Pig-to-nonhuman primates pancreatic islet xenotransplantation: an overview.

The therapy of type 1 diabetes is an open challenging problem. The restoration of normoglycemia and insulin independence in immunosuppressed type 1 diabetic recipients of islet allotransplantation has shown the potential of a cell-based diabetes therapy. Even if successful, this approach poses a problem of scarce tissue supply. Xenotransplantation can be the answer to this limited donor availability and, among possible candidate tissues for xenotransplantation, porcine islets are the closest to a future clinical application. Xenotransplantation, with pigs as donors, offers the possibility of using healthy, living, and genetically modified islets from pathogen-free animals available in unlimited number of islets. Several studies in the pig-to-nonhuman primate model demonstrated the feasibility of successful preclinical islet xenotransplantation and have provided insights into the critical events and possible mechanisms of immune recognition and rejection of xenogeneic islet grafts. Particularly promising results in the achievement of prolonged insulin independence were obtained with newly developed, genetically modified pigs islets able to produce immunoregulatory products, using different implantation sites, and new immunotherapeutic strategies. Nonetheless, further efforts are needed to generate additional safety and efficacy data in nonhuman primate models to safely translate these findings into the clinic.

Introduction

In the year 2000 the Edmonton protocol proved that clinical pancreatic islet allotransplantation (alloTx) can be successfully performed to treat type 1 diabetes (T1D) using a steroid-free immunosuppressive regimen [1]. Even if islet replacement could be considered a preferable alternative to insulin therapy in long-term diabetic patients, this therapeutic option will be practically limited by the number of islet donors that will never be sufficient. A possible solution to the problem of tissue supply may be found by investigating the potential of embryonic as well as induced pluripotent stem cells to generate functional insulin-producing cells. Clinical applications await successful testing in animal models. Alternatively, xenotransplantation (xenoTx) of pig islets is currently the most advanced and appealing approach with respect to a possible clinical application [2]. Pigs are the best candidates as human substitutes [3] for several reasons: pig insulin differs from human insulin by just one amino acid; pig islets have lower sensitivity to destruction by recurrent T1D autoimmunity than human islets [4], they do not accumulate amyloid [5], and pig donors can be genetically modified to improve immunomodulation and cytoprotection of pig islets. The experimental results of pig islets to non-human diabetic primates xenoTx are more encouraging than those obtained using pig whole organs, which makes their employment predictable in clinical trials in the next few years [6••]. To make this technique a clinically feasible treatment option we need to generate more convincing preclinical data in the pig-to-primate xenoTx model.

Rationale for Pig Islet XenoTx

Clinical human islet transplantation is emerging as a suitable therapeutic option in T1D patients with uncontrollable glycemic management limited by hypoglycemia unawareness and effective hormonal counter-regulation [7, 8]. Improving the islet processing techniques and introducing new immunomodulatory strategies, we expect to increase the benefit/risk ratio of human islet alloTx. However, the discrepancy between the number of potential islet recipients (ie, patients with T1D with frequent episodes of severe hypoglycemia and those with devastating microvascular diabetes complications) [9] and the number of available donors remains the major crucial issue to be solved, before a broader use of islet transplantation might become a reliable clinical alternative [1].

Pig islet xenoTx currently represents a very promising solution to the limited donor supply [10]. It is important to underline that pig islets might have different additional distinct advantages over human islets for this purpose. First, the quality of prepared pig islets from a pig donor is consistently higher than human islets from a deceased donor (no comorbidity, senescence, brain death, and cold ischemia injury). Second, porcine islet xenografts may be resistant to destruction by recurrent autoimmunity [11]. Third, the risk of infectious disease transmission associated with xenoTx of pancreatic islets is lower than the one observed in human islet alloTx. Furthermore, it is possible to induce donor-specific immunologic hyporesponsiveness pretreating the recipient with donor antigen(s) [12] or using genetically modified pig islets with the overexpression of genes encoding cytoprotective and immunomodulatory molecules [13].

