Abstract
Clinical islet transplantation is currently being explored as a treatment for persons with type 1 diabetes and hypoglycaemia unawareness. Although ‘proof-of-principle’ has been established in recent clinical studies, the procedure suffers from low efficacy. At the time of transplantation, the isolated islets are allowed to embolise the liver after injection in the portal vein, a procedure that is unique in the area of transplantation. A novel view on the engraftment of intraportally transplanted islets is presented that could explain the low efficacy of the procedure.
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Clinical islet transplantation is currently being explored as a treatment for patients with type 1 diabetes who experience recurrent severe hypoglycaemic episodes. The procedure is highly successful, with >80% of the recipients being protected from hypoglycaemic episodes for as much as 5 years after transplantation; most of the recipients then have to resume insulin therapy, but at lower doses than originally [1]. The insulin secretion capacity in these recipients has been estimated to be only ~20–40% of that in a healthy person [2, 3], even when islets are obtained from two to four donors [1, 4], or in some studies as many as eight to 12 donors [5, 6].
The survival of islets from organ procurement to islet isolation and transplantation is depicted in Fig. 1. As in the case of all transplanted organs, there seems to be a gradual loss of islet function over time [1]. Even a minor reduction in beta cell mass in a patient not receiving insulin but with only 20–40% of normal islet mass would lead to the patient requiring exogenous insulin therapy at a low dose. This reduction in endocrine function may depend on the side effects of immunosuppression [7, 8], but is likely to be reinforced by phenomena such as glucose [9] and lipid toxicity [10, 11].
Engraftment of cells and islets embolised in the portal vein
At the time of transplantation, the isolated islets are allowed to embolise the liver after infusion into the portal vein, a procedure that is unique in the area of organ transplantation. Tumours in the gastrointestinal tract are common, and a feared complication is metastasis to the liver, i.e. a situation similar to islet transplantation. This process is multi-step [12], involving: (1) growth of the primary tumour to the extent that a local venous blood vessel is penetrated; (2) seeding of tumour cells into the bloodstream; (3) intraportal entrapment of the tumour cells due to size restraints; (4) adherence of the tumour cells to the vessel wall; (5) penetration through the vessel wall; and finally (6) growth and initiation of the process of revascularisation within the parenchyma of the liver [13]. Only if all these steps are successfully completed can metastasis be established. The efficacy of the engraftment of tumour cells seems to be extremely low. In a rat model of colon cancer metastasis entailing the injection of 5 × 106 tumour aggregates into the portal vein, only few metastases were established; when 0.5 × 106 tumour aggregates were injected, no metastases were formed; and when 107 cell aggregates were injected, three out of five rats died as a result of portal thrombosis [14].
Islets injected into the portal vein should follow the same steps to successfully complete the engraftment process. However, once they have become entrapped in the portal vein because of size restrictions, the isolated islets have only a limited capacity to actively adhere to and penetrate the venular wall.
Entrapment of islets as a result of size restriction in the portal veins may cause a drop in pressure in the portal vein distal to the islet, a change that could markedly alter the regional blood flow. The portal vein and the hepatic artery follow the same branching system throughout their route within the liver (Fig. 2a–c). Both vessels branch repeatedly and empty into the sinusoids (capillaries) of the liver parenchyma. The low pressure formed in the portal vein distal to an entrapped islet could cause a back-flow of blood from small arterial branches. The blood encompassing the islet will subsequently be delivered via portal vein branches into the surrounding sinusoids.
