Islet Transplantation in Type 1 Diabetic Recipients of Kidney Transplants
Description
This trial is designed to replicate the protocol currently being tested by the Immune Tolerance Network (ITN) in a population of patients that have been previously transplanted (recipients of functioning renal allografts) and are therefore immunosuppressed.
The data will be generated using substantially identical techniques for islet preparation, re transplantation with additional islets to meet the minimum islet cell mass, and an identical steroid-free post-transplant regimen utilizing sirolimus, low dose tacrolimus, and daclizumab.
3.1. Primary and secondary endpoints and additional measures
Study efficacy endpoints and additional measures are described in the following subsections. Measures relating to the islet preparation quality (Section 3.1.3) and other variables relating to key cellular and genetic markers (Section 3.1.4) followed during the study are not considered clinical outcome variables. Details describing requirements for efficacy testing are found in Section 6.1. Safety measures are described in Section 7.
3.1.1. Primary endpoint
The primary endpoint for this study is independence from insulin injections with adequate control of blood glucose in subjects with Type 1 diabetes at one year post final transplant. Subjects will be considered as a success when at the one year assessment they are not using insulin, they have a HbA1c <6.5% and they achieve fasting glucose levels not exceeding 7.8 mmol/L (140 mg/dL) more than three times in a week (using the morning fasting glucose level), and not exceeding two hour post-prandial (using any post meal glucose level) values of 10 mmol/L (180 mg/dL) more than four times in a week. A subject will still be considered a success if an intercurrent illness or other event (e.g., high tacrolimus level) causes a participant to require insulin use for a period not exceeding a total of 14 days, and assessment after this event demonstrates insulin independence and adequate glucose control as defined above. This assessment must be completed no later than two weeks after the scheduled one year assessment.
3.1.2. Secondary parameters
Secondary parameters that support the primary goal of the investigation will be assessed at generally the same intervals as the primary endpoint, with some taken more or less frequently as indicated in detail in Sections 5.2 and 6.1. Additional clinical measurements are also taken during the study that are not considered endpoints for formal analyses, but are to be carefully followed as a part of the study. The schedule for these additional elements is listed in Sections 5.2, 6.2 and 7.2. The secondary variables include the following measures:
Basal C-peptide levels
HbA1C levels
Glucose tolerance
C-peptide response to arginine
MAGE improvement
Mixed Meal Test
Durability of insulin independence and adequate blood glucose control
3.1.3. Islet quality endpoints
Islet cell preparations for each transplant will be assessed using the following elements:
Islet yield per isolation used for clinical transplantation, expressed as i) total islet equivalents and ii) islet equivalents per kg recipient body weight.
Islet viability, as assessed by a fluorescent dye inclusion/exclusion assay to assess metabolic activity and membrane integrity.
In vitro islet responsiveness to glucose challenge, as measured by 2-hour static incubation following 12-24 hour culture at 37º C in CMRL 1066 (10% FCS, 25 mmol HEPES). A stimulation index, a ratio of insulin secretion during high glucose over insulin secretion during low basal secretion is calculated as an index of islet function.
Islet cell immunohistochemical composition and purity assessment, (as determined by JDRF Center for Islet Transplantation at Harvard Medical School - Islet Morphology Core Laboratory)
Evidence of no microbial contamination, as documented by a negative Gram stain of the islet preparation immediately pre-transplant, and by negative microbial cultures reported after at least 5 days incubation for aerobes, anaerobes, fungi.
Evidence of a low endotoxin content of the final islet preparation.
3.1.4. Cellular and genetic markers
Samples will be collected before and after transplant for immunologic studies to be processed in the laboratories of Dr. Terry Strom at the Beth Israel Deaconess Medical Center and Dr. Mohamed Sayegh at the Brigham and Women's Hospital.
These include:
Alteration in autoimmune markers for GAD65, ICA512, and mIAA, comparing blood samples drawn pre-transplant and 3, 6, 9, 12, 24 and 36 months after final transplant.
Changes in autoantibody and other immune markers comparing blood samples drawn pre-transplant and 3, 6, 12, 24, and 36 months after final transplant
Samples will also be taken for future laboratory and genetic studies comparing blood samples drawn pre-transplant and usually 3, 6, and 12 months after final transplant.
3.2. Description of trial design and schematic diagram of procedures and stages
Because this is an open-label, single-arm study, a schematic diagram of the design is omitted for simplicity. For a general description of the trial design, please refer to Section 2. A tabular listing of visit schedules and tests is found in Appendix 1.
3.3. Measures to minimize bias
This study is an open-label feasibility study with definitive clinical endpoints of insulin independence, blood glucose and C peptide production as measures of procedural success. As donor islets become available the appropriate ABO compatible blood types will be matched to eligible participants. Clinical investigators are not masked to treatment assignment or follow up assessment information for this pilot study.
3.4. Description of trial treatments and dosage regimen & labeling
Each islet cell transplantation procedure under this protocol is derived from an individual donor pancreas, processed for immediate transplantation. All containers and components are appropriately labeled during preparation. Each final islet preparation released for use is labeled to indicate its identity and date of preparation. Records regarding donor identity will be kept in a coded manner for quality control purposes and will be kept absolutely confidential in accordance with standard procedures.
3.4.1. Islet Infusion(s)
A target total of > 10,000 IE/kg recipient body weight will be infused via a percutaneous transhepatic catheter inserted into the portal vein (see Section 1.4.2). This will in all likelihood require more than one islet infusion to achieve this goal. The first infusion must contain at least 5,000 IE/kg recipient body weight. In the event that a subject does not achieve insulin-independence with normoglycemia after two fresh islet infusions, a third transplant may be considered as described in Section 5.1.
3.4.2. Immunosuppressive Therapy
Beginning with the initial transplant, a immunosuppressive regimen will be administered to all subjects. Subjects will receive initial doses of daclizumab, sirolimus, and low dose tacrolimus according to the following schedule.
3.4.2.1. Daclizumab regimen
Daclizumab will be administered at a dose of 1 mg/kg peripheral IV given immediately pre-transplant, and at 2, 4, 6, and 8 weeks after transplant, for a total of 5 doses (over 8 weeks). If a subsequent islet infusion is required beyond this induction period, then a further 5 dose course of daclizumab will be given according to the same schedule. If the second (or third) transplant occurs and no daclizumab was given in the preceding 7 days, then the dosing regimen will begin at the time of transplant. If daclizumab has been administered within the past 7 days, then the dose at transplant is omitted, and the first dose given 2 weeks post transplant.
3.4.2.2. Sirolimus regimen
All patients enrolled in this trial will already be on Sirolimus therapy. If needed, the dose will be increased to 0.1 mg/kg/day PO and adjusted to the target range of 12-15 ng/ml for the 3 months following the most recent islet infusion. After three months following last transplant, the target whole blood level will be lowered to 7-10ng/mL.
3.4.2.3. Tacrolimus regimen
All patients enrolled in this trial will already be on Tacrolimus therapy. As soon as trough levels are available, the dose will be adjusted to the target range of 3-6 ng/ml throughout the study.
