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Characterization of Integrin Expression in Islets Isolated from Hamster, Canine, Porcine, and Human Pancreas
Ren Nian Wanga, Steve Paraskevasa, and Lawrence Rosenbergaa Department of Surgery, McGill University, and Montreal General Hospital Research Institute, Montreal, Quebec, Canada
Correspondence to: Lawrence Rosenberg, Dept. of Surgery, Montreal General Hospital Research Inst., 1650 Cedar Ave., Room C9-133, Montreal, Quebec H3G 1A4, Canada.
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Summary |
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The reasons for the failure of clinical islet transplantation remain obscure. Islet isolation, however, exposes the islet to variety of cellular stresses, including disruption of the cell–matrix relationship, an event associated with apoptosis. The cell–matrix relationship is characterized by an interaction between cell surface integrin receptors and matrix molecules of the surrounding basement membrane (BM). The purpose of this study was to characterize integrin expression and the distribution of the peri-insular BM in human, porcine, canine, and hamster pancreas, and after routine islet isolation. Whereas islets in the porcine pancreas do not have a demonstrable BM, islets in the human, canine, and hamster pancreas have an almost continuous BM with very little direct exocrine to endocrine cell–cell contact. After islet isolation, the BM was destroyed, only to be reestablished during the period of culture. In the pancreas of all four species, integrin 
3 was expressed only on islet cells, and integrin 5 was present on islet cells as well as on acinar, centroacinar, and duct cells. Integrin V was detected only in human and canine pancreas. Integrin ß1 was demonstrated only in the human pancreas. In isolated islets, integrin 3, 5, and V expression decreased during the culture period and the intensity of the staining was observed to be coincident with the distribution of the BM. In summary, this is the first report of integrin expression in hamster, canine, porcine, and human islets. After islet isolation, the altered islet cell–matrix relationship is reflected both in the decrease in integrin expression and in the destruction of the peri-insular BM. These profound changes will need to be considered as the process of islet isolation for transplantation is refined. (J Histochem Cytochem 47:499–506, 1999)
Key Words: integrin, basement membrane, islet isolation, islet cell culture, immunocytochemistry
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Introduction |
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TopSummaryIntroductionMaterials and MethodsResultsDiscussionLiterature Cited |
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Islet transplantation has been proposed as an alternative approach to vascularized pancreas transplantation because of the potentially more favorable risk:benefit ratio (
Factors that mediate cell survival include those found in the local microenvironment, such as extracellular matrix (ECM), and those associated with the cell itself, the integrin family of cell surface proteins (
ECM is present in two forms, interstitial matrix and basement membrane (BM). In the pancreas, BM contains laminin, fibronectin, and collagen Types IV and V (
Integrins, expressed on virtually every cell type, are a diverse class of ß heterodimeric receptors through which cells interact with matrix proteins, providing the physical basis for cell adhesion (
In this study we characterized the presence and distribution of the islet BM and the expression of integrins in normal human, porcine, canine, and hamster pancreas. We then compared the findings to those obtained from purified islets after isolation.
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Materials and Methods |
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Sources of Pancreatic Tissue and Isolated Islets
Pancreata from female Syrian Golden hamsters (body weight 85–100 g; n = 3) and mongrel dogs of both sexes (2–4 years old, body weight 10–20 kg; n = 4) were excised under general anesthesia. All procedures were in compliance with Canadian Council for Animal Care standards and were approved by the institutional animal care committee. Pancreatic islets from porcine pancreas were obtained from Boehringer Mannheim Company (Indianapolis, IN) (n = 4) and porcine pancreata (n = 3) were a gift from Dr. Ray C.J. Chiu (Montreal General Hospital, Research institute, Canada). Human pancreata were procured from cadaveric donors (ages 25–60 years; n = 3). Prior consent for research use of these tissues was in accordance with the policies of Quebec–Transplant, the local organ procurement agency.