Pig Islet Source, Isolation, and Preparation

In human islet alloTx, an average of 10,000 human islet equivalents (IEQ)/kg of recipient body weight are considered necessary to achieve insulin independence [1]. There is not a consensus for their minimal number in xenoTx [14]. Different groups have proposed islet numbers in the range of 25,000 to 85,000 IEQ/kg of body weight as the requirement to achieve blood glucose normalization in diabetic non-human primates (NHPs) with either neonate or adult pig islets [15•, 16, 17]. Pig fetal or neonatal islet-like clusters are easy to isolate, but require a period of several weeks to mature into glucose-sensing and insulin-producing cells [18]. The immature cells are more resistant to inflammation and ischemia, and endure the engraftment process better than adult islets. The major advantage of the islet transplantation using islets isolated from adult pigs [18] is that graft function can be achieved and monitored immediately after transplantation.

Fetal Islets

The isolation of fetal islets requires relatively easy techniques [19]. Because of the limited amount of exocrine tissue, isolation can be completed just using a simple mixture of exogenous digestive enzymes. Pure islet-like cell clusters (ICCs), also called proislets, can be obtained by simple culture without any technical purification step [19]. However, even if ICCs can normalize blood glucose levels in rodents, several studies have shown that ICCs have poor insulin response to glucose for relatively long periods [20]. Fetal islets are more resistant to ischemic injuries consequent to pancreas procurement, probably due to the relative lack of exocrine tissue retained within ICCs and also for other various characteristics typical of fetal tissue itself [19]. Putative precursor cells, located in the pancreatic ducts or among the ICCs, allow for proliferation after transplantation. Even fetal porcine pancreas fragments have the potential to grow, mature, and function normally when transplanted in a neovascularized site [21].

As previously mentioned, perhaps the major disadvantage of fetal islets is their immaturity, which is associated with delayed functionality: it may take over 2 months before achieving blood glucose normalization in in vivo transplantation experiments [22] and, during this period, there is a poor insulin response to glucose. A second disadvantage is the high expression of α-1,3-galactose (Gal) on the surface of the fetal pig islets—the sugar responsible for hyperacute rejection—which renders those islets more susceptible to rejection than adult pig islets, which, in contrast, express little Gal [23]. Due to the size of the fetal pancreas, only relatively small numbers of ICCs can be obtained, posing an ethical problem on how many fetuses may be necessary to normalize glycemia in diabetic NHPs, let alone humans. Unless better ways to increase the β-cell numbers in vitro become available, it is necessary to use tens of pig fetuses to restore normoglycemia in a patient.

Neonatal Islets

Neonatal pig islets (NPIs) (ie, islets obtained from piglets aged 1–5 days) can be easily procured and isolated by enzymatic digestion [24]; freshly isolated NPIs consist only of 7% endocrine cells, and 11% epithelial cells, whereas exocrine cells represents approximately 74% of the cell pool. During in vitro culture, however, acinar cells undergo apoptosis leading to enrichment of the endocrine component (35% after 9 days of culture) and of the pool of nongranulated epithelial cells [24]. During in vitro culture NPIs, and more specifically β cells, proliferate, as indicated by studies of bromodeoxyuridine (BrdU) incorporation over time [25]. Interestingly, BrdU incorporation shows two higher peaks: initially after isolation and around days 9 to 12, when the cell cluster assume an islet-like morphology [25]. Neonatal pig β cells are more responsive to glucose than fetal pig β cells are [24] but yet not as fully functional as adult cells. The process of maturation of the secretory machinery in neonatal pancreatic islets involves cell-to-cell contact, expression of gap and adherence junctional proteins, and can be accelerated by prolactin [26]. After transplantation in immunodeficient mice the β-cell mass of NPIs increases up to 20 times further, confirming that β cells proliferate and/or that epithelial precursor cells differentiate into β cells [24]. Although insulin secretion is also delayed after transplantation, the maturation period is generally shorter than after fetal islet transplantation.

