Gorczynski R M, Chen Z, Zeng H, Gorczynski L, Terzioglu E
Department of Surgery, University of Toronto, Ontario, Canada.
Immunology. 1998 Feb;93(2):221-9. doi: 10.1046/j.1365-2567.1998.00403.x.
Irradiated (800 rads) AKR mice received intravenous (i.v.) reconstitution with a mixture of B10.BR T-depleted bone marrow cells and spleen cells. Only in groups of mice treated additionally with i.v. cyclophosphamide (Cy; 150 mg/kg), 24 hr before transplantation, was long-term (> 60% at 50 days) survival seen. In mice receiving only irradiation all animals died by 30 days post-transplantation. Histological changes consistent with graft-versus-host disease (GVHD) were seen in the liver of reconstituted mice at 30 days, along with an organ-specific increase in V beta 3 T-cell receptor-positive (TCR+) cells. No such increase in V beta 3 TCR+ cells was seen in the spleen from the same mice. These data are consistent with a tissue antigen-driven expansion of V beta 3 TCR+ cells associated with GVHD in the liver in this model. When we analysed cytokine production in vitro from CD3+ cells restimulated with 'host' (AKR) antigen-presenting cells (APC), we found a transition in cytokine production from preferential synthesis of type-1 cytokines [interleukin-2 (IL-2) and interferon-gamma (IFN-gamma)] at early times (day 15) post-reconstitution to increased production of type-2 cytokines [IL-4, transforming growth factor-beta (TGF-beta) and IL-10] at later times (day 30) post-reconstitution in Cy-treated recipients. Animals not receiving Cy did not show this 'switch' in cytokine production at later time points. We have observed a similar polarization in cytokine production, along with increased graft survival, in recipients of vascularized and non-vascularized allografts after portal venous (p.v.), but not i.v., pretransplant donor-specific immunization. We next studied AKR mice receiving 800 rads and subsequently reconstituted with B10.BR stem cells via the p.v. route. Again these mice showed prolonged survival (> 50% at 50 days), with polarization to IL-4, IL-10 and TGF-beta on restimulation of CD3+ cells in vitro at 30 days post-transplant and increased V beta 3 TCR+ cells in the liver. Infusion of anti-IL-12 monoclonal antibodies into irradiated mice receiving i.v. cell reconstitution produced a similar pattern of changes to those seen after p.v. reconstitution, while a combination of anti-IL-10 and anti-TGF-beta monoclonal antibodies reversed the changes seen after p.v. reconstitution. These data are consistent with an important role for differential cytokine production in the regulation of GVHD following allogeneic bone marrow transplantation.
用B10.BR T细胞去除的骨髓细胞和脾细胞混合物对经800拉德照射的AKR小鼠进行静脉内重建。只有在移植前24小时额外接受静脉内环磷酰胺(Cy;150毫克/千克)治疗的小鼠组中,才观察到长期(50天时>60%)存活。在仅接受照射的小鼠中,所有动物在移植后30天内死亡。在重建小鼠的肝脏中,在30天时观察到与移植物抗宿主病(GVHD)一致的组织学变化,同时Vβ3 T细胞受体阳性(TCR+)细胞出现器官特异性增加。在同一只小鼠的脾脏中未观察到Vβ3 TCR+细胞的这种增加。这些数据与该模型中肝脏中与GVHD相关的Vβ3 TCR+细胞的组织抗原驱动的扩增一致。当我们分析用“宿主”(AKR)抗原呈递细胞(APC)重新刺激的CD3+细胞的体外细胞因子产生时,我们发现在重建后早期(第15天)细胞因子产生从优先合成1型细胞因子[白细胞介素-2(IL-2)和干扰素-γ(IFN-γ)]转变为重建后后期(第30天)2型细胞因子[IL-4、转化生长因子-β(TGF-β)和IL-10]产生增加,在接受Cy治疗的受体中。未接受Cy的动物在后期时间点未显示这种细胞因子产生的“转换”。在门静脉(p.v.)而非静脉内进行移植前供体特异性免疫后,我们在血管化和非血管化同种异体移植物的受体中观察到类似的细胞因子产生极化以及移植物存活增加。接下来,我们研究了接受800拉德照射并随后通过p.v.途径用B10.BR干细胞重建的AKR小鼠。同样,这些小鼠显示出延长的存活(50天时>50%),在移植后30天体外重新刺激CD3+细胞时向IL-4、IL-10和TGF-β极化,并且肝脏中Vβ3 TCR+细胞增加。将抗IL-12单克隆抗体注入接受静脉内细胞重建的照射小鼠中产生了与p.v.重建后所见类似的变化模式,而抗IL-10和抗TGF-β单克隆抗体的组合逆转了p.v.重建后所见的变化。这些数据与异基因骨髓移植后细胞因子产生差异在GVHD调节中的重要作用一致。