Revascularisation of intraportally transplanted islets
To our knowledge, there are no reports of one vessel growing into the lumen of another vessel. The basement membrane of the endothelial cell lining seems to constitute an insurmountable biological barrier to other vessels. Also, the flow of blood around the entrapped islets prevents the establishment of physiological concentration gradients of relevant growth factors (e.g. fibroblast growth factor [FGF] and vascular endothelial growth factor A [VEGFA]), which are released from the transplanted islets, across the blood vessel wall to stimulate the penetration of new blood vessels into an existing vessel. A single standardised islet equivalent (IEQ), with an average diameter of 150 μm, generally becomes entrapped in a relatively large branch of the portal vein. These branches have a complete vessel wall with its various layers, making it even more unlikely that a proper revascularisation process will be induced. In line with this notion is a recent study from a group in Zurich showing superior functional outcome of small islets compared with large islets in clinical transplantation [15].
The relative success of intraportal islet transplantation in rodents is not consistent with the scenario described above, probably because of the large size of rodent islets compared with the diameter of the portal veins in these animals. Rodent islets are often reported to be even larger than human islets, and if injected in the portal vein they generate large necrotic areas (Fig. 3) due to acute ischemia induced by the sudden obstruction of a large portal branch. This process initiates a cascade of growth factors that stimulate hepatocyte proliferation and re-modulation of the liver parenchyma. Several noteworthy studies in rodents have demonstrated that transplanted islets respond with proliferation and improved engraftment when exposed to growth factors released during liver regeneration [16, 17]. By this process, the islets become incorporated in the newly formed liver parenchyma and induce revascularisation from the hepatic artery [18, 19] within the first week after transplantation (cf. tumour cells actively penetrating the portal venous wall).
Observations in human and non-human primates
In humans [20, 21] or non-human primates [22–30], islets entrapped in the portal veins after intraportal transplantation seem unable to escape the vascular compartment. In fact, we have been unable to find any publication reporting the presence, in non-human primates or humans, of intraportally transplanted islets located in the liver parenchyma. Instead, all the published studies show the islets within the portal vein lumen or incorporated in portal vein walls, several months or even years after transplantation. Also, in humans or non-human primates most islets are recognised by the innate immune response and become covered with fibrin and platelets (i.e. the instant blood-mediated inflammatory reaction [IBMIR] occurs [31]) (Fig. 2d–f). If an islet escapes the other detrimental features of the IBMIR, these platelets may actually facilitate adherence to the vessel wall. The resulting islet-thrombus, like all clots, is at least partially resolved over time, leaving fibrin strands extending between the vessel wall and the islet. Finally, endothelial cell coverage demarcates the islet-thrombus mass from the vessel lumen, allowing the re-canalisation of the lumen of the portal vein, with the blood being able to bypass the site of islet adherence. Through this process, the islet finally becomes incorporated into the vessel wall. It is possible that such islets will become revascularised and receive blood from the vas vasorum. However, this process is slow and cannot be initiated until the original vessel wall has been re-modelled.
Revisiting the rationale for selecting the intraportal route of administration for clinical islet transplantation
The late P. Lacy and his co-authors, working with a rat model of diabetes, concluded that the liver was the optimal site for islet transplantation [32]. However, the other sites evaluated in his comparative study were (1) the intraperitoneal injection of free islets or (2) their subcutaneous transplantation, neither of which support islet survival. Other studies in rodents have clearly shown that transplantation under the kidney capsule produces superior long-term results compared with intraportal transplantation [33], and results in dogs have shown superior long-term outcomes after intrasplenic compared with intraportal islet transplantation [34, 35]. The argument that insulin would be delivered more physiologically after intraportal transplantation has received little support in the literature. It has clearly been demonstrated in experimental studies that intraportally transplanted islets respond to glucose stimulation only when perfused via the hepatic artery; no response is observed after challenge via the portal vein [19]. Similar findings come from the area of tumour biology (cf. delivery of anti-cancer drugs or for interventions designed to occlude the blood supply to the tumour).
