Gallon Lorenzo, Traitanon Opas, Yu Yuming, Shi Bo, Leventhal Joseph R, Miller Joshua, Mas Valeria, L Xu, Mathew James M
1 Department of Medicine-Nephrology, Northwestern University Feinberg School of Medicine, Chicago, IL. 2 Comprehensive Transplant Center, Northwestern University Feinberg School of Medicine, Chicago, IL. 3 Department of Surgery, Northwestern University Feinberg School of Medicine, Chicago, IL. 4 Department of Medicine and Rheumatology Division, Northwestern University Feinberg School of Medicine, Chicago, IL. 5 Department of Microbiology-Immunology, Northwestern University Feinberg School of Medicine, Chicago, IL. 6 Department of Surgery, University of Virginia, Charlottesville, VA.
Transplantation. 2015 Sep;99(9):1774-84. doi: 10.1097/TP.0000000000000717.
Previously, we had reported the role of tacrolimus (TAC) versus sirolimus (SRL) on the generation of regulatory T cells (Tregs) in primary MLR assays with SRL, demonstrating a uniquely supportive effect. However, the mechanisms associated with their actions on alloreactive human T cells are not fully understood. Therefore, we tested whether TAC and SRL differentially affect already alloactivated human CD4 T-cell subsets.
Alloreactive CD4CD45RA/CD45RO T cells generated in 9-day MLR were cocultured with anti-CD3 and autologous antigen presenting cells plus interleukin (IL)-2 in presence of TAC, SRL, or both, and the Tregs generated after another 5 to 6 days were phenotypically, molecularly, and functionally characterized.
Tacrolimus significantly and SRL modestly inhibited interferon (IFN)-γ (Th1) and IL-17 (Th17)-producing cells. At clinical therapeutic concentrations, SRL, however, significantly increased forkhead/winged helix transcription factor P3 (FOXP3) Tregs, whereas TAC inhibited this T-cell population dose dependently and significantly. When used in combination, TAC and SRL had additive effects on inhibition of IFN-γ- and IL-17-producing cells. This was in contrast to the ability of SRL to reverse TAC-mediated inhibition of FOXP3-expressing cells. Proinflammatory cytokines (IL-1β, IL-6, and tumor necrosis factor-α) added to cultures caused significant decrease in FOXP3 Tregs that was again reversed by SRL. Sirolimus-derived Tregs were phenotypically normal, anergic to allostimulation, and suppressed proliferation of allogeneic effector T-cells.
Thus, although TAC inhibits all alloreactive T cells, SRL promotes the differentiation and expansion of donor-specific Tregs without secondary reprogramming to IFN-γFOXP3 and IL-17FOXP3 Treg subsets. These results, although performed in an artificial in vitro model, add clinically applicable information on how these agents affect T-cell subpopulations.
此前,我们曾报道过在使用西罗莫司(SRL)的初次混合淋巴细胞反应(MLR)试验中,他克莫司(TAC)与西罗莫司对调节性T细胞(Tregs)生成的作用,显示出独特的支持作用。然而,它们对同种异体反应性人类T细胞作用的相关机制尚未完全明确。因此,我们测试了TAC和SRL是否对已经被同种异体激活的人类CD4 T细胞亚群有不同影响。
在9天的MLR中产生的同种异体反应性CD4CD45RA/CD45RO T细胞,在TAC、SRL或两者存在的情况下,与抗CD3、自体抗原呈递细胞以及白细胞介素(IL)-2共同培养,另外5至6天后产生的Tregs进行表型、分子和功能特征分析。
他克莫司显著抑制、西罗莫司适度抑制产生干扰素(IFN)-γ(Th1)和IL-17(Th17)的细胞。然而,在临床治疗浓度下,西罗莫司显著增加叉头/翼状螺旋转录因子P3(FOXP3)Tregs,而他克莫司剂量依赖性且显著地抑制这群T细胞。当联合使用时,TAC和SRL对抑制产生IFN-γ和IL-17的细胞有相加作用。这与西罗莫司逆转他克莫司介导的对表达FOXP3细胞的抑制能力形成对比。添加到培养物中的促炎细胞因子(IL-1β、IL-6和肿瘤坏死因子-α)导致FOXP3 Tregs显著减少,而这又被西罗莫司逆转。源自西罗莫司的Tregs表型正常,对同种异体刺激无反应,并抑制同种异体效应T细胞的增殖。
因此,尽管他克莫司抑制所有同种异体反应性T细胞,但西罗莫司促进供体特异性Tregs的分化和扩增,而不会二次重编程为IFN-γFOXP3和IL-17FOXP3 Treg亚群。这些结果尽管是在人工体外模型中进行的,但增加了关于这些药物如何影响T细胞亚群的临床适用信息。
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