From the Department of Medical Cell Biology, Biomedical Center, Uppsala University, Uppsala, Sweden
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ABSTRACT |
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INTRODUCTION |
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Endogenous pancreatic islets have a unique glomerular-like angioarchitecture with a high blood perfusion of 57 ml · min-1 · g-1 tissue (3,4). This secures an optimal delivery of oxygen and nutrients to islet cells and ensures an adequate dispersal of secreted hormones. When islets are isolated and cultured before transplantation, the islet endothelium dedifferentiates or degenerates (5). A rapid revascularization is therefore crucial for islet function after transplantation, and this has been shown to occur within 714 days (6,7). However, the extent of revascularization has not been thoroughly studied, and recent experiments on islets transplanted to the renal, splenic, or hepatic subcapsular space have suggested that this process is insufficient to achieve optimal oxygenation of the transplanted islets (810).
The aim of the present study was to compare the vascular density of endogenous pancreatic islets to that of mouse islets syngeneically implanted into different organs. Measurements were performed 1 month posttransplantation, i.e., at a time point when transplanted islets have become fully revascularized. Connective tissue was found to constitute a substantial part of the transplant and to surround individual islets in grafts consisting of several islets (islets implanted to the kidney and spleen). Therefore, the vascular densities in this connective tissue and the transplanted islets of these grafts were determined separately.
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RESEARCH DESIGN AND METHODS |
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Islet isolation, culture, and transplantation.
Pancreatic islets were prepared by collagenase digestion, as previously described (11). The isolated islets were cultured free-floating in groups of 150 for 34 days in 5 ml culture medium consisting of RPMI 1640 (Sigma-Aldrich, St. Louis, MO) supplemented with L-glutamine (Sigma-Aldrich), benzylpenicillin (100 units/ml) (Roche Diagnostics Scandinavia, Bromma, Sweden), streptomycin (0.1 mg/ml; Sigma-Aldrich), and 10% (vol/vol) fetal calf serum (Sigma-Aldrich). The culture medium was changed every second day. After culture, 250350 islets were either packed in a braking pipette and implanted beneath the renal capsule of the left kidney or packed in a butterfly needle (25 gauge) and injected into the splenic parenchyma or portal vein (12). All recipients were anesthetized intraperitoneally with avertin: 0.02 ml/g body wt of a 2.5% (vol/vol) solution consisting of 10 g of 97% (vol/vol) 2,2,2-tribromo-ethanol (Sigma-Aldrich) in 10 ml 2-methyl-2-butanol (Kemila, Stockholm, Sweden).
Preparation of histological sections and staining procedures.
One month posttransplantation, the transplanted animals were killed by cervical dislocation, and the graft-bearing organ was removed. Separate, nontransplanted C57BL/6 mice of the same age were also killed, but only their pancreas was removed. The organs were fixed in 10% (vol/vol) neutral buffered formalin for 24 h, dehydrated in ethanol, and embedded in paraffin. Sections, 5 µm thick, were mounted on glass slides. The slides were pretreated with neuraminidase type X (Sigma-Aldrich), and the microvascular endothelium was stained with the lectin Bandeiraea simplicifolia (BS-1) (Sigma-Aldrich), as previously described (13). Briefly, the sections were incubated with normal goat serum (NGS) (Dakopatts, Glostrup, Denmark) for 1 h at room temperature (20°C). Biotinylated BS-1 was applied to the sections, which were incubated at 4°C overnight. The slides were washed in Tris-buffered saline (TBS) (3 x 5 min) and incubated with StreptABComplex (Dakopatts) for 30 min at 20°C. The slides were washed again, and new fuchsin substrate system (Dakopatts) was applied to the slides and developed. To exclude endogenous alkaline phosphatase activity in the new fuchsin substrate system, 1 mol/l levamisole (Sigma-Aldrich), dissolved in redistilled water, was added before development. The slides were counterstained with hematoxylin. Negative control slides were incubated with NGS (Dakopatts) diluted in TBS containing 0.1% bovine serum albumin (BSA) (dilution 1:20) instead of BS-1.
To find the islet grafts in the liver sections, the latter were also stained with antibodies against insulin. The slides were washed, incubated for 10 min with 8% (wt/vol) hydrogen peroxide in TBS, and washed again. The sections were thereafter incubated with normal swine serum (Dakopatts) diluted 1:20 with TBS containing 0.1% (wt/vol) BSA for 1 h. Primary antibodies against insulin (ICN Biomedicals, Aurora, OH), diluted in TBS containing 0.1% (wt/vol) BSA, were applied to the slides for 1 h. The slides were washed (TBS; 3 x 5 min) and incubated for 30 min with secondary swine anti-rabbit antibody (Dakopatts) diluted 1:100 in TBS. The slides were then washed again. Rabbit peroxidase anti-peroxidase antibody (Dakopatts), diluted 1:100 in TBS, was applied to the slides for 30 min. The slides were washed and developed with Vector SG substrate kit (Immunkemi, Järfälla, Sweden) for 8 min, washed again (TBS; 3 x 5 min), stained with BS-1 as above, and counterstained with the nuclear stain methyl green (Immunkemi) according to the suppliers instructions. Negative control slides were incubated with normal rabbit serum instead of primary antibody and lectin. A protocol similar to that used for the insulin immunostaining of islet grafts in the liver was used to stain pancreatic sections with antibodies against insulin (ICN Biomedicals), glucagon (Novo Nordisk, Copenhagen, Denmark), and somatostatin (Dakopatts). The same pancreatic sections were also stained for BS-1.
