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Determination of helper T-cell precursor frequencies against non-haemopoietic cells: comparison of co-stimulation provided by anti-CD28 antibody versus the cellular ligand B7-1

机译:确定针对非造血细胞的辅助性T细胞前体频率:抗CD28抗体与细胞配体B7-1共同刺激的比较

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摘要

Helper T-cell precursor frequency assays (HTLp-assays) are commonly used in transplantation to examine the frequency of T cells reactive against donor or host alloantigens. In these assays, peripheral blood mononuclear cells (PBMCs) are most often used as stimulator cells. However, cells targeted after transplantation do not always belong to the haematopoietic lineage and may express different alloantigens, especially minor histocompatibility antigens (mHags). Non-haematopoietic cells lack expression of the B7 co-stimulatory molecules needed to activate primary T cells that can be supplied by anti-CD28 (alphaCD28) antibodies or transfection with B7-1 coding sequences. At present, it is not known how these two ways of supplied co-stimulation compare in HTLp assays. B7-1-transfected A431 keratinocytes (A431B7-1) induced higher proliferative responses in allogeneic primary T cells and more interleukin (IL) 2 production than that induced by A431 cells plus alphaCD28, whereas the kinetics of proliferation and IL-2 production were similar. Neither cross-linking of alphaCD28 bound to T cells nor prevention of IL-2 resorption by the anti-IL-2 receptor resulted in improved proliferation or IL-2 production. Results of HTLp assays indicated that A431B7-1 activated on average 7.5 times more alloreactive IL-2-producing T cells than A431 cells plus alphaCD28. We conclude that primary T-cell alloresponses against major histocompatibility complexes (MHCs) and mHags expressed on non-haematopoietic cells can be measured in HTLp assays using supplied co-stimulation, although alphaCD28 yields an intrinsic underestimation of actual frequencies
机译:辅助性T细胞前体频率测定法(HTLp测定)通常用于移植中,以检查对供体或宿主同种抗原具有反应性的T细胞的频率。在这些测定中,外周血单核细胞(PBMC)最常用作刺激细胞。但是,移植后靶向的细胞并不总是属于造血谱系,并且可能表达不同的同种抗原,尤其是次要的组织相容性抗原(mHags)。非造血细胞缺乏激活原代T细胞所需的B7共刺激分子的表达,而原代T细胞可以由抗CD28(alphaCD28)抗体或B7-1编码序列转染来提供。目前,尚不知道如何在HTLp分析中比较这两种提供的共刺激方式。 B7-1转染的A431角质形成细胞(A431B7-1)在同种异体原代T细胞中诱导更高的增殖反应,并比A431细胞加alphaCD28诱导的白介素(IL)2产生更多,而增殖和IL-2产生的动力学相似。既不将αCD28交联到T细胞上,也没有通过抗IL-2受体阻止IL-2的吸收,不会导致增殖或IL-2产生的改善。 HTLp分析的结果表明,与A431细胞加alphaCD28相比,A431B7-1激活的产生同种异体反应性IL-2的T细胞平均活化7.5倍。我们得出的结论是,尽管αCD28产生固有的低估实际频率,但可以使用提供的共刺激在HTLp分析中测量针对非组织细胞表达的主要组织相容性复合体(MHC)和mHags的原代T细胞过敏反应

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