NPIs express xenoantigens, such as human-serum stained epitopes and IB4 (eg, Gal) epitopes but also other undefined xenoantigens [25], with potential relevance for possible clinical improved treatments. The availability of α-1,3-Gal knockout (GT-KO) pigs as a source of neonatal islet cells can therefore prove useful to attenuate, although not completely abrogate, the problem of hyperacute rejection.

Neonatal islets from 1- to 5-day-old piglets do not differ substantially from 1-month-old piglet islets, showing a similar response to glucose stimulation in vitro during incubation, as well as comparable β-cell mass and function, and can therefore be considered a valid alternative source of islets to adult ones.

The advantage of using neonatal over fetal pig islets consists of the possibility of preventing the sow from undergoing surgery necessary for the fetus harvesting. The number of ICCs isolated from the neonatal pig pancreas is not significantly different than that of fetal ICCs, leaving yet unresolved the problem of supply, thus the need for numerous neonatal pigs to treat an NHP or a patient.

Adult Islets

In contrast to fetal and neonatal islets, adult porcine islets (pig donor age >6 months), due to their mature status, start functioning immediately following isolation and transplantation [27]. Their immunogenicity, despite a low expression of Gal, is highly variable and the technique for their isolation rather difficult. The isolation outcome varies and the effects/damage of isolation can influence their functional performance following transplantation [28]. In adult pigs, the peri-insular matrix is poorly developed; this makes islets susceptible to fragmentation and, consequently, cell breakage during the isolation process. Generally, retired breeders (sows that underwent multiple pregnancies) are preferred as pancreas donors, providing islets with a more compact shape and more resistant to isolation and culture. One adult pig pancreas can provide a sufficient quantity of functional islets to perform xenoTx in one or two NHPs. In contrast to fetal and neonatal islets, β cells from adult pigs are able to respond to hyperglycemia within hours after transplantation. However, several studies reported low insulin secretion even from isolated adult pig islets [18, 29]. The poor insulin secretion of isolated pig islets in vitro, however, does not necessarily imply a lack of function in vivo. Published data show that both isolated neonatal and adult pig islets have been able to correct diabetes in NHPs [15•, 16, 17].

Isolation and Preparation

Pancreata are recovered during a non-survival surgical procedure. Concerning fetuses and neonates pancreatic organs, these are dissected immediately after exsanguination and euthanasia of the piglet. Retained blood in the tissue reduces islet yield, possibly because of inhibition of the collagenolytic activities of the digestive enzymes; for this reason, extensive flushing of the organ before, during, and directly after pancreatectomy is necessary. In adult pigs the pancreas is harvested with a technique similar to the one utilized to harvest the pancreas from deceased organ donors [30]. Islet viability is strongly influenced by warm and cold ischemia time, the isolation process, and the period of storage, but it is difficult to evaluate the exact influence of each factor [26, 31]. Warm ischemia must be kept as minimal as possible to avoid autolysis of the pancreas by proteolytic and lipolytic enzymes [31]. In adult pancreata, intraductal injection with collagenase solution early after pancreas dissection (before its cold preservation) seems to contribute to a higher islet yield; however, collagenase is commonly injected intraductally after cold preservation, just before the isolation begins [31].

