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cDNA display: a novel screening method for functional disulfide-rich peptides by solid-phase synthesis and stabilization of mRNA–protein fusions

机译:cDNA显示:通过固相合成和稳定mRNA-蛋白质融合物的方法,对富含二硫键的功能性多肽进行新型筛选

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We report a robust display technology for the screening of disulfide-rich peptides, based on cDNA–protein fusions, by developing a novel and versatile puromycin-linker DNA. This linker comprises four major portions: a ‘ligation site' for T4 RNA ligase, a ‘biotin site' for solid-phase handling, a ‘reverse transcription primer site' for the efficient and rapid conversion from an unstable mRNA–protein fusion (mRNA display) to a stable mRNA/cDNA–protein fusion (cDNA display) whose cDNA is covalently linked to its encoded protein and a ‘restriction enzyme site' for the release of a complex from the solid support. This enables not only stabilizing mRNA–protein fusions but also promoting both protein folding and disulfide shuffling reactions. We evaluated the performance of cDNA display in different model systems and demonstrated an enrichment efficiency of 20-fold per selection round. Selection of a 32-residue random library against interleukin-6 receptor generated novel peptides containing multiple disulfide bonds with a unique linkage for its function. The peptides were found to bind with the target in the low nanomolar range. These results show the suitability of our method for in vitro selections of disulfide-rich proteins and other potential applications.
机译:我们报道了一种强大的显示技术,可通过开发新颖而通用的嘌呤霉素-连接子DNA来筛选基于cDNA-蛋白质融合体的富含二硫键的肽。该接头包括四个主要部分:一个用于T4 RNA连接酶的“连接位点”,一个用于固相处理的“生物素位点”,一个用于从不稳定的mRNA与蛋白融合物(mRNA)快速有效转化的“逆转录引物位点”展示)与稳定的mRNA / cDNA-蛋白融合体(cDNA展示),其cDNA共价连接至其编码的蛋白和“限制酶位点”,以从固相支持物中释放复合物。这不仅可以稳定mRNA与蛋白质的融合,还可以促进蛋白质折叠和二硫键改组反应。我们评估了在不同模型系统中cDNA展示的性能,并证明了每个选择回合的20倍富集效率。针对白介素6受体的32个残基的随机文库的选择生成了包含多个具有其功能独特键的二硫键的新型肽。发现这些肽在低纳摩尔范围内与靶标结合。这些结果表明我们的方法适用于体外选择富含二硫键的蛋白质和其他潜在应用。

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