抗cd40培养人B淋巴细胞抗原特异性抗体诱导的研究。

B M Schilizzi, M C Harmsen, T H The, L De Leij
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引用次数: 1

摘要

B细胞需要T细胞提供的共刺激信号来产生针对T依赖性抗原的特异性抗体。我们研究了CD40培养系统在以巨细胞病毒(CMV)或破伤风类毒素(TT)为抗原的ag特异性人B细胞增殖和分化中的适用性。我们对CD40培养系统(cd32转染的L细胞、抗CD40细胞和IL-4细胞)进行了改进,通过连续的细胞因子刺激,并将总B细胞培养与预先筛选的抗原特异性B细胞进行了比较。当抗原选择的B细胞在CD40系统中培养7天诱导克隆扩增,然后再添加IL-2和IL-10诱导7天诱导浆细胞分化时,特异性抗体的检测成为可能。我们得出结论,我们最初无法在CD40系统中检测特异性抗体是由于非特异性B细胞克隆的过度生长,而通过筛选抗原特异性B细胞克服了这一问题。当在筛选过程中与抗原的初次接触限制在1至24小时之间时,发现抗原特异性抗体产生的诱导是最佳的。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Studies on the induction of antigen-specific antibody in anti-CD40 cultured human B lymphocytes.

Costimulatory signals provided by T cells are required for B cells to produce specific antibody to T-dependent antigen. We have investigated the suitability of using the CD40 culture system for the proliferation and differentiation of Ag-specific human B cells using cytomegalovirus (CMV) or tetanus toxoid (TT) as antigen. We modified the CD40 culture system (CD32-transfected L cells, anti-CD40, and IL-4) by applying a sequential cytokine stimulation and compared total B-cell cultures with antigen-specific B cells preselected by panning. The detection of specific antibody became possible when antigen-selected B cells were cultured for 7 days in the CD40 system to induce clonal expansion, followed by the addition of IL-2 and IL-10 for an additional 7 days to induce plasma-cell differentiation. We conclude that our initial inability to detect specific antibody in the CD40 system is due to overgrowth of nonspecific B-cell clones and that selection of antigen-specific B cells by panning overcomes this problem. Induction of antigen-specific antibody production was found to be optimal when the initial contact with antigen during panning was limited to between 1 to 24 hours.

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