Disturbing results have come from a large and well-conducted study of diabetic BB rats receiving intraportal islet transplants (without the need for streptozotocin to induce diabetes or for any immunosuppressive drugs) [36]: in rats with long-term partial function, there was a remarkably high incidence of adenomas, and even hepatocellular carcinoma. The initial stages in the process leading to these pathological conditions were hepatocyte steatosis and glycogen deposits in the vicinity of the transplanted islets, findings that are analogous to those reported in patients from several transplant centres [37, 38]. In addition, islets in the liver are exposed to toxic products from the gastrointestinal tract, including high concentrations of the immunosuppressive drugs being administered [7, 8].
Alternative sites for clinical islet transplantation
An obvious solution to the problems discussed above would be to establish an alternative site for clinical islet transplantation. One of the most attractive sites that has been proposed thus far is the omental pouch [39], into which islets can be transplanted via a laparoscopic procedure. Several groups are already working to address this challenge in non-human primates ([40]; J. Contreras, University of Alabama at Birmingham, personal communication; B. Hering, University of Minnesota, personal communication). An advantage to this route is that insulin would be delivered to the liver via the portal vein. The details of the procedure are currently being explored in several ongoing studies in non-human primates.
A readily available alternative would be to use the same site for islet transplantation that has been employed successfully for decades in the autotransplantation of parathyroid glands [41]. The parathyroid glands are small multiple organs composed of highly metabolic active endocrine cells that produce parathormone, the only hormone that increases the concentration of extracellular Ca2+ in the body. These glands are highly vascularised and continuously sense the Ca2+ concentration in the blood; the release of parathormone is a direct response to changes in Ca2+ concentration. Since the half-life of parathormone in the circulation is about 5 min, there is a need for a stringent and continuous Ca2+-sensing mechanism tied to a stimulus-coupled release of parathormone. The close relationship between the parathyroid glands and the islets is further illustrated by the fact that both organs are affected in the genetic disorder multiple endocrine neoplasia type 1 (MEN 1).
In parathyroid autotransplantation the glands are cut into small pieces and usually implanted between the muscle fibres in the forearm. Once in place, the endocrine cells begin a process of engraftment and revascularisation. The long-term outcome of the procedure is excellent, with almost no side effects [42]. The similarities between the parathyroid glands and pancreatic islets, as well as a few experimental [43, 44] and clinical observations [45–47] suggest that the intramuscular site holds promise for clinical islet transplantation also. If anything, the small size of the islets would facilitate their engraftment. The intramuscular site would also allow transplantation of composite islet–endothelial cell grafts [46, 48] or the application of various matrices carrying growth factors that would facilitate the formation of a new endocrine organ at the new site of implantation. Indeed, in autotransplants, we have successfully transplanted isolated islets of Langerhans intramuscularly into the forearm of a patient undergoing total pancreatectomy because of recurrent life-threatening pancreatitis [49].
In conclusion, recent advances in biotechnology and cell therapy allow creation of an extrapancreatic insulin-producing organ, allowing transplantation to a site outside the liver, e.g. into the omental pouch or intramuscularly. The goal is to establish an extrapancreatic insulin-producing organ that initially is composed of islets, supporting cells and resorbable biomaterials to trigger high-density revascularisation of the islets and a complete integration into surrounding tissues. Several transplant centres are actively working to establish an alternative site for clinical islet transplantation as a first step to make this development possible. Procedures developed will be of immense importance not only for clinical islet transplantation but also for future stem cell therapy.
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Acknowledgements
This study was supported by grants from the Swedish Research Council, the Nordic Insulin Fund, the Ernfors Family Fund, Barn Diabetes Fonden, the Swedish Diabetes Association, the Juvenile Diabetes Foundation International and the National Institutes of Health. The authors would like to thank Vibggor HB and D. Woodroffe for the illustrations.
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Korsgren, O., Lundgren, T., Felldin, M. et al. Optimising islet engraftment is critical for successful clinical islet transplantation. Diabetologia 51, 227–232 (2008). https://doi.org/10.1007/s00125-007-0868-9
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DOI: https://doi.org/10.1007/s00125-007-0868-9