Medicine and Surgery, San Raffaele Hospital Scientific Institute, Milan, Italy; the University of Milan, Milan, Italy; and the University San Raffaele Vita-Salute, Milan, Italy
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ABSTRACT |
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INTRODUCTION |
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Transplantation in type 1 diabetes is performed in the presence of an active or memory autoimmune response to islet autoantigens (6). That this autoimmune background also potentially contributes to allograft rejection and therefore also needs to be controlled by immunosuppression is suggested by 1) reports of inflammatory islet infiltration and selective ß-cell destruction after human pancreas and islet transplantation (7,8,9), 2) a profoundly lower success rate of islet allotransplantation in autoimmune diabetes models than in nonautoimmune models (10,11,12), 3) a lower success rate of islet transplantation in patients with type 1 diabetes than in nonautoimmune patients (1,13,14), 4) associations of graft failure with the presence of islet autoantibodies pretransplantation (15,16), and 5) rises in autoantibody titers and T-cell responses posttransplantation that correlate with subsequent graft failure (16,17,18,19,20,21). The relative contribution of islet autoimmunity to graft survival, however, remains unclear.
Type 1 diabetesassociated autoimmunity is readily measurable at the humoral level with standardized assays to the three major diabetes-related autoantigens: insulin, GAD, and IA-2 (22). We have shown that despite being under immunosuppression, a minority of patients who received pancreas plus kidney allografts showed a marked rise in antibodies to GAD (GADA) and/or protein tyrosine phosphatase IA-2 (IA-2A) from 1 to 3 years posttransplantation, and that the rise was associated with subsequent pancreas but not kidney graft failure (19). We studied 36 patients who received islet plus kidney or islet-only allografts, and remarkably, despite antilymphocyte (ALG)/antithymocyte (ATG) globulin and immunosuppressive treatment, we observed subjects with major rises in IgG1 GADA within 7 days posttransplantation, indicating indirect or direct presentation of autoantigen. Some but not all of these cases were accompanied by the appearance of HLA class I or class IIspecific antibodies, suggesting that autoreactivity may be independent of allorejection. There was a relationship between response characteristics and both the immunosuppressive treatment received by the patients and graft function. These data indicate that autoimmunity in patients with type 1 diabetes is likely to contribute significantly to islet allograft survival and should be considered in patient management and when designing therapeutic regimens.
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RESEARCH DESIGN AND METHODS |
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In five patients, islets were transplanted simultaneously with kidney graft. The remaining 28 transplantations were performed after kidney graft alone or after a simultaneous pancreas and kidney graft in which pancreas failed mainly for thrombosis (median time after kidney transplantation, 21 months [1126]).
In the five patients who received simultaneous islet and kidney transplants, islets were always from the same donor of the kidney, and in two of these patients, they were also from two additional donors; in the 28 islet transplants performed after kidney transplant, islets were transplanted from a single donor in 11, from two donors in 14, from three donors in 2, and from four donors in 1 case.
Donors were heart-beating cadavers selected for ABO blood compatibility and negative cross-match. HLA type was not considered as a criterion for the donor-recipient matching. Human islets were isolated and purified from pancreata of cadaver donors using an automated procedure as previously described (23), with subsequent modifications (24). In all cases, islets were injected into the liver. In the first seven patients of this series, islets were injected into a branch of a mesenteric vein reached through a small midline laparotomy under general anesthesia; the remainder received islets injected directly into the portal vein, using a percutaneous transhepatic approach, under local anesthesia with continuous portal pressure monitoring. In 25 cases, patients received >6,000 islet equivalents (IEQ)/kg body wt.
Immunosuppression was based on a combination of cyclosporin and either azathioprine (18 cases) or mycophenolate (15 cases), with an additional course of 410 days of ALG or ATG globulin beginning immediately before the transplant procedure. A single shot of 500 mg of methylprednisolone was administered on the day of islet transplantation in 31 cases, and in 27 cases, the patient also received prednisone as part of the chronic immunosuppressive treatment. All transplantation protocols were approved by the institutional ethical committee, and all patients gave informed consent to the procedure.
Solitary islet transplants.
