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A rapid screening and production method using a novel mammalian cell display to isolate human monoclonal antibodies

机译:一种使用新型哺乳动物细胞展示物分离人单克隆抗体的快速筛选和生产方法

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摘要

Antibody display methods are increasingly being used to produce human monoclonal antibodies for disease therapy. Rapid screening and isolation of specific human antibody genes are valuable for producing human monoclonal antibodies showing high specificity and affinity. In this report, we describe a novel mammalian cell display method in which whole human IgG is displayed on the cell surface of CHO cells. Cells expressing antigen-specific human monoclonal IgGs with high affinity on the cell surface after normal folding and posttranscriptional modification were screened using a cell sorter. The membrane-type IgG-expressing CHO cells were then converted to IgG-secreting cells by transfection with a plasmid coding Cre recombinase. This mammalian cell display method was applied to in vitro affinity maturation of monoclonal C9 IgG specific to the human high-affinity IgE receptor (FcεRIα). The CDR3 of the C9 heavy chain variable region gene was randomly mutated and inserted into pcDNA5FRT/IgG. A C9 IgG (CDRH3r)-expressing CHO cell display library consisting of 1.1 × 106 independent clones was constructed. IgG-displaying cells showing high reactivity to FcεRIα antigen were screened by the cell sorter, resulting in the establishment of a CHO cell line producing with higher reactivity than the parent C9 IgG.
机译:抗体展示方法越来越多地用于生产用于疾病治疗的人单克隆抗体。快速筛选和分离特定人类抗体基因对于产生显示高特异性和亲和力的人类单克隆抗体很有价值。在这份报告中,我们描述了一种新型的哺乳动物细胞展示方法,其中整个人IgG在CHO细胞的细胞表面上展示。使用细胞分选仪筛选在正常折叠和转录后修饰后在细胞表面具有高亲和力的表达抗原特异性人单克隆IgG的细胞。然后通过用编码Cre重组酶的质粒转染,将表达膜型IgG的CHO细胞转化为分泌IgG的细胞。该哺乳动物细胞展示方法应用于对人高亲和力IgE受体(FcεRIα)特异的单克隆C9 IgG的体外亲和力成熟。 C9重链可变区基因的CDR3被随机突变并插入pcDNA5FRT / IgG。构建了一个表达C9 IgG(CDRH3r)的CHO细胞展示文库,该文库由1.1×106个独立克隆组成。通过细胞分选仪筛选对FcεRIα抗原具有高反应性的IgG展示细胞,从而建立了与亲本C9 IgG相比具有更高反应性的CHO细胞系。

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