Trivedi H L, Vanikar A V, Modi P R, Shah V R, Vakil J M, Trivedi V B, Khemchandani S I
Department of Nephrology and Clinical Transplantation, Institute of Kidney Diseases & Research Centre and Institute of Transplantation Sciences, Gujarat, India.
Transplant Proc. 2005 Mar;37(2):737-42. doi: 10.1016/j.transproceed.2005.01.028.
We designed a prospective, randomized, and controlled clinical trial to evaluate the efficacy and safety of achieving a mixed chimerism-associated tolerance protocol for recipients of living related donor (LRD) renal allografts.
Sixty-six consecutive patients were divided into two equal groups of 33 patients with end-stage renal disease. They were enrolled for transplantation after negative lymphocytotoxicity cross-matching (LCM). Both groups (treated [Tn] and control [Cn]) showed similar clinical and laboratory parameters and donor HLA match profiles. The Tn group underwent thymic transplantation of donor renal tissue, two donor-specific transfusions, low-intensity conditioning, and high-dose hematopoietic stem-cell transplantation (HSCT) before renal transplantation. The conditioning regimen included low-dose, target-specific irradiation (to abdominal and inguinal lymph nodes, bone marrow [BM] from thoracolumbar vertebrae and part of the pelvis on alternate days, 100 rad x 4), anti-T-cell antibodies (1.5 mg/kg body weight [BW]), cyclophosphamide (10 mg/kg BW x 2 consecutive days), and cyclosporine (CyA; >3 mg/kg BW/d). Unfractionated HSCT procured from the donor marrow was administered into the BM, portal and peripheral circulations, within 24 hours of achieving CD 4+/CD 8+ T-cell count less than 10% of normal. This infusion was supplemented with a dose of peripherally mobilized stem cells (mean total dose of 20 x 10(8) cells/kg recipient BW) administered peripherally. Renal transplantation was performed after negative LCM. Donor-specific cytotoxic antibodies were eliminated with intravenous immunoglobulins and plasmapheresis before renal transplantation. Mixed chimerism was evaluated before and after transplantation at monthly intervals in patients with donors of opposite gender by the FISH technique. Both groups received CyA and prednisolone for immunosuppression; Cn subjects also received mycophenolate mofetil/azathioprine. Rejection was treated with standard treatment. Immunosuppression was withdrawn 6 months after renal transplantation for patients with consistently positive chimerism. Clinical tolerance was defined as stable allograft function for more than 100 days without immunosuppression and confirmed by allograft biopsy.
Over a mean follow-up of 210 days, all Tn patients showed stable allograft function with mean serum creatinines (SCr) of 1.20 mg/dL, no rejection/CMV infections/graft or patient loss. A low-level donor-specific cytotoxic antibody was observed in all Tn patients. The CyA toxicity was noted in 10 (30.3%) patients. Persistent mixed hematopoietic chimerism was seen in all 21 patients irrespective of donor-recipient HLA matching (mean 0.5% before and 1 +/- 0.3% after transplantation). All four patients on drug withdrawal have shown donor-specific tolerance at a mean follow-up of 129.8 days. Other Tn patients are in the process of being weaned off immunosuppression. Mean SCr of controls was 1.45 mg/dL over a mean follow-up of 216 days. Acute rejection was observed in 17 (51.5%) patients; no CMV infection/patient loss was noted and one (3.03%) graft was lost in controls. No patient was lost in controls. No graft-versus-host disease was observed in Tn patients.
We have achieved mixed hematopoietic chimerism-associated tolerance with high-dose HSCT, intrathymic donor renal tissue transplantation, and minimal conditioning without any adverse effects.
我们设计了一项前瞻性、随机对照临床试验,以评估实现混合嵌合相关耐受方案对活体亲属供体(LRD)肾移植受者的疗效和安全性。
66例连续性患者被分为两组,每组33例终末期肾病患者。他们在淋巴细胞毒性交叉配型(LCM)阴性后入选进行移植。两组(治疗组[Tn]和对照组[Cn])显示出相似的临床和实验室参数以及供体HLA匹配情况。Tn组在肾移植前接受供体肾组织胸腺移植、两次供体特异性输血、低强度预处理以及高剂量造血干细胞移植(HSCT)。预处理方案包括低剂量、靶向性照射(隔日照射腹部和腹股沟淋巴结、胸腰椎和部分骨盆的骨髓[BM],100拉德×4)、抗T细胞抗体(1.5毫克/千克体重[BW])、环磷酰胺(10毫克/千克BW×连续2天)以及环孢素(CyA;>3毫克/千克BW/天)。在CD4+/CD8+T细胞计数低于正常水平的10%后24小时内,将从供体骨髓中获取的未分离HSCT注入BM、门静脉和外周循环。此次输注还补充了一剂外周动员干细胞(平均总剂量为20×10⁸细胞/千克受者BW),经外周给予。在LCM阴性后进行肾移植。在肾移植前,通过静脉注射免疫球蛋白和血浆置换消除供体特异性细胞毒性抗体。对于性别相反供体的患者,在移植前后每月通过FISH技术评估混合嵌合情况。两组均接受CyA和泼尼松龙进行免疫抑制;Cn组患者还接受霉酚酸酯/硫唑嘌呤。排斥反应采用标准治疗。对于嵌合持续阳性的患者,在肾移植后6个月停用免疫抑制药物。临床耐受定义为在无免疫抑制的情况下移植肾功能稳定超过100天,并通过移植肾活检证实。
在平均210天的随访期内,所有Tn组患者移植肾功能均稳定,平均血清肌酐(SCr)为1.20毫克/分升,无排斥反应/巨细胞病毒感染/移植肾或患者丢失情况。所有Tn组患者均观察到低水平的供体特异性细胞毒性抗体。10例(30.3%)患者出现CyA毒性。所有21例患者均出现持续的混合造血嵌合,无论供体 - 受体HLA匹配情况如何(移植前平均为0.5%,移植后为1±0.3%)。所有4例停药患者在平均129.8天的随访期内均表现出供体特异性耐受。其他Tn组患者正在逐渐减少免疫抑制药物用量。对照组在平均216天的随访期内平均SCr为1.45毫克/分升。17例(51.5%)患者发生急性排斥反应;未观察到巨细胞病毒感染/患者丢失情况,对照组有1例(3.03%)移植肾丢失。对照组无患者死亡。Tn组患者未观察到移植物抗宿主病。
我们通过高剂量HSCT、胸腺内供体肾组织移植以及最小化预处理实现了混合造血嵌合相关耐受,且无任何不良反应。