Evaluation of vascular density.
In each animal, 12 tissue sections from all parts of the pancreas or islet transplants were randomly chosen and evaluated. The number of blood vessels in endogenous or transplanted islets in each section was counted at a magnification of x600 in a stereo microscope. In the multi-islet grafts implanted into the kidney or spleen, connective tissue surrounded the individual islets in the grafts, and the number of blood vessels in the endocrine and connective tissue parts was counted separately. All connective tissue in the islet grafts was then evaluated; the demarcation of an islet graft was considered to be the parenchyma of the graft-bearing organ. The fractions of endocrine and connective tissue were determined by a direct point-counting method (14,15). For this purpose, the number of intersections overlapping connective tissue and endocrine cells within the islet grafts was counted (at magnification x600). Approximately 12 fields (corresponding to
1,500 intersections) were counted in each islet graft. The areas of the investigated endogenous islets and grafted islets were determined by using a computerized system for morphometry (MOP-Videoplan; Carl Zeiss, Stockholm, Sweden). Vascular density, i.e., the number of blood vessels per measured islet or graft area (mm2), was then calculated.
Implantation of microspheres.
Approximately 300 green cross-linked polystyrene-divinylbenzene microspheres (diameter 200 µm; E-Z Trac, San Diego, CA) were packed in a braking pipette and implanted, using the same technique as for the islets, beneath the renal capsule of separate animals. One month later, the kidneys implanted with microspheres were retrieved and processed similarly to the islet transplants. The number of blood vessels in the connective tissue surrounding the implanted microspheres was determined as in the islet grafts.
Statistical analysis.
All values are given as means ± SE. Multiple comparisons between data were performed by ANOVA (Statview; Abacus Concepts, Berkeley, CA) with correction of P values using the Bonferroni method (16). When only two groups were compared, unpaired or paired Students t test was used. P < 0.05 was considered to be statistically significant for all comparisons.
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RESULTS |
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Vascular density.
The vascular density of the transplanted islets was decreased compared with that of the endogenous pancreatic islets, irrespective of the implantation organ (Fig. 2). Islets transplanted into the spleen had a lower vascular density than islets transplanted beneath the renal capsule or into the liver (Fig. 2). In the connective tissue stroma of grafts implanted into kidney or spleen, the number of capillaries was markedly higher than in the endocrine parts of these grafts (Fig. 3). The density of intra-graft stromal capillaries appeared to be higher in the immediate vicinity of the islets at all three implantation sites.
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DISCUSSION |
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We have recently evaluated various markers for microvascular endothelial cells in tissue samples from rodents and found that the lectin BS-1, which binds to -D-galactosyl residues on endothelial cells (22), enabled us to detect these cells in all tissues examined (13). Of particular interest was the finding that BS-1 consistently stained endothelium in endogenous pancreatic islets and in syngeneically transplanted rat and mouse pancreatic islets irrespective of implantation site. As found previously, the microvessels of the intraportal and renal subcapsular islet grafts were distinctly stained with BS-1 in the present study. The blood vessels within the islet grafts implanted to the spleen were, however, more faintly stained. The reason is unknown, but may reflect revascularization from the unique vascular system that occurs in the spleen. Unknown confounding factors for the staining technique may also be present within the spleen. Despite the more faint staining, the endothelium within the intrasplenically grafted islets and their surrounding connective tissue could be discerned. A further evaluation of the staining specificity of BS-1 was added in the present study, by applying staining with BS-1 and antibodies for insulin, glucagon, or somatostatin in the same pancreatic slides. The rationale for this was that expression of
-galactosyl epitopes on neonatal porcine islet cells has previously been shown (23). No staining of any of these islet endocrine cells with BS-1 was detected, which is consistent with the findings that these epitopes are not expressed in adult pig (24) or adult mouse (22) pancreatic tissue.