Since the introduction of an efficient method for the bulk isolation of pig pancreatic islets by Ricordi et al. [18], most groups use a similar, semiautomatic isolation method also for pig islets. The pancreas, following collagenase injection, is mechanically disrupted in a digestive chamber under controlled temperature [26]. Continuous exposure of the tissue to digestive enzymes is necessary, but it is important to avoid overexposure and damage to the islets. The enzymatic/mechanical digestion is followed by a purification step, thus the separation of the porcine islets from the exocrine tissue. The standard method for islet purification is based on a density-gradient centrifugation, taking advantage of the fact that islets have a lower density than exocrine tissue. Usually a purity of 70% to 90% (islets/whole tissue) is efficiently obtained with various, equally valid, gradient types [31]. For fetal and neonatal islets a culture time of several days is required to facilitate cell re-aggregation and to eliminate the exocrine cells [32]. However, adult pig islets seem to be more fragile than fetal and neonatal ICCs during culture, and loss of islet mass and viability are observed over time. Short-term culture is therefore desirable for adult islets. Typical functional assays to assess the functionality of the isolated islets include in vitro glucose-stimulated insulin release tests, and in vivo function determined by transplanting islets into small diabetic, immunodeficient rodents, such as nonobese diabetic/scid mice [31].

Induction of Diabetes in NHPs

Studies in the pig-to-NHPs islet xenoTx model are needed to provide evidence of safety and efficacy prior to clinical phase 1 and 2 trials. To meet these criteria, preclinical studies should be performed in diabetic NHPs; to obtain these, three different approaches have been used. Spontaneous diabetes, reported in several strains of monkeys including cynomolgus, is usually associated with age, obesity, β-cell degeneration, and extensive amyloid deposition [33]; the availability of these monkeys is limited, and their diabetes could not be considered as a faithful T1D model. Surgical pancreatectomy is a second option, but its execution is difficult and it has associated morbidity problems. This technique is probably the most convincing in the generation of irreversible diabetes, but pancreatectomy needs to be total to avoid potential residual function and possibly β-cell regeneration, and it has the disadvantage of eliminating the endogenous exocrine pancreatic function. The third approach currently used is chemical induction of hyperglycemia through streptozotocin (STZ) [34]. STZ is a compound derived from the bacterium Streptomyces achromogenes with the ability to selectively destroy β cells by DNA damage and nicotinamide adenine dinucleotide depletion [34]. Its intravenous administration successfully achieves killing of β cells and subsequent induction of hyperglycemia, but a discussion on the optimal dose remains an open problem.

A single dose of 30 mg/kg of STZ is not sufficient to induce complete diabetes; although larger doses (100–150 mg/kg) are, they are also associated with harmful side effects [11, 35]. Nephrotoxicity and hepatotoxicity are some of the major disadvantages of high-dose STZ; nonetheless, STZ-induced diabetic monkeys usually remain diabetic and insulin dependent for years, with no significant endogenous C-peptide release even after glucose stimulation and histologic evidence of only a few insulin-staining cells surviving in the pancreas [11]. There is interspecies variation in the effectiveness of STZ also due to the different expression of low-affinity glucose transporter 2 (GLUT-2), which is the receptor through with STZ accesses the β cells but also, to a lower extent, renal and hepatic cells, where this receptor is also expressed. STZ could thus cause hepato- and nephrotoxicity.

There are other important variables that can influence the effectiveness of STZ after intravenous administration, such as the age of the NHPs and an intrinsic sensitivity of the β cells to the drug [36]. Post-STZ hyperglycemia is typically the main indication that a diabetic status has been established; however, C-peptide levels are usually measured for a correct diagnosis. Primate C-peptide levels less than 0.9 ng/mL are considered sufficient to indicate a diabetic status; however, our group has established that diabetes is durable when at least a 75% reduction in C-peptide levels post STZ is recorded [35, 37] and a negative response (lack of C-peptide increase) after a challenge is confirmed [4, 37]. The intravenous glucose tolerance and arginine stimulation tests are the most used challenge tests. The diabetic status of NHPs can be further evaluated by checking the variations in hemoglobin A1c (HbA1c) levels [38]. The effect of STZ on β cells can also be evaluated by histologic examination of pancreatic biopsies, but this requires a surgical procedure and, because some residual insulin immunostaining is always present, it is difficult to quantify the real extent of the damage. The combination of hyperglycemia, insulin dependence, failure to increase C-peptide levels after stimulation, and increase in HbA1c levels allows for a correct diagnosis of STZ-induced diabetes.

