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Detailed Kinetics of the Direct Allo-Response in Human Liver Transplant Recipients: New Insights from an Optimized Assay

机译:人类肝脏移植受者中直接同种异体反应的详细动力学:优化分析的新见解

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摘要

Conventional assays for quantification of allo-reactive T-cell precursor frequencies (PF) are relatively insensitive. We present a robust assay for quantification of PF of T-cells with direct donor-specificity, and establish the kinetics of circulating donor-specific T cells after liver transplantation (LTx). B cells from donor splenocytes were differentiated into professional antigen-presenting cells by CD40-engagement (CD40-B cells). CFSE-labelled PBMC from LTx-recipients obtained before and at several time points after LTx, were stimulated with donor-derived or 3rd party CD40-B cells. PF of donor-specific T cells were calculated from CFSE-dilution patterns, and intracellular IFN-γ was determined after re-stimulation with CD40-B cells. Compared to splenocytes, stimulations with CD40-B cells resulted in 3 to 5-fold higher responding T-cell PF. Memory and naïve T-cell subsets responded equally to allogeneic CD40-B cell stimulation. Donor-specific CD4+ and CD8+ T-cell PF ranged from 0.5 to 19% (median: 5.2%). One week after LTx, PF of circulating donor-specific CD4+ and CD8+ T cells increased significantly, while only a minor increase in numbers of T cells reacting to 3rd party allo-antigens was observed. One year after LTx numbers of CD4+ and CD8+ T cells reacting to donor antigens, as well as those reacting to 3rd party allo-antigens, were slightly lower compared to pre-transplant values. Moreover, CD4+ and CD8+ T cells responding to donor-derived, as well as those reacting to 3rd party CD40-B cells, produced less IFN-γ. In conclusion, our alternative approach enables detection of allo-reactive human T cells at high frequencies, and after application we conclude that donor-specific T-cell PF increase immediately after LTx. However, no evidence for a specific loss of circulating T-cells recognizing donor allo-antigens via the direct pathway up to 1 year after LTx was obtained, underscoring the relative insensitiveness of previous assays.
机译:用于定量同种反应性T细胞前体频率(PF)的常规测定相对不敏感。我们提出了一种具有定量的直接供体特异性T细胞PF的强大测定方法,并建立了肝移植(LTx)后循环供体特异性T细胞的动力学。来自供体脾细胞的B细胞通过CD40参与而分化成专业的抗原呈递细胞(CD40-B细胞)。在供体来源或第3方CD40-B细胞刺激下,在LTx之前和之后几个时间点获得的,来自LTx受体的CFSE标记的PBMC。由CFSE稀释模式计算供体特异性T细胞的PF,并用CD40-B细胞再次刺激后测定细胞内IFN-γ。与脾细胞相比,CD40-B细胞刺激导致应答性T细胞PF升高3至5倍。记忆和幼稚T细胞亚群对同种异体CD40-B细胞刺激的反应相同。供体特异性CD4 + 和CD8 + T细胞PF范围为0.5%至19%(中位数:5.2%)。 LTx一周后,循环供体特异性CD4 + 和CD8 + T细胞的PF显着增加,而对3 rd 方同种抗原。 CD4 + 和CD8 + T细胞与供体抗原以及与3 rd 缔约方同种异体抗原反应的LTx数量一年后与移植前的值相比,抗原含量略低。此外,对供体来源的CD4 + 和CD8 + T细胞以及对3 rd 方CD40-B细胞有反应的细胞,产生较少的IFN-γ。总而言之,我们的替代方法使得能够以高频率检测同种反应性人类T细胞,并且在应用后我们得出结论,供体特异性T细胞PF在LTx之后立即增加。然而,没有证据表明直到LTx后长达1年都通过直接途径识别供体同种异体抗原的循环T细胞发生了特定损失,强调了先前测定的相对敏感性。

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