In addition to the 33 patients who received islet and kidney allografts, another 3 patients (aged 22, 37, and 49 years; duration of diabetes, 14, 21, and 19 years, respectively) without diabetic nephropathy received solitary islet allografts; the transplant procedure was the same as in the kidney transplant cases, and the 3 patients received >6,000 IEQ/kg body wt from two donors in two cases and from one donor in the other. Immunosuppression was based on an experimental protocol without cyclosporin, including a single shot of 500 mg of methylprednisolone on the day of islet transplantation, ATG for 9 days in one subject (patient 1) or anti-IL2R antibodies (Simulect) on the day of islet transplantation in the other two patients, with an additional dose on day 4 in one of these; all three patients received mycophenolate and, in addition, vitamin D3 and metformin as adjuvants. The protocol was approved by the institutional ethical committee, and all patients gave informed consent for the procedure.
Posttransplantation monitoring, blood glucose management, and assessment of islet function.
During the first 10 days after transplantation, the blood glucose level was kept at 5.5 to 8.2 mmol/l by continuous intravenous insulin administration and subsequently by intensified subcutaneous insulin therapy (34 injections/day). Insulin doses were progressively tapered according to blood glucose levels and discontinued when fasting and postprandial blood glucose levels were <6.6 and <8.8 mmol/l, respectively (25). Patients were considered insulin-independent when these blood glucose levels were maintained without exogenous insulin for at least 1 week. In insulin-treated transplantation patients, the target level of glycated hemoglobin was <7.0%. An assessment of islet function measurement of fasting serum C-peptide was performed by radioimmunoassay (Diagnostic Products, Los Angeles, CA) daily during the first month, as long as patients remained hospitalized, and at least once 3, 6, and 12 months and every subsequent year after transplantation. The intra- and interassay coefficients of variation of C-peptide measurement were 3 and 5%, respectively.
Measurement of GADA, IA-2A, and antibodies to insulin.
GADA and IA-2A measurements were performed by radiobinding assay with in vitro translated 35S-methioninelabeled GAD65 or IA-2, as previously described (26,27). Results were converted into arbitrary units by extrapolation from a standard curve with a local standard, designated as 100 units. The thresholds for positivity were determined from the 99th centile of control subjects and corresponded to 3 units for GADA and 1 unit for IA-2A. These GADA: and IA-2A assays obtained the and following performances at the First Combined Islet Autoantibody Workshop: GADA: 88% sensitivity, 98% specificity, 100% reproducibility; and IA-2A: 70% sensitivity, 99% specificity, and 100% reproducibility (22). Antibodies to insulin (IAs) were measured using a competitive protein A/G insulin radiobinding microassay (28).
GAD epitope antibody reactivity.
GAD epitope antibody reactivity was measured against GAD65, GAD67, and GAD65/67 chimeras by radiobinding assay as previously described (29). The following GAD constructs were used to measure antibody binding: full-length GAD65 and GAD67, the GAD65195/GAD67102593 (amino-terminal GAD65 epitopes), the GAD671101/GAD6596234/GAD67244593 (amino-central GAD65 epitopes), the GAD671101/GAD65235444/GAD67453593 (carboxy-central GAD65 epitopes), and the GAD671452/GAD65445585 (carboxy-terminal GAD65 epitopes) chimeras. Radiobinding assays were carried out as for GADA.
GADA and IA-2A IgG subclass and isotype.
For GADA and IA-2A IgG subclass (IgG1, IgG2, IgG3, and IgG4) and isotype (IgM, IgA, and IgE) antibody analysis, the protein A/G radiobinding assays were used, substituting the addition of the protein A/G Sepharose with IgG subclass or isotype-specific antibody-bound Sepharose beads, as previously described (30). Results were expressed as SD scores calculated from the mean ± SD of results obtained after subtraction of nonspecific binding to beads coated with anti-rat IgM for control subjects. The mean + 3 SD was used as the threshold for detection.
HLA class I and class II antibodies.
Antibodies to HLA class I and class II antigens were measured by flow cytofluorimetry using a commercial kit (One Lambda, Canoga Park, CA).
Statistical analyses.
Insulin independence was defined as a condition of normoglycemia in the absence of administration of exogenous insulin. The achievement of insulin independence and 95% CI were calculated by Kaplan-Meier analysis, and comparison between groups was performed using the log-rank test. For all statistical methods, the Statistical Package for Social Sciences (SPSS, Chicago, IL) was used.
