An easy-to-use high-throughput selection system for the discovery of recombinant protein binders from alternative scaffold libraries.

IF 2.6 4区 生物学 Q3 BIOCHEMISTRY & MOLECULAR BIOLOGY
Marit Möller, Malin Jönsson, Magnus Lundqvist, Blenda Hedin, Louise Larsson, Emma Larsson, Johan Rockberg, Mathias Uhlén, Sarah Lindbo, Hanna Tegel, Sophia Hober
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Abstract

Selection by phage display is a popular and widely used technique for the discovery of recombinant protein binders from large protein libraries for therapeutic use. The protein library is displayed on the surface of bacteriophages which are amplified using bacteria, preferably Escherichia coli, to enrich binders in several selection rounds. Traditionally, the so-called panning procedure during which the phages are incubated with the target protein, washed and eluted is done manually, limiting the throughput. High-throughput systems with automated panning already in use often require high-priced equipment. Moreover, the bottleneck of the selection process is usually the screening and characterization. Therefore, having a high-throughput panning procedure without a scaled screening platform does not necessarily increase the discovery rate. Here, we present an easy-to-use high-throughput selection system with automated panning using cost-efficient equipment integrated into a workflow with high-throughput sequencing and a tailored screening step using biolayer-interferometry. The workflow has been developed for selections using two recombinant libraries, ADAPT (Albumin-binding domain-derived affinity proteins) and CaRA (Calcium-regulated affinity) and has been evaluated for three new targets. The newly established semi-automated system drastically reduced the hands-on time and increased robustness while the selection outcome, when compared to manual handling, was very similar in deep sequencing analysis and generated binders in the nanomolar affinity range. The developed selection system has shown to be highly versatile and has the potential to be applied to other binding domains for the discovery of new protein binders.

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一种易于使用的高通量选择系统,用于从替代支架库中发现重组蛋白结合物。
噬菌体展示筛选是一种流行且广泛使用的技术,用于从大型蛋白质库中发现用于治疗用途的重组蛋白质结合物。蛋白质库显示在噬菌体的表面,噬菌体使用细菌(优选大肠杆菌)扩增,以在几轮选择中富集结合剂。传统上,将噬菌体与靶蛋白孵育、洗涤和洗脱的所谓摇摄程序是手动进行的,这限制了产量。已经在使用的具有自动平移的高通量系统通常需要高价设备。此外,筛选过程的瓶颈通常是筛选和表征。因此,在没有按比例筛选平台的情况下进行高通量摇摄程序并不一定会增加发现率。在这里,我们介绍了一个易于使用的高通量选择系统,该系统使用成本效益高的设备进行自动平移,集成到高通量测序的工作流程中,并使用生物层干涉测量法进行定制的筛选步骤。该工作流程已开发用于使用两个重组文库ADAPT(白蛋白结合结构域衍生的亲和蛋白)和CaRA(钙调节的亲和力)进行选择,并已对三个新靶点进行了评估。新建立的半自动化系统大大减少了动手时间,提高了稳健性,而与手动操作相比,选择结果在深度测序分析中非常相似,并产生了纳摩尔亲和力范围内的结合剂。所开发的选择系统已显示出高度通用性,并有潜力应用于其他结合结构域,以发现新的蛋白质结合剂。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Protein Engineering Design & Selection
Protein Engineering Design & Selection 生物-生化与分子生物学
CiteScore
3.30
自引率
4.20%
发文量
14
审稿时长
6-12 weeks
期刊介绍: Protein Engineering, Design and Selection (PEDS) publishes high-quality research papers and review articles relevant to the engineering, design and selection of proteins for use in biotechnology and therapy, and for understanding the fundamental link between protein sequence, structure, dynamics, function, and evolution.
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