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纳米抗体缀合物和蛋白融合物作为生物分析试剂的评价。

Evaluation of Nanobody Conjugates and Protein Fusions as Bioanalytical Reagents.

机构信息

Department of Chemistry and ‡Department of Biochemistry & Molecular Biology, Colorado State University , Fort Collins, Colorado 80523, United States.

出版信息

Anal Chem. 2017 Apr 4;89(7):3819-3823. doi: 10.1021/acs.analchem.7b00470. Epub 2017 Mar 20.

Abstract

Enzyme-linked immunosorbent assay (ELISA), flow cytometry, and Western blot are common bioanalytical techniques. Successful execution traditionally requires the use of one or more commercially available antibody-small-molecule dyes or antibody-reporter protein conjugates that recognize relatively short peptide tags (<15 amino acids). However, the size of antibodies and their molecular complexity (by virtue of post-translational disulfide formation and glycosylation) typically require either expression in mammalian cells or purification from immunized mammals. The preparation and purification of chemical dye- or reporter protein-antibody conjugates is often complicated and expensive and not commonplace in academic laboratories. In response, researchers have developed comparatively simpler protein scaffolds for macromolecular recognition, which can be expressed with relative ease in E. coli and can be evolved to bind virtually any target. Nanobodies, a minimalist scaffold generated from camelid-derived heavy-chain IgGs, are one such example. A multitude of nanobodies have been evolved to recognize a diverse array of targets, including a short peptide. Here, this peptide tag (termed BC2T) and BC2 nanobody-dye conjugates or reporter protein fusions are evaluated in ELISA, flow cytometry, and Western blot experiments and compared to analogous experiments using commercially available antibody-conjugate/peptide tag pairs. Collectively, the utility and practicality of nanobody-based reagents in bioanalytical chemistry is demonstrated.

摘要

酶联免疫吸附测定(ELISA)、流式细胞术和 Western blot 是常见的生物分析技术。传统上,成功执行这些技术需要使用一种或多种市售的抗体-小分子染料或抗体-报告蛋白缀合物,这些缀合物可识别相对较短的肽标签(<15 个氨基酸)。然而,抗体的大小及其分子复杂性(由于翻译后二硫键形成和糖基化)通常需要在哺乳动物细胞中表达或从免疫的哺乳动物中纯化。化学染料或报告蛋白-抗体缀合物的制备和纯化通常很复杂且昂贵,并且在学术实验室中并不常见。为了应对这一挑战,研究人员开发了用于大分子识别的相对简单的蛋白质支架,这些支架可以相对容易地在大肠杆菌中表达,并可以进化以结合几乎任何目标。纳米抗体就是一个这样的例子,它是从小麦衍生的重链 IgG 中产生的最小化支架。已经进化出了多种纳米抗体来识别各种不同的目标,包括短肽。在这里,研究人员评估了这种肽标签(称为 BC2T)和 BC2 纳米抗体-染料缀合物或报告蛋白融合物在 ELISA、流式细胞术和 Western blot 实验中的应用,并将其与使用市售抗体-缀合物/肽标签对的类似实验进行了比较。总的来说,纳米抗体基试剂在生物分析化学中的实用性和实用性得到了证明。

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