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Methods for comprehensive identification of membrane proteins recognized by a large number of monoclonal antibodies.

机译:全面鉴定被大量单克隆抗体识别的膜蛋白的方法。

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摘要

In order to isolate monoclonal antibodies (mAbs) that bind to tumor-associated antigens (Ags) we developed the following strategy. Using the phage-display Ab library we isolated a large number of mAbs that bind to the surface of human tumor cells. The mAbs were individually screened by immunostaining, and clones that preferentially and strongly stained the malignant cells were chosen. Thereafter, the Ags recognized by the mAbs were identified. For identification of the Ags by MS candidate molecules had to be purified either by immunoprecipitation or by affinity chromatography. We isolated several hundred mAbs that showed cancer-specific staining patterns. In order to identify the Ags that were recognized by the numerous mAbs within a short time we developed two methods. Using the GFC [grouping of clones by flow cytometry (FCM)] method many Abs could be grouped by comparing the staining patterns of FCM. Members in each group turned out to bind to the same molecule in many cases. After a candidate Ag was revealed, the polypeptide corresponding to its extracellular portion was prepared and used for identification of clones that bound to the Ag among all the mAbs by SITE (simultaneous identification of clones through three dimensional ELISA) method. Both methods can be generally applicable to various kinds of membrane proteins and the mAbs against them.
机译:为了分离与肿瘤相关抗原(Ags)结合的单克隆抗体(mAb),我们开发了以下策略。使用噬菌体展示抗体库,我们分离了许多与人肿瘤细胞表面结合的单克隆抗体。通过免疫染色分别筛选mAb,并选择优先和强烈染色恶性细胞的克隆。此后,鉴定了被mAb识别的Ag。为了通过MS鉴定Ag,必须通过免疫沉淀或亲和色谱法纯化候选分子。我们分离了显示癌症特异性染色模式的几百个mAb。为了鉴定在短时间内被众多mAb识别的Ag,我们开发了两种方法。使用GFC [通过流式细胞术(FCM)对克隆进行分组]方法,可以通过比较FCM的染色模式将许多Abs分组。事实证明,在许多情况下,每个组中的成员都与同一分子结合。在揭示候选Ag后,制备对应于其细胞外部分的多肽,并用于通过SITE(通过三维ELISA同时鉴定克隆)方法鉴定所有mAb中与Ag结合的克隆。两种方法通常可适用于各种膜蛋白以及针对它们的mAb。

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