Chemicals and Antibodies
All chemicals for routine use were obtained from GIBCO (Gibco; Burlington, Ont, Canada). For islet isolation, Liberase and Liberase CI (Boehringer Mannheim) were used for both human and canine pancreata, and collagenase P was used for hamster pancreata (Boehringer Mannheim; Montreal, QC, Canada). For islet cell culture, CMRL1066 supplemented with 10% fetal bovine serum (FBS) was purchased from GIBCO. The following primary antibodies were used for immunocytochemical staining. Monoclonal anti-human integrin 1, 2, 3, ß1, and ß2 antibodies, and polyclonal anti-human integrin 5, 6, and V antibodies were purchased from Chemicon International (Temecula, CA), monoclonal anti-human insulin antibody, polyclonal anti-human glucagon and somatostatin antibodies were obtained from Biogenex (San Ramon, CA), and monoclonal anti-human collagen IV and polyclonal anti-human laminin were purchased from Sigma (St Louis, MO). The optimal concentrations of all primary antibodies were preliminarily determined.
Islet Isolation and Culture
Human pancreata were removed from cadaveric donors after an in situ flush with UW solution (Dupont Pharma; Montreal, QC, Canada). Canine pancreata were removed from anesthetized dogs without the use of an in situ preservation solution. Islets were separated from the surrounding exocrine tissue by enzymatic digestion with Liberase [2.5 mg/ml Liberase in Hanks' balanced salt solution (HBSS)] supplemented with 0.1 mg/ml DNase I (Boehringer Mannheim) at 37C using a semiautomated technique described by
Collagenase P was used for the digestion of hamster pancreata. Purification was carried out by a two-step discontinuous bovine serum albumin (BSA) gradient (Sigma), as previously described (
After overnight incubation, islets were cultured in suspension in CMRL1066 medium supplemented with 10% FBS at 37C in a CO2 incubator (95% air/5% CO2). Porcine islets isolated at the Indianapolis facility were shipped the same day, by overnight courier, in serum-supplemented CMRL1066. Islets selected at random during the digestion period, before and after purification, and then at 2-day intervals for at least 10 days were fixed in 4% paraformaldehyde (PFA) overnight at 4C.
Reticulin Staining
The reticular fibers of the basement membrane were stained by silver impregnation techniques (
Immunocytochemistry
The fixed islet samples from each time point were embedded in 2% agarose according to a standardized protocol of dehydration and paraffin embedding. Sets of 10 serial sections (thickness 4 µm) were cut from the paraffin blocks. Consecutive sections of pancreata or isolated islets were immunostained for integrins, pancreatic hormones, and matrix proteins, using the avidin–biotin (AB) complex method (streptavidin–biotin–horseradish peroxidase complex; Dako, Glostrup, Denmark), as described previously (3 and collagen IV, a pretreatment with either 0.1% trypsin or 0.1% protease was used. The sections were incubated overnight at 4C with the appropriate primary antibodies. Bound antibodies were visualized with the ABC immunoperoxidase system using biotinylated goat anti-mouse and goat anti-rabbit immunoglobulin G (IgG) (Amersham; Poole, UK), and developed with DAB (3,3'-diaminobenzidinetetrahydrochloride; Sigma) as chromogen. For negative controls, the primary antibodies were omitted.
A quantitative evaluation of the number of cells stained was performed. Three randomly selected sections of the first 10 islets from each species were used for counting, and at least 200 acinar cells, duct cells, or isolated islet cells were counted. Data are expressed as mean percentage ± SD.
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Results |
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TopSummaryIntroductionMaterials and MethodsResultsDiscussionLiterature Cited |
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Expression of Basement Membrane Components
The human (Figure 1A), canine (Figure 1D), and hamster (Figure 1G) pancreas each showed the presence of a continuous peri-insular BM. In the porcine pancreas, the BM around islets was either discontinuous or absent (Figure 2A). Within the islet, BM was observed only around capillaries.
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The BM of isolated islets was lost immediately after enzymatic digestion (Figure 1B, Figure 1E, and Figure 1H). After 5 days of culture, the BM was gradually recovered (Figure 1C, Figure 1F, and Figure 1I). Unlike the in situ findings, isolated porcine islets developed a continuous BM within 5 days of culture (Figure 2C).
Immunocytochemical localization of laminin and collagen IV demonstrated that they were components of the peri-insular BM membrane in the pancreas, although staining was of very low or only moderate intensity. Laminin and collagen IV were destroyed during the islet isolation process and were absent immediately after isolation. Immunocytochemical staining, however, returned by Day 5 in culture.
