Dextran-conjugated anti-IgD antibodies inhibit T cell-mediated IgE production but augment the synthesis of IgM and IgG.

免疫球蛋白D 同型 免疫球蛋白类转换 免疫球蛋白E 抗体 B细胞 分子生物学 生物 分泌物 细胞因子 白细胞介素4 免疫学 内分泌学 单克隆抗体
作者
L. M. T. Pecanha,Hideko Yamaguchi,Andrew Lees,R. J. Noelle,James J. Mond,Clifford M. Snapper
出处
期刊:Journal of Immunology [The American Association of Immunologists]
卷期号:150 (6): 2160-2168 被引量:12
标识
DOI:10.4049/jimmunol.150.6.2160
摘要

Abstract We previously demonstrated that anti-IgD antibodies conjugated to dextran (alpha delta-dex) were a potent co-stimulus for Ig secretion by resting murine B cells in the presence of cytokines. However, although alpha delta-dex stimulated the secretion of most Ig isotypes it selectively failed to costimulate IgE production even in the presence of high concentrations of IL-4. Earlier reports indicated that unconjugated anti-IgM, which was not an effective costimulus for Ig secretion, in fact inhibited Ig production induced by LPS. We determined the effect of alpha delta-dex, at concentrations that costimulated cytokine-induced Ig secretion, on Ig production by LPS- or T cell-activated B cells, and whether IgE production was affected in a selective manner. We observed that alpha delta-dex inhibited Ig isotype production (IgE > IgG > IgM) by LPS-activated B cells, while further stimulating their proliferation. This effect of alpha delta-dex was mediated directly at the level of the B cell and was accompanied by a comparable inhibition in Ig class switching, as assessed by flow cytometric analysis of membrane Ig isotype-positive cells. The inhibitory effects of alpha delta-dex on LPS-induced Ig secretion and class switching occurred at 1000-fold lower concentrations of anti-IgD than that reported necessary for inhibition by unconjugated anti-IgM. Whereas IL-4 + IL-5 costimulated Ig isotype production by alpha delta-dex-activated cells, the further addition of LPS led to a marked ablation of the Ig secretory response indicating the cross-inhibitory effects of these two modes of B cell activation. By contrast, alpha delta-dex augmented IgM and IgG1 secretion by resting B cells stimulated with either an anti-CD3-activated CD4+ Th2 clone or with activated T cell membranes in combination with IL-4 + IL-5. However, alpha delta-dex potently inhibited T cell-mediated IgE secretion. These findings underscore the existence of, and demonstrate a number of novel interrelationships between, three distinct pathways of B cell differentiation induced by different modes of activation. Further, the observation that pg/ml quantities of alpha delta-dex selectively inhibits T cell-induced IgE production in vitro suggests a novel strategy to down-regulate this Ig isotype in vivo.
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