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A Rapid Method to Characterize Mouse IgG Antibodies and Isolate Native Antigen Binding IgG B Cell Hybridomas

机译:一种表征小鼠IgG抗体并分离天然抗原结合IgG B细胞杂交瘤的快速方法

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摘要

B cell hybridomas are an important source of monoclonal antibodies. In this paper, we developed a high-throughput method to characterize mouse IgG antibodies using surface plasmon resonance technology. This assay rapidly determines their sub-isotypes, whether they bind native antigen and their approximate affinities for the antigen using only 50 μl of hybridoma cell culture supernatant. Moreover, we found that mouse hybridomas secreting IgG antibodies also have membrane form IgG expression without Igα. Based on this surface IgG, we used flow cytometry to isolate rare γ2a isotype switched variants from a γ2b antibody secreting hybridoma cell line. Also, we used fluorescent antigen to single cell sort antigen binding hybridoma cells from bulk mixture of fused hybridoma cells instead of the traditional multi-microwell plate screening and limiting dilution sub-cloning thus saving time and labor. The IgG monoclonal antibodies specific for the native antigen identified with these methods are suitable for in vivo therapeutic uses, but also for sandwich ELISA assays, histology, flow cytometry, immune precipitation and x-ray crystallography.
机译:B细胞杂交瘤是单克隆抗体的重要来源。在本文中,我们开发了一种高通量方法来使用表面等离子体共振技术表征小鼠IgG抗体。仅使用50μl杂交瘤细胞培养上清液,该测定即可快速确定其亚型,它们是否结合天然抗原及其对抗原的近似亲和力。而且,我们发现分泌IgG抗体的小鼠杂交瘤也具有膜形式的IgG表达而没有Igα。基于此表面IgG,我们使用流式细胞仪从分泌γ2b抗体的杂交瘤细胞系中分离了罕见的γ2a同型转换变体。此外,我们使用荧光抗原将融合杂交瘤细胞的大量混合物用于单细胞分类抗原结合杂交瘤细胞,而不是传统的多孔板孔板筛选和限制稀释亚克隆,从而节省了时间和精力。用这些方法鉴定的对天然抗原具有特异性的IgG单克隆抗体既适合体内治疗用途,也适合夹心ELISA分析,组织学,流式细胞仪,免疫沉淀和X射线晶体学检查。

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