Porcine Islets XenoTx Survival in NHPs

Currently, pig islet xenoTx studies in NHPs have been reported by 15 institutions, including transplantation in nondiabetic (Table 1) [19, 23, 39–43] and diabetic recipients (Table 2) [13], [15•, 16, 17, 38, 39, 42, 44–48]. However, prolonged restoration (>3 months) of insulin independence after porcine islet xenoTx in NHPs with spontaneous, chemical, or surgically induced diabetes has only been reported by a few groups [16, 17, 46–48], with xenograft survival exceeding 6 months in even fewer cases. These promising findings indicate that pig islet xenoTx has the potential to cure diabetes in NHPs, and provide a strong rationale to envision clinical future applications.

Table 1

Pig islet cell xenografts in nondiabetic nonhuman primates

Donor pig age	Recipient	Site of transplantation	Immunosuppression, encapsulation, and/or genetic engineering	Maximum graft survival	Reference
Adult	Cyno (n = 8)	Intraportal	None (n = 7) Pretreatment with sCR1 (n = 1)	Post-transplant follow-up for 60 min only	Bennet et al. [23]
Adult	Baboon (n = 2)	Intraportal	Whole-body and thymic irradiation + ATG + EIA + MMF + CsA + CVF + steroids + αCD154	>14 d and <28 d	Buhler et al. [39]
Adult	Baboon (n = 4)	Intraportal	ATG + CsA or LF−195 + MMF + steroids	2 d	Cantarovich et al. [40]
	Cyno (n = 1)
Adult	Group 1	Renal subcapsular and intraportal	Group 1: (cyno) CP + CsA + steroids (rhesus) ATG + α−IL−2R + CsA; steroids	Group 1: 11 d	Rijkelijkhuizen et al. [41]
	Cyno (n = 4)
	Rhesus (n = 4)
	Group 2		Group 2: ATG + α−IL−2R + CsA; steroids	Group 2: 53 d
	Rhesus (n = 4)
Adult	Rhesus (n = 2)	Intraportal	None	> 3 d	Kirchhof et al. [42]
Adult	Cyno (n = 15)	Renal subcapsular	Group 1 (n = 12): encapsulation	Group 1: < 180 d	Dufrane et al. [43]
			Group 2 (n = 2): no encapsulation	Groups 2 & 3: < 7 d
			Group 3 (n = 1): empty capsule
Fetal	Cyno (n = 5)	Renal subcapsular	Group 1: no immunosuppression	Group 1: < 7 d	Mandel [19]
			Group 2: CsA + steroids + CP or BQR	Group 2: > 40 d

Effects of donor pig age, recipient species, and immunotherapeutic strategy on maximum islet xenograft survival.

α-IL-2R anti-interleukin 2 receptor antibody; ATG anti-thymocyte globulin; BQR brequinar; CP cyclophosphamide; CsA cyclosporin A; CVF cobra venom factor; Cyno cynomolgus; EIA extracorporeal immunoadsorption; LF-195 deoxyspergualin analogue; MMF mycophenolate mofetil; sCR1 soluble complement receptor 1; d days.

