Institut Curie-Research Center, 26 rue d'Ulm, Paris cedex 05, France.
BMC Biotechnol. 2010 Aug 22;10:59. doi: 10.1186/1472-6750-10-59.
Due to their unique ability to bind their targets with high fidelity, antibodies are used widely not only in biomedical research, but also in many clinical applications. Recombinant antibodies, including single chain variable fragments (scFv), are gaining momentum because they allow powerful in vitro selection and manipulation without loss of function. Regardless of the ultimate application or type of antibody used, precise understanding of the interaction between the antibody's binding site and its specific target epitope(s) is of great importance. However, such data is frequently difficult to obtain.
We describe an approach that allows detailed characterization of a given antibody's target(s) using the yeast two-hybrid system. Several recombinant scFv were used as bait and screened against highly complex cDNA libraries. Systematic sequencing of all retained clones and statistical analysis allowed efficient ranking of the prey fragments. Multiple alignment of the obtained cDNA fragments provided a selected interacting domain (SID), efficiently narrowing the epitope-containing region.Interactions between antibodies and their respective targets were characterized for several scFv. For AA2 and ROF7, two conformation-specific sensors that exclusively bind the activated forms of the small GTPases Rab6 and Rab1 respectively, only fragments expressing the entire target protein's core region were retained. This strongly suggested interaction with a non-linear epitope. For two other scFv, TA10 and SF9, which recognize the large proteins giantin and non-muscle myosin IIA, respectively, precise antibody-binding regions within the target were defined. Finally, for some antibodies, secondary targets within and across species could be revealed.
Our method, utilizing the yeast two-hybrid technology and scFv as bait, is a simple yet powerful approach for the detailed characterization of antibody targets. It allows precise domain mapping for linear epitopes, confirmation of non-linear epitopes for conformational sensors, and detection of secondary binding partners. This approach may thus prove to be an elegant and rapid method for the target characterization of newly obtained scFv antibodies. It may be considered prior to any research application and particularly before any use of such recombinant antibodies in clinical medicine.
由于抗体具有与靶标高亲和力结合的独特能力,因此不仅在生物医学研究中得到广泛应用,而且在许多临床应用中也得到广泛应用。包括单链可变片段(scFv)在内的重组抗体由于能够在不丧失功能的情况下进行强大的体外选择和操作而受到关注。无论最终应用或使用的抗体类型如何,精确了解抗体结合位点与其特定靶标表位(s)之间的相互作用都非常重要。但是,此类数据通常难以获得。
我们描述了一种使用酵母双杂交系统来详细表征给定抗体的靶标的方法。使用几种重组 scFv 作为诱饵,并针对高度复杂的 cDNA 文库进行筛选。对所有保留的克隆进行系统测序和统计分析,可有效地对猎物片段进行排序。获得的 cDNA 片段的多序列比对提供了一个选择的相互作用域(SID),有效地缩小了包含表位的区域。对几种 scFv 进行了抗体与其各自靶标的相互作用特征分析。对于 AA2 和 ROF7,这两种分别是特异性结合小 GTPase Rab6 和 Rab1 激活形式的构象传感器,仅保留表达整个靶蛋白核心区域的片段。这强烈表明存在非线性表位的相互作用。对于另外两种 scFv,TA10 和 SF9,分别识别大蛋白巨球蛋白和非肌肉肌球蛋白 IIA,分别定义了靶标内和靶标之间的精确抗体结合区域。最后,对于某些抗体,可以揭示种内和种间的次要靶标。
我们的方法利用酵母双杂交技术和 scFv 作为诱饵,是一种简单而强大的方法,可用于详细表征抗体靶标。它允许对线性表位进行精确的结构域作图,对构象传感器的非线性表位进行确认,并检测次级结合伴侣。因此,该方法可能是一种用于新获得的 scFv 抗体的靶标表征的优雅而快速的方法。在进行任何研究应用之前,特别是在将此类重组抗体用于临床医学之前,都可以考虑使用该方法。
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