We did not quantitatively compare the vascular density in the surface and interior regions of the renal subcapsular grafts, but there were no obvious regional differences in vascular density within these grafts. This result is in line with previous findings of an absence of oxygen-tension gradients in such islet grafts (8). We have previously observed that both blood perfusion and oxygen tension are similar in renal subcapsular islet grafts curing a diabetic animal and in islet grafts implanted to normoglycemic recipients (10). It is therefore anticipated that similar results would have been obtained if cured diabetic recipients had been investigated in the present study rather than normoglycemic recipients. However, this awaits further study.
Besides their main endocrine constituent, islet grafts consist of blood vessels, connective tissue, and, at least initially, a few contaminating exocrine cells. The amount of connective tissue found within the grafts varies between implantation sites, and most likely depends on, at least partially, a foreign body reaction. Both the endocrine and stromal compartments of islet grafts contribute to graft blood flow as measured by, for example, laser-Doppler flowmetry. The oxygenation of the hormone-producing cells, however, depends only on closely adjacent capillaries, i.e., mainly (or only) blood vessels in the endocrine parts of the grafts. We therefore decided to evaluate the endocrine and stromal compartments separately for vascular density. Surprisingly, whereas the vascular density in transplanted islets per se was low, a large number of blood vessels were found in the connective tissue surrounding the renal subcapsular and intrasplenic islets. To elucidate whether this reflected inherent properties of a normal foreign body reaction or a compensation for the low revascularization of the endocrine parts of the grafts, plastic microspheres, rather than islets, were implanted in separate animals. Interestingly, no accumulation of newly formed blood vessels was seen in the foreign body reaction of connective tissue surrounding the implanted microspheres. Thus, an angiogenic response initiated by the cells within the transplanted islets seems to induce a compensatory increase in vascular density in the surrounding connective tissue. Indeed, the predominant location of capillaries in the connective tissue stroma to the immediate vicinity of the endocrine tissue is also consistent with this. To our knowledge, this preferential distribution of graft blood vessels to the connective tissue stroma has not been previously described.
In a previous study, a similar vascular density as in the present study was found in endogenous rat pancreatic islets (25). Because of the use of entirely different techniques to visualize blood vessels, it is difficult to compare our results on vascular density in transplanted islets to previous studies quantitating graft blood vessels (6,20,21). Merchant et al. (20) did not mention whether endocrine and connective tissue parts were evaluated separately, and Menger et al. (6) and Heuser et al. (21) evaluated only single islets implanted into a skinfold chamber preparation.
The islet grafts investigated in the present study contained insulin-producing ß-cells at all implantation sites, as confirmed by immunohistochemistry. Previous studies have also shown that islets in similar numbers normalize the hyperglycemia of alloxan-diabetic recipients (11). Thus, despite the decreased vascular density of transplanted islets, functional activity remains. However, we have previously noted a 75% decrease in insulin content of transplanted islets compared with islets cultured in vitro (10). Although ß-cell death in the immediate posttransplantation period may explain some of the difference, low revascularization with concomitant decreased tissue oxygen tension may also contribute at later stages by suppressing insulin production (26). Indeed, we have previously observed a markedly decreased tissue oxygen tension in transplanted rat islets compared with endogenous islets up to 9 months after implantation (9). This low tissue oxygen tension of islet grafts seems to be independent of implantation site (10) and related to a high degree of nonoxidative glucose metabolism (27). Also, islet graft blood flow, as investigated by means of nonradioactive microspheres or laser Doppler flowmetry, has been found to be decreased compared with endogenous islets (810,28,29). In this context, it should be noted that a laser Doppler flow probe measures whole-blood perfusion, i.e., all moving blood cells within the illuminated tissue. In view of the preferential location of blood vessels to the connective tissue in composite islet grafts, as described in the present study, it may therefore be envisaged that the blood flow within the endocrine parts of the grafts is even lower than previous estimates (4 ml · min- 1 · g-1) (29). Indeed, in experiments using a combination of microspheres and an ultrasonic flow probe, a nutritional islet graft blood perfusion of only
10% of that seen in endogenous islets (57 ml · min-1 · g-1) was observed (8). An islet blood flow more similar to that of endogenous islets was recorded in islets autotransplanted beneath the renal capsule of partially pancreatectomized animals (30,31). However, in the latter experiments, the influence of the partial pancreatectomy has been difficult to assess.
In conclusion, we found a marked decrease in vascular density of transplanted islets compared with that of endogenous islets. In contrast, the connective tissue surrounding the transplanted islets contained a large number of blood vessels. As suggested by previous studies on blood flow, oxygen tension, and metabolism, the low revascularization of transplanted islets may influence islet graft function.
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ACKNOWLEDGMENTS |
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Astrid Nordin and Eva Törnelius are gratefully acknowledged for their skilled technical assistance.
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FOOTNOTES |
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Received for publication 26 October 2001 and accepted in revised form 7 February 2002.
BS-1, Bandeiraea simplicifolia; BSA, bovine serum albumin; NGS, normal goat serum; TBS, Tris-buffered saline.
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REFERENCES |
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