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在正常小鼠CD4(+) T淋巴细胞中,抗体诱导的CD3-CD4共连接在缺乏共刺激信号的情况下抑制TCR/CD3激活。

Antibody-induced CD3-CD4 coligation inhibits TCR/CD3 activation in the absence of costimulatory signals in normal mouse CD4(+) T lymphocytes.

作者信息

Portolés P, de Ojeda G, Criado G, Fernández-Centeno E, Rojo J M

机构信息

Centro Nacional de Biología Fundamental, Instituto de Salud Carlos III-C.S.I.C., Madrid, E-28220, Spain.

出版信息

Cell Immunol. 1999 Aug 1;195(2):96-109. doi: 10.1006/cimm.1999.1529.

DOI:10.1006/cimm.1999.1529
PMID:10448009
Abstract

The effect of CD3-CD4 coligation on CD3-mediated activation of normal mouse CD4(+) T lymphocytes has been analyzed in the absence of exogenous lymphokines. If anti-CD3 and anti-CD4 antibodies are adsorbed to culture wells by means of previously adsorbed anti-Ig antibodies (indirect binding), CD3-CD4 coligation inhibits activation measured as cell proliferation or as secretion of IL-2, IL-4, and IFN-gamma. Addition of IL-2, anti-CD28 antibodies, or phorbol esters, but not IL-1, IL-4, or ionomycin, blocked CD4-mediated inhibition and restored the response to levels equal or higher than those of cultures activated by anti-CD3 alone. In contrast, CD3-CD4 coligation by antibodies directly adsorbed to culture wells potentiated anti-CD3-induced activation, either in the absence or in the presence of exogenous costimuli. Similar results were observed when CD4(+) T cells of naive phenotype (CD44(low), CD45RB(high)) were used in the experiments. The analysis of early tyrosine phosphorylation in CD4(+) T cells shows that phosphorylation of many cell substrates is clearly enhanced upon CD3-CD4 coligation using indirectly or directly bound antibodies, yet certain substrates are mainly phosphorylated under inhibitory conditions. Although CD28 ligation does not produce any clear change in the tyrosine phosphorylation pattern in lysates from cells activated by indirectly bound anti-CD3 plus anti-CD4 antibodies, the analysis of active forms of the MAP kinase ERK suggests that downstream signaling pathways involved in IL-2 gene activation can be differentially activated depending on the direct or indirect CD3-CD4 adsorption and CD28 ligation.

摘要

在不存在外源性淋巴因子的情况下,分析了CD3-CD4共结合对正常小鼠CD4(+) T淋巴细胞CD3介导的激活作用。如果抗CD3和抗CD4抗体通过预先吸附的抗Ig抗体吸附到培养孔中(间接结合),CD3-CD4共结合会抑制以细胞增殖或IL-2、IL-4和IFN-γ分泌来衡量的激活。添加IL-2、抗CD28抗体或佛波酯,但不添加IL-1、IL-4或离子霉素,可阻断CD4介导的抑制作用,并将反应恢复到等于或高于仅用抗CD3激活的培养物的水平。相反,直接吸附到培养孔中的抗体进行的CD3-CD4共结合,无论是否存在外源性共刺激,都会增强抗CD3诱导的激活。当在实验中使用幼稚表型(CD44(low),CD45RB(high))的CD(+) T细胞时,观察到了类似的结果。对CD4(+) T细胞早期酪氨酸磷酸化的分析表明,使用间接或直接结合的抗体进行CD3-CD4共结合时,许多细胞底物的磷酸化明显增强,但某些底物主要在抑制条件下磷酸化。尽管CD28结合不会使间接结合的抗CD3加抗CD4抗体激活的细胞裂解物中的酪氨酸磷酸化模式产生任何明显变化,但对MAP激酶ERK活性形式的分析表明,参与IL-2基因激活的下游信号通路可根据CD3-CD4的直接或间接吸附以及CD28结合而被差异激活。

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