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首页> 外文期刊>Journal of Immunological Methods >Stable expression and purification of a functional processed Fab' fragment from a single nascent polypeptide in CHO cells expressing the mCAT-1 retroviral receptor.
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Stable expression and purification of a functional processed Fab' fragment from a single nascent polypeptide in CHO cells expressing the mCAT-1 retroviral receptor.

机译:在表达mCAT-1逆转录病毒受体的CHO细胞中从单个新生多肽中稳定表达并纯化功能性加工Fab'片段。

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摘要

Monoclonal antibodies and derivative formats such as Fab' fragments are used in a broad range of therapeutic, diagnostic and research applications. New systems and methodologies that can improve the production of these proteins are consequently of much interest. Here we present a novel approach for the rapid production of processed Fab' fragments in a CHO cell line that has been engineered to express the mouse cationic amino acid transporter receptor 1 (mCAT-1). This facilitated the introduction of the target antibody gene through retroviral transfection, rapidly producing stable expression. Using this system, we designed a single retroviral vector construct for the expression of a target Fab' fragment as a single polypeptide with a furin cleavage site and a FMDV 2A self-cleaving peptide introduced to bridge the light and truncated heavy chain regions. The introduction of these cleavage motifs ensured equimolar expression and processing of the heavy and light domains as exemplified by the production of an active chimeric Fab' fragment against the Fas receptor, routinely expressed in 1-2mg/L yield in spinner-flask cell cultures. These results demonstrate that this method could have application in the facile production of bioactive Fab' fragments.
机译:单克隆抗体及其衍生物形式(例如Fab'片段)被广泛用于治疗,诊断和研究应用。因此,可以改善这些蛋白质产生的新系统和方法学引起了人们的极大兴趣。在这里,我们提出了一种新方法,可在CHO细胞系中快速生产已加工的Fab'片段,该片段已被工程化以表达小鼠阳离子氨基酸转运蛋白受体1(mCAT-1)。这有助于通过逆转录病毒转染引入靶抗体基因,从而快速产生稳定的表达。使用该系统,我们设计了一个单一的逆转录病毒载体构建体,用于将目标Fab'片段表达为具有弗林蛋白酶切割位点和FMDV 2A自切割肽的单个多肽,以桥接轻链和截短的重链区域。这些裂解基序的引入确保了等摩尔表达以及重链和轻链域的加工,例如产生抗Fas受体的活性嵌合Fab'片段,在旋转烧瓶培养中通常以1-2mg / L的产量表达。这些结果表明,该方法可用于简便地生产生物活性Fab'片段。

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