Hall B M, Pearce N W, Gurley K E, Dorsch S E
Department of Renal Medicine, Royal Prince Alfred Hospital, Camperdown, New South Wales, Australia.
J Exp Med. 1990 Jan 1;171(1):141-57. doi: 10.1084/jem.171.1.141.
The cellular basis of the specific unresponsiveness that develops in DA rats treated with cyclosporine (CSA) for 10 d after grafting a PVG heart was examined using an adoptive transfer assay. CD4+ cells from rats with long survival grafts specifically lack the capacity to restore PVG heart graft rejection, and can also inhibit the capacity of naive T cells to restore rejection, while in the first few weeks post-transplant, both CD4+ and CD8+ T cells from CSA-treated hosts have the capacity to effect PVG graft rejection. In this study, we demonstrated the CD4+ suppressor cells also had the capacity to inhibit restoration of rejection by CD4+ cells from CSA-treated DA rats recently transplanted with PVG hearts, and from rats sensitized to third party, but not from those specifically sensitized to PVG. They also inhibited the capacity of both naive CD8+ and sensitized CD8+ cells to effect rejection. These results showed that the CD4+ suppressor cell was capable of overriding the capacity to effect rejection of the CD4+ cell and activated CD8+ cells that were present in the CSA-treated host shortly after transplantation. The failure of naive CD8+ cells to augment suppression and the capacity of CD4+ suppressor cells to transfer unresponsiveness to irradiated hosts in which regeneration of CD8+ cells was abolished by thymectomy suggested that it was the CD4+ cell alone that mediated suppression. However, the failure of CD4+ suppressor cells to reinduce unresponsiveness in irradiated hosts whose CD8+ cells had been depleted by therapy with the mAb MRC Ox8 showed that a radioresistant CD8+ cell was required to reestablish the state of specific unresponsiveness. The induction of CD4+ suppressor cells in thymectomized hosts suggested that these cells were derived from long-lived CD4+ lymphocytes. However, their sensitivity to cyclophosphamide and their loss of suppressor function both after removal of the graft and after 3 d in culture demonstrated that the suppressor cell itself had a short lifespan. The CD4+ suppressor was shown to be MRC Ox22+ (CD45R+), MRC Ox17+ (MHC class II), and MRC Ox39+ (CD25, IL-2-R). These studies demonstrated the CD4+ suppressive cell identified in rats with specific unresponsiveness induced by CSA therapy had many features of the suppressor inducer cell identified in in vitro studies of the alloimmune response.(ABSTRACT TRUNCATED AT 400 WORDS)
采用过继转移试验,研究了环孢素(CSA)处理10天的DA大鼠在移植PVG心脏后产生特异性无反应性的细胞基础。长期存活移植的大鼠的CD4 +细胞特别缺乏恢复PVG心脏移植排斥反应的能力,并且还可以抑制幼稚T细胞恢复排斥反应的能力,而在移植后的最初几周内,CSA处理宿主的CD4 +和CD8 + T细胞都有能力引起PVG移植排斥反应。在本研究中,我们证明CD4 +抑制细胞也有能力抑制最近移植PVG心脏的CSA处理的DA大鼠以及对第三方致敏的大鼠的CD4 +细胞恢复排斥反应,但不能抑制对PVG特异性致敏的大鼠的CD4 +细胞恢复排斥反应。它们还抑制了幼稚CD8 +和致敏CD8 +细胞引起排斥反应的能力。这些结果表明,CD4 +抑制细胞能够超越移植后不久CSA处理宿主中存在的CD4 +细胞和活化CD8 +细胞的排斥反应能力。幼稚CD8 +细胞未能增强抑制作用,以及CD4 +抑制细胞将无反应性转移至经胸腺切除术消除CD8 +细胞再生的辐照宿主的能力,表明单独的CD4 +细胞介导了抑制作用。然而,CD4 +抑制细胞未能在经单克隆抗体MRC Ox8治疗耗尽CD8 +细胞的辐照宿主中重新诱导无反应性,表明需要抗辐射的CD8 +细胞来重新建立特异性无反应状态。在胸腺切除的宿主中诱导CD4 +抑制细胞表明这些细胞来源于长寿的CD4 +淋巴细胞。然而,它们对环磷酰胺的敏感性以及在移除移植物后和培养3天后抑制功能丧失表明抑制细胞本身寿命较短。CD4 +抑制细胞显示为MRC Ox22 +(CD45R +),MRC Ox17 +(MHC II类)和MRC Ox39 +(CD25,IL-2-R)。这些研究表明,在CSA治疗诱导的特异性无反应性大鼠中鉴定出的CD4 +抑制细胞具有在同种免疫反应的体外研究中鉴定出的抑制诱导细胞的许多特征。(摘要截断于400字)
