首页> 外文期刊>Journal of Immunological Methods >Phage display of a cellulose binding domain from Clostridium thermocellum and its application as a tool for antibody engineering.
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Phage display of a cellulose binding domain from Clostridium thermocellum and its application as a tool for antibody engineering.

机译:来自热纤梭菌的纤维素结合域的噬菌体展示及其作为抗体工程设计的工具的应用。

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Phage display of antibody fragments has proved to be a powerful tool for the isolation and in vitro evolution of these biologically important molecules. However, the general usefulness of this technology is still limited by some technical difficulties. One of the most debilitating obstacles to the widespread application of the technology is the accumulation of "insert loss" clones in the libraries; phagemid clones from which the DNA encoding part or all of the cloned antibody fragment had been deleted. Another difficulty arises when phage technology is applied for cloning hybridoma-derived antibody genes, where myeloma derived light chains, irrelevant to the hybridoma's antibody specificity may be fortuitously cloned. Here, we report the construction of a novel phage-display system designed to address these problems. In our system a single-chain Fv (scFv) is expressed as an in-frame fusion protein with a cellulose-binding domain (CBD) derived from the Clostridium thermocellum cellulosome. The CBD domain serves as an affinity tag allowing rapid phage capture and concentration from crude culture supernatants, and immunological detection of both displaying phage and soluble scFv produced thereof. We demonstrate the utility of our system in solving the technical difficulties described above, and in speeding up the process of scFv isolation from combinatorial antibody repertoires.
机译:抗体片段的噬菌体展示已被证明是这些生物学上重要分子的分离和体外进化的有力工具。但是,该技术的一般用途仍然受到某些技术困难的限制。该技术广泛应用的最大障碍之一是库中“插入丢失”克隆的积累。噬菌粒克隆,其中已删除了编码部分或全部克隆抗体片段的DNA。当将噬菌体技术应用于克隆杂交瘤来源的抗体基因时,另一个困难出现了,其中可能会克隆与杂交瘤的抗体特异性无关的骨髓瘤来源的轻链。在这里,我们报告旨在解决这些问题的新型噬菌体展示系统的建设。在我们的系统中,单链Fv(scFv)表示为符合框架的融合蛋白,并带有衍生自热纤梭菌纤维素体的纤维素结合域(CBD)。 CBD结构域用作亲和标签,允许从粗培养上清中快速捕获噬菌体并对其进行浓缩,并对展示的噬菌体及其产生的可溶性scFv进行免疫检测。我们展示了我们的系统在解决上述技术难题以及加快从组合抗体库中分离scFv的过程中的实用性。

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