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RESULTS |
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In three patients who received islet after kidney transplantation (patients A, B, and C), marked rises in GADA were seen within 5 days posttransplantation (Figs. 1 and 2A). These reached a peak 812 days posttransplantation and subsequently declined. GADA were of the IgG1 subclass in all three patients (Fig. 2B) and were directed against the major carboxy central 235444 and carboxy terminal 445585 epitopes and showed no evidence of spreading (Fig. 2C). Patient A also had lesser concomitant rises in IgG2 and IgG3-GADA. No IgG4-GADA were detected in any patients. In patient A, additional IgG1 IA-2 antibody levels rose gradually from 6 months posttransplantation to very high levels almost 2 years posttransplantation. A second rise in GADA directed against the same carboxy central 235444 and carboxy terminal 445585 epitopes was also seen 2 years posttransplantation in this patient. In a fourth patient (D), a rise in GADA was seen 3.2 years posttransplantation. This was of an IgM and not IgG isotype (Fig. 2B) and was directed against the carboxy central 235444 epitope (Fig. 2C). Significant changes in IA titers were not found in these four patients, and in none of these four patients could antibodies to HLA class I or class II molecules be demonstrated posttransplantation (data not shown). All four patients received >6,000 IEQ/kg body wt from a single donor. Three (patients A, B, and C) previously had received a pancreas allograft.
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Increased islet autoimmunity is associated with decreased graft function.
Insulin independence was achieved in 13 of the 33 patients for periods of 148 months. All 13 were in the group of 25 patients who had received >6,000 IEQ/kg body wt. None of the four patients with marked rises in islet autoantibodies achieved insulin independence during follow-up (P = 0.04 vs. remainder receiving >6,000 IEQ/kg body wt) (Fig. 3). Nevertheless, all four had prolonged periods (>4 months) of C-peptide levels of >1 ng/ml, and insulin requirement was reduced by >50% in all four patients, suggesting partial islet function. A marked reduction in C-peptide coincided with the rise in IA-2A and the second rise in GADA in patient A (Fig. 2A).
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DISCUSSION |
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The only unequivocal example of rapid transplant-induced reactivation of ß-cellspecific autoimmunity reported so far in human type 1 diabetes is the recurrence of insulitis and clinical disease weeks after technically successful segmental pancreatic transplantation between identical and nonimmunosuppressed twins (7). In those studies, a recurrent T-cell (mainly CD8+)mediated autoimmunity was not accompanied by a reactivation of humoral autoimmunity as assessed by immunohistochemistry of graft biopsies.
Unlike the twin-to-twin transplant model, our cases are HLA-mismatched and immunosuppressed. Under these conditions, an immediate elevation of GADA after islet transplantation was seen in five patients, four of whom had low GADA titer before transplantation. Evidence that this was a recurrence of a quiescent but already mature autoimmune memory is seen in the rapidity and intensity of the IgG response and the absence of a detectable IgM response to autoantigens in these patients. HLA antibodies were readily detectable in one patient who received solitary islet allografts (patient 1), indicating that the accompanying autoantibody response may have arisen indirectly from islet damage and inflammation associated with acute rejection in this case. Although assays used for the measurement of alloantibodies may be less sensitive than the autoantibody radiobinding assays, we found no evidence of an accompanying alloimmune response at the humoral level in the remaining four patients with immediate GAD antibody responses, suggesting that these patients had a direct and selective recurrence of autoimmunity. T-cell studies were not performed, but it should be noted that previous studies of T-cell response to alloantigen after islet transplantation could also demonstrate autoreactivity without accompanying alloresponses (21). Recently, a rise in GADA was also reported after the transplantation of fetal islets in nonimmunosuppressed patients with type 1 diabetes, further indicating the ability of islets to recall autoimmune memory (31). Of potential interest was the observation that two of the patients who showed immediate GADA rises were identical twins, suggesting genetic influence.
The immediate GADA responses in patients A, B, and C were short-lived. The responses reached peak levels within 2 weeks posttransplantation and subsequently declined at rates not largely divergent from the half-life of circulating IgG1 (32). A short-lived response could be explained by direct presentation of antigen by donor antigen-presenting cells, T-cellindependent B-cell stimulation by soluble antigen, clearance of immunogenic autoantigen, and active immune regulation or immunosuppression. Complete mismatch of genotyped HLA loci was observed in two of the patients with GAD responses, but direct presentation via HLA-DP or cross-presentation is possible in these cases. An alternative scenario is that soluble autoantigen is released from damaged islets and either taken up by recipient antigen-presenting cells relocated in the inflammatory response or reaches immune cell sites containing autoreactive memory lymphocytes, such as pancreatic draining lymph nodes. Resolution of the autoimmune response and stable C-peptide levels after this immediate autoantibody response suggest that it is not associated with an ongoing active immune-mediated ß-cell destruction if immunosuppression is adequate. Indeed, such antibody responses may not necessarily be accompanied by T-cellmediated islet destruction. Inadequate immunosuppression resulting in allorejection (patient 1) or unsuppressed autoimmunity (patient 2) was, however, associated with rapid islet allograft failure.
