmic fractions, a time- and labour-intensive method that is difficult to parallelise. Therefore, approaches for high throughput quantification of periplasmic protein accumulation offer advantages in rapid process development.

摘要

革兰氏阴性菌的周质空间是许多重组蛋白(包括生物制药产品)积累的理想位置。它是形成二硫键的部位,某些蛋白质(如抗体片段)需要二硫键才能正确折叠和发挥功能。它还允许比细胞质积累更简单的蛋白质释放和下游加工。因此,将重组蛋白靶向大肠杆菌周质是生物制造的关键策略。然而,每个重组蛋白的表达和易位都需要优化,包括选择最佳的信号肽以及生长和生产条件。传统方法需要分离和分析周质和细胞质部分的蛋白质组成,这是一种费时费力且难以并行化的方法。因此,高通量定量周质蛋白积累的方法在快速工艺开发中具有优势。

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