Table 2

Pig islet cell xenografts in diabetic nonhuman primates

Donor pig age	Recipient	Site of transplantation	Immunosuppression, encapsulation, and/or genetic engineering	Maximum graft survival	Reference
Adult	Baboon (n = 3)	Intraportal	ATG + CsA + Aza	< 2 d	Buhler et al. [39]
Adult	Rhesus (n = 6)	Intraportal	None	> 3 d	Kirchhof et al. [42]
Adult	Cyno (n = 7)	Renal subcapsular	Group 1 (n = 3): wild-type	Group 1: 3 d	Komoda et al. [44]
			Group 2 (n = 4): GnT-III transgenic islets	Group 2: 5 d
Adult	Cyno (n = 12)	Intraportal	Group 1 (n = 3): anti-IL-2R + FTY720 + everolimus-anti-CD154	Group 1: 45 d	Hering et al. [17]
			Group 2 (n = 4): anti-IL-2R + anti-CD154 + FTY720 + everolimus	Group 2: > 187 d
			Group 3 (n = 5): anti-IL-2R + anti-CD154 + FTY720 + everolimus + leflunomide	Group 3: > 158 d
Adult	Rhesus (n = 5)	Intraportal	Anti-CD25 + anti-CD154 + SRL + belatacept	> 76 d	Cardona et al. [45]
Adult	Cyno (n = 10)	Intraportal	Group 1 (n = 2): ATG + Tac + SRL + anti-CD20	Group 1: < 5 d	Rood et al. [13]
			Group 2 (n = 4): ATG + MMF + CVF + anti-CD154	Group 2: Partial function > 58 d
			Group 3 (n = 1): ATG + MMF + DS + anti-CD154	Group 3: 3 d
Adult	Cyno (n = 9)	Intraportal	Group 1 (n = 4) wild-type islets	Group 1: < 46 d	van der Windt et al. [15•]
			Group 2 (n = 5) hCD46 transgenic islets
			Same regimen: ATG + MMF + DS + anti-CD154	Group 2: > 90 d
Adult	Cyno (n = 4)	Subcutaneous with islet monolayer device	Encapsulation	180 d	Gianello and Dufrane [47]
Neonatal	Rhesus (n = 9)	Intraportal	Group 1 (n = 2): no immunosuppression	Group 1: 5 d	Cardona et al. [16]
			Group 2 (n = 7): ): α-IL-2R + anti-CD154 + SRL + belatacept	Group 2: > 260 d
Embryonic	Cyno (n = 3)	Omentum	ATG + anti-CD20 + anti-IL-2R + CTLA4-Ig + FTY720 + everolimus	> 393 d	Hecht et al. [48]

Effects of donor pig age, recipient species, and immunotherapeutic strategy on maximum islet xenograft survival.

α-IL-2R anti-interleukin 2 receptor antibody; ATG anti-thymocyte globulin; Aza azathioprine; CD46 membrane cofactor protein; CsA cyclosporin A; CVF cobra venom factor; Cyno cynomolgus; DS dextran sulphate; GnT-III N-acetylglucosaminyltransferase III; MMF mycophenolate mofetil; SRL sirolimus; Tac tacrolimus; d days.

Long-term insulin independence has been achieved using different strategies, such as: 1) intraportal infusion of wild-type adult and neonatal pigs islet in immunosuppressed diabetic NHPs [15•, 17]; 2) intraportal infusion of islets from adult α-1,3-Gal-deficient animals transgenic for human membrane cofactor protein (CD46) in STZ-diabetic immunosuppressed NHPs [15•, 46]; 3) implantation of embryonic pig pancreatic precursor tissue in STZ-diabetic animals [48]; 4) intraperitoneal transplantation of microencapsulated adult pig islets in nonimmunosuppressed spontaneously diabetic NHPs; and 5) subcutaneous implantation of a monolayer of encapsulated adult islets on a collagen matrix in a nonimmunosuppressed NHP [48, 49••]. The choice of the anatomical site for the implantation of porcine islets in the recipient is a crucial aspect in xenoTx. The current clinical practice is to put islets into the liver, through the portal vein. However, it has now been recognized that this implantation site has several characteristics that can hamper islet engraftment and survival, such as low oxygen tension, an active innate immune system, and induction of a strong inflammatory response (the immediate blood-mediated inflammatory reaction [IBMIR]) [50] and that is therefore associated with considerable early graft loss. When placed under the renal capsule, islets are more protected from immediate destruction, but ischemic injury can be a major problem in this site. Although it is a very successful site in rodent recipients, unfortunately, low or no porcine (graft) C-peptide production has been reported after subcapsular transplantation of islets in NHPs [19, 43].

