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首页> 外文期刊>Journal of Immunological Methods >Efficient generation of monoclonal antibodies from single human B cells by single cell RT-PCR and expression vector cloning.
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Efficient generation of monoclonal antibodies from single human B cells by single cell RT-PCR and expression vector cloning.

机译:通过单细胞RT-PCR和表达载体克隆从单个人B细胞高效生成单克隆抗体。

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摘要

We have developed an efficient strategy that combines immunoglobulin (Ig) gene repertoire analysis and Ig reactivity profiling at the single cell level. Based on surface marker expression individual cells at different stages of human B cell development are isolated by fluorescence-activated cell sorting. For each cell Ig heavy and corresponding Ig light chain gene transcripts are amplified by nested RT-PCR and cloned into eukaryotic expression vectors to produce monoclonal human antibodies of the same specificity in vitro. All reactions are performed in 96-well plates and allow cloning of large numbers of Ig genes. The recombinant antibodies are tested for reactivity with diverse self- and non-self antigens and the reactivity profile can be directly linked to the complete Ig heavy and Ig light chain gene sequence information that is obtained as part of the cloning strategy. In summary, our method to clone and express human monoclonal antibodies is unbiased, highly efficient, requires only small cell numbers and the recombinant antibodies allow direct conclusions on the frequency of specific human B cells in a diverse repertoire.
机译:我们已经开发了一种有效的策略,可以在单个细胞水平上结合免疫球蛋白(Ig)基因库分析和Ig反应性分析。根据表面标志物的表达,通过荧光激活细胞分选法分离人类B细胞发育不同阶段的单个细胞。对于每个细胞,通过嵌套RT-PCR扩增Ig重链和相应的Ig轻链基因转录物,并将其克隆到真核表达载体中,以在体外产生相同特异性的单克隆人抗体。所有反应均在96孔板上进行,并允许克隆大量Ig基因。测试了重组抗体与各种自身和非自身抗原的反应性,反应性谱可直接链接至完整的Ig重链和Ig轻链基因序列信息,该信息是克隆策略的一部分。总而言之,我们克隆和表达人单克隆抗体的方法是无偏见的,高效的,仅需少量细胞,重组抗体可以直接推断出不同谱系中特定人B细胞的频率。

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