首页> 外文期刊>Journal of Molecular Biology >Directed Evolution of an Anti-prion Protein scFv Fragment to an Affinity of 1 pM and its Structural Interpretation.
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Directed Evolution of an Anti-prion Protein scFv Fragment to an Affinity of 1 pM and its Structural Interpretation.

机译:指导抗-病毒蛋白scFv片段进化到1 pM的亲和力及其结构解释。

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摘要

Bovine spongiform encephalopathy (BSE) is a fatal neurodegenerative prion disease affecting cattle that is transmissible to humans, manifesting as a variant of Creutzfeldt-Jakob disease (vCJD) likely following the consumption of meat contaminated with BSE prions. High-affinity antibodies are a prerequisite for the development of simple, highly sensitive and non-invasive diagnostic tests that are able to detect even small amounts of the disease-associated PrP conformer (PrP(Sc)). We describe here the affinity maturation of a single-chain Fv antibody fragment with a binding affinity of 1 pM to a peptide derived from the unstructured region of bovine PrP (BoPrP (90-105)). This is the tightest peptide-binding antibody reported to date and may find useful application in diagnostics, especially when PrP(Sc) is pretreated by denaturation and/or proteolysis for peptide-like presentation. Several rounds of directed evolution and off-rate selection with ribosome display were performed using an antibody library generated from a single PrP binder with error-prone PCR and DNA-shuffling. As the correct determinations of affinities in this range are not straightforward, competition biosensor techniques and KinExA methods were both applied and compared. Structural interpretation of the affinity improvement was performed based on the crystal structure of the original prion binder in complex with the BoPrP (95-104) peptide by modeling the corresponding mutations.
机译:牛海绵状脑病(BSE)是一种致命的神经变性病毒病,影响到牛,可传播给人类,表现为克雅氏病(vCJD)的变体,可能是食用被BSE pr病毒污染的肉类所致。高亲和力抗体是开发简单,高度灵敏和非侵入性诊断测试的前提,该测试能够检测甚至少量的疾病相关PrP构象体(PrP(Sc))。我们在这里描述单链Fv抗体片段的亲和力成熟,其结合亲和力为1 pM,该肽与衍生自牛PrP(BoPrP(90-105))非结构化区域的肽结合。这是迄今为止报道的最紧密的肽结合抗体,可能在诊断中找到有用的应用,尤其是当PrP(Sc)通过变性和/或蛋白水解预处理以呈肽样呈递时。使用由单个PrP结合物生成的抗体文库,通过易错PCR和DNA改组,进行了几轮定向进化和核糖体展示的脱速率选择。由于亲和力在此范围内的正确测定并不简单,因此应用了竞争生物传感器技术和KinExA方法并进行了比较。通过模拟相应的突变,基于与BoPrP(95-104)肽复合的原始病毒结合剂的晶体结构,进行亲和力改善的结构解释。

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