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Test bacterial inclusion body for activity prior to start denaturing and refolding processes to obtain active eukaryotic proteins

机译:在开始变性和重新折叠过程以获得活性真核蛋白之前的活性测试细菌包涵体

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摘要

One of a major drawbacks correlated with expressing antibody fragments in bacterial cells is insolubility, which is often regarded as an obstacle in obtaining active molecules. Recombinant proteins aggregated as inclusion bodies within bacterial cells are thought to be unfolded or misfolded, and therefore inactive. So, denaturing and refolding strategies, which are laborious and sometime inefficient, are used to obtain correctly-folded active proteins. In the current study, we show that large quantities of correctly folded and completely active scFv molecules are there in bacterial inclusion bodies; they only need to be isolated from inclusion bodies.
机译:与表达细菌细胞中表达抗体片段相关的主要缺点之一是不可溶性,其通常被认为是获得活性分子的障碍。 将重组蛋白聚集为细菌细胞内的包合物体被认为是展开或错误的,因此不活跃。 因此,诸多效率且有时低效的变性和重度策略用于获得正确折叠的活性蛋白质。 在目前的研究中,我们表明,在细菌包涵体中有大量的正确折叠和完全活跃的SCFV分子; 他们只需要从包涵体隔离。

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