Porcine islet transplantation in the subcutaneous tissue showed triggering of early inflammatory responses, whereas encapsulated porcine islets in a macrodevice inserted under the skin more successfully controlled diabetes for up to 6 months, even in the absence of immunosuppression [49••]. In a pig alloTx model, it has been shown that when islets are transplanted into the gastric submucosal space, a site where direct contact with the blood stream is delayed, while a rich arterial blood supply for delivery of oxygen and nutrients is maintained, the graft can survive [30]. This site has several characteristics that could favor islet Tx and islet engraftment: a similar embryonic origin as the pancreas, a delayed direct contact with the blood stream while a rich arterial blood supply for delivery of oxygen and nutrients is maintained, and venous drainage of produced insulin into the portal vein blood stream for direct utilization in the liver; a clinical advantage is that transplantation can be performed endoscopically and endoscopic biopsies of the transplanted islets can be carried out.

Immunological Response to Transplanted Islets

The numerous preclinical studies of pig-to-NHP islet xenoTxs have offered important insights into the immune mechanisms and the pathways involved in causing graft damage. The source of pig islets, the microenvironment at the implantation site, and the immunosuppressive therapy significantly affect engraftment and rejection of xenogeneic islets. Pig islet xenografts, where pig islets were isolated from wild-type pigs, can survive for weeks and months in NHP recipients; this indicates that they do not undergo hyperacute rejection as, instead, it occurs in vascularized organ transplantations. In this study neither increases in Gal-specific IgG or IgM circulating antibody levels nor IgG/IgM with associated C9 deposition on islets were observed [17]. When present, the humoral response is mainly characterized by anti-Gal antibody production. Anti-Gal antibodies are natural preformed antibodies directed against pig epitopes in humans and old-world monkeys. However, the Gal epitope is expressed only on 5% of adult islets and on 11% of NPI cells. The use of GT-KO pigs (in association with the human CD46 transgenes) as pig islet donors did not show a substantial protective effect toward early islet loss, suggesting that perhaps antibody binding to non-Gal antigens would likely be a more potent complement activator [16, 17, 23]. In some studies, considerable IgM and moderate-to-strong C3, C5, and C9 deposition were present on islet surface 2 to 3 days after xenoTx [39-41]. Rejection of pig islets in NHPs is probably a result of a combination of innate responses, evidenced by macrophage infiltration and antibody- and complement-mediated injury, followed by a major T-cell response.

More potent immunosuppressive regimens have been used to protect wild-type pig islets from rejection [17], whereas the introduction of transgenic pigs expressing graft-protecting factors has been shown to require a less toxic immunosuppressive protocol [15•].

Regarding pig islet infusion into the portal vein of NHP, this is associated with a considerable early graft loss, regardless of immune rejection. This loss is not just due to antibody-mediated complement activation, but it involves the nonspecific response IBMIR [51]. The mechanisms behind early graft loss remain poorly understood; it is in part the result of tissue factor production [52] and expression in the pancreatic cells. Recent data point to a relatively underestimated role for natural antibodies, complement, and coagulation [53], and platelet binding to the islets surface and leukocyte infiltration have been demonstrated. Triggering of numerous and not mutually exclusive pathologic events after contact of islets with xenogeneic blood is certainly the answer; despite the substantial loss of islet mass (estimated up to 60% to 80%) in the early phase post-transplantation due to IBMIR, data suggest that a sufficient islet mass survive, achieving and maintaining normoglycemia for months in NHP recipients.