Although numbers remain small, the ability to achieve insulin independence in patients who received sufficient islet numbers seemed to be markedly decreased in patients with autoantibody elevations posttransplantation. None of these patients became insulin-independent, whereas in the series of patients who received similar islet/kidney transplantation, insulin independence within 12 months posttransplantation was achieved in >60% of patients who did not show elevations in autoantibodies. It may be argued, therefore, that recurrent autoimmunity is a major cause for the decreased function of islet allografts in patients with type 1 diabetes compared with islets autotransplanted (33,34) or transplanted into patients with type 2 diabetes (14) or without diabetes (13). Our data also suggest that some therapies may be better suited for the prevention of this recurrence than others and may therefore be more effective in maintaining islet allograft function in patients with type 1 diabetes. Immediate GAD antibody responses were observed in two of the three patients who received solitary islet transplants; this was significantly more frequent than in patients receiving islet/kidney transplants (P < 0.05). Although there were several differences between these patients and those who received islet/kidney transplants, it is noteworthy that these three patients did not receive cyclosporin or other calcineurin inhibitors. Also noteworthy is that the recently reported successful solitary islet transplantation using a combination of the calcineurin inhibitor FK506, antiIL-2 receptor, and rapamycin did not show rises in islet autoantibodies (4).
This study identified GAD as a key autoantigen in the reexposure of patients with autoimmune diabetes to ß-cells. Responses in all but one case were against the major autoantibody epitopes (29). It is interesting that epitope recognition differed in the one patient who had concurrent strong alloreactivity (patient 1), in whom the dominant response was against the minor NH2-terminal epitope. This anecdotal finding may indicate diversity when autoimmunity accompanies allorejection. Studies of the early response to native ß-cell autoantigens suggest insulin autoantibodies as the first to appear (35). Although IAs were not studied systematically in all patients because of a confounding humoral response to exogenously administered insulin in these patients, we were unable to demonstrate a rise in IA in any of the patients who exhibited rises in GADA, and indeed patients B, C, and 2 had undetectable levels of IA throughout follow-up. Several reasons could be postulated for the relative absence of insulin reactivity, including the possibility that treatment with exogenous insulin induces tolerance. IA-2A responses were rare, but in the one patient in whom IA-2A did rise while on immunosuppressive therapy, the antibody response occurred several months after GADA, was sustained, and was followed by a second rise in GADA and a concomitant fall in C-peptide levels. Late responses to autoantigen while receiving immunosuppression were found in one other patient (patient D). In this case, the response was atypical, with relatively strong IgM antibodies against the major GAD epitope, persisting for >12 months without a switch to IgG, and not accompanied by obvious decreased graft function. The late rise in autoantibodies seen in patient A is similar to what we have previously observed in a minority of patients with type 1 diabetes who underwent pancreas transplantation (19). Patients who underwent pancreas transplantation did not, however, show an immediate rise in islet autoantibodies, suggesting an overall lower capacity to stimulate the memory autoimmune response.
In conclusion, this study demonstrated that autoimmunity after islet transplantation is a clinically relevant occurrence in patients with type 1 diabetes. Its avoidance is likely to be of benefit for islet allograft survival and function, and therapies that can prevent the recurrence of memory autoimmune responses are therefore advocated for successful islet transplantation.
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ACKNOWLEDGMENTS |
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We are indebted to Dr. Elena Bazzigaluppi and Cristina Belloni for help in autoantibody measurements and epitope characterization; Dr. Lucilla Monti for C-peptide measurement; Dr. Elena Benazzi for help in HLA antibody measurements; Dr. Eliana Porta and the Nord Italia Transplant team for providing HLA typing data; Dr. Luciano Adorini and Dr. Alberto Davalli for collaboration in the solitary islet transplant program; and Professor Valerio Di Carlo, Dr. Luca Aldrighetti, Dr. Carlo Socci, and the transplant team for collaboration and support.
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FOOTNOTES |
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Received for publication 21 May 2001 and accepted in revised form 31 July 2001.
ALG, antilymphocyte; ATG, antithymocyte; GADA, antibodies to GAD; IA, antibodies to insulin; IA-2A, antibodies to IA-2; IEQ, islet equivalents.
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REFERENCES |
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