Future Directions for Pig Islets XenoTx

Pig islet xenoTx shows important, but not insurmountable limitations, even if recent accomplishments in preclinical pig-to-NHP model hold great promises and may have future implications. Concerning preclinical animal models of islet xenoTx there are some relevant considerations on species-specific glucose metabolism. For instance, pigs and humans share blood glucose levels in similar concentrations, whereas nondiabetic monkeys exhibit lower unstimulated blood glucose. Endogenous C-peptide levels in monkeys are in higher ranges than in humans, and substantially higher than in pigs. When porcine islets engraft in diabetic NHPs they need to adapt to the higher metabolic demands of their recipients. This results in new cutoff parameters of glucose metabolism associated with good graft islet function, intermediate between donor and recipient baselines [37]. We may envision that, based on the metabolic differences between humans and monkeys, humans and pigs, porcine islets would perform more efficiently in humans than in monkeys. Nonetheless, to pursue the use of porcine islets in preclinical as well as clinical models it is necessary to modify the immunosuppressive protocols and to evaluate agents that can be substitutes for anti-CD154 antibodies, critical and effective components of major studies [16, 17, 46] because of their thromboembolic effect. Preliminary studies suggest that antagonistic anti-CD40 monoclonal antibodies could be equally effective when combined with IL-2R antibodies, CD28 antagonists, and sirolimus. Several other immunosuppressant agents are currently under investigation [54].

In the future, immunosuppressive molecules should be selected based on their ability to facilitate negative vaccination systems during the pretransplantation phase by administration of donor antigen to the recipient. The immunological obstacles to xenoTx are significant. A way to reduce the immune response after implantation of pig islet cells in the recipient is the use of transgenic animals. Good results using pigs expressing hCD46 (a human complement-regulatory protein) suggest that protection from complement activation is beneficial to survival of the graft (Fig. 1) [15•]. Furthermore, the inhibition of the T-cell–mediated immune response is a necessary component to prevent rejection following xenoTx. The generation of transgenic pigs producing cytotoxic T lymphocyte-associated antigen (CTLA4) antibodies may also be useful in prolonging graft acceptance [55].

Fig. 1

a, Blood glucose (BG) (solid lines) and exogenous insulin (broken line) profiles in a streptozotocin-diabetic recipient of porcine islet graft (M7273). After porcine xenotransplantation no exogenous insulin is required to maintain BG levels lower than 5 mmol/L (red line) for 1 year. b, In the same animal, primate C-peptide (solid lines) and pig (graft) C-peptide (broken line) levels confirm, respectively, the diabetic status (primate C-peptide) and the positive effect of the pig islet transplantation (Tx) (pig C-peptide) [15•].

A large number of islet product-directed strategies are currently under investigation to allow minimal immunosuppressive treatment. These include pretransplant islet culture in the presence of mitomycin C to upregulate transforming growth factor-β production of islets [56], surface heparinization, pegylation [57] of islets, and transfection with immunorepellant SDF-1. Alginate-encapsulated islets have also been proposed to attenuate antibody and T-cell contact. Optimization of encapsulation protocols may prove to be a successful approach, as promising results indicate [49••, 58]. All these strategies share the central objective of creating an immunoprivileged environment at the islet implantation site. Integrating controlled release of immunoregulatory, cytoprotective, and proangiogenic factors together with the use of bioscaffolds, microspheres and nanoparticles [58, 59] could be key to success.

The potential for porcine endogenous retroviruses (PERV) to harm a recipient of pig tissue has been a concern. These potential risks are now considered to be much less significant since activation of PERV can be prevented by small interfering RNA technology [60]. Nevertheless, regulatory requirements will be necessary to monitor and reduce the risk of contracting xenozoonosis in xenoTx.

Conclusions

Building on the remarkable recent progress in the preclinical pig-to-NHP model, it appears that adult porcine islets have the best potential, from both a logistic and immunologic point of view, to reverse diabetes in NHPs and furthermore in humans. The simultaneous development of suitable sources of genetically modified pigs and more resistant-engineered pig islets, together with the establishment of clinically applicable immunosuppressive regimens, could be translated into tangible benefits for patients with T1D in the very near future. However, questions remain and detailed problems need to be adequately addressed.