Integrin Expression
The data on integrin expression are summarized in Table 1. The presence of ß2, 1, and 6 was not detected in this study (not shown). Integrin ß1 was strongly positive in human acinar cells, much less so in human islet cells, and negative in all other species of pancreas, except for duct cells of the porcine pancreas. Some isolated canine and porcine islets demonstrated positive staining, but those cells appeared to be associated with ducts. Islet cells from all four species were positive for integrin 3 (Figure 3). Integrin 2 was positive only in porcine islets. Interestingly, the intensity of integrin 2 immunoreactivity in isolated porcine islets appeared to increase from Day 1 to Day 5, but the staining was then lost at Day 9. Integrin 5 was strongly expressed in islet, epithelial, and endothelial cells (Figure 4). In the human and hamster pancreas, staining for integrin 5 was positive in acinar cells (Figure 4A), whereas in the canine and porcine pancreas, positive staining was obtained only for the centroacinar cells. Human and canine pancreas also showed strong staining for integrin V (Figure 5), but negative results were found in porcine and hamster pancreas. There was positive integrin 5 and V staining in isolated islet cells of all four species, which was coincident with the distribution of the BM at Day 5 of culture (Figure 4C and Figure 5C).
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The correlation of integrin expression and pancreatic hormones was determined by immunocytochemical staining in consecutive sections (Figure 3). Cells in isolated islets were positive for integrin 3, 5, and V. The staining was strong the day after islet isolation, but then gradually decreased in intensity during the period of culture (Figure 3C, Figure 4C, and Figure 5C). A similar decrease in staining was also observed for insulin (Figure 3D), glucagon, and somatostatin (data not shown).
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Discussion |
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TopSummaryIntroductionMaterials and MethodsResultsDiscussionLiterature Cited |
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This is the first report of integrin expression on islet cells in the hamster, canine, porcine, and human pancreas. This comparative study, in which islets from four commonly used species were examined before and after islet isolation, is unique and contributes new and important information to the field of islet cell biology. We also show that the peri-insular basement membrane is destroyed during the process of islet isolation.
The only previous report of integrin expression in the human pancreas is that by
The pattern of integrin expression on acinar, duct, and islet cells in the normal pancreas of the four different species was similar but not identical. Moreover, integrin expression also varied among cell types in each species. This observation is interesting from an ontogenetic viewpoint, given that the duct cell is presumed to give rise to both islet and acinar cells (
The role of integrin family members in the regulation of apoptosis has recently been recognized, based, in part, on their capacity to trigger discrete intracellular phosphorylation events and to initiate gene transcription (5 appeared to be reduced in all four species. This finding may be of considerable importance in view of a recent report that linked integrin 5ß1 to support of cell survival through the upregulation of the expression of bcl-2, an important regulatory protein that inhibits apoptosis (
The second morphological finding of the present study was the loss of the peri-insular BM as a result of the isolation process. BM is one of the two forms of extracellular matrix (ECM), the other being the interstitial matrix (
The composition and distribution of pancreatic ECM, and in particular the peri-insular BM, in rat, dog, pig, and human, have been reported by
Although a variable loss of the peri-insular BM has also been reported by other investigators (
ECM also plays an essential role in maintenance of cell differentiation (
In summary, we have characterized the integrin expression and distribution of the peri-insular BM in the human, porcine, canine, and hamster pancreas. We show that, after islet isolation, the BM is destroyed and integrin expression is altered. The resulting cell–matrix disruption could have profound implications for normal islet function and survival, both before and after islet transplantation. These alterations in normal islet structure and function offer a new explanation for the difference in the success of vascularized pancreas grafts compared to isolated islet transplants. If these preliminary findings are confirmed, then new strategies that take advantage of pharmacological manipulation of the cell–matrix relationship may offer a valuable new approach to improving the outcome of islet transplantation.
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Acknowledgments |
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Supported by grants from the Sam Soloman Fund of the Canadian Diabetes Association (CDA) and the Medical Research Council (MRC) of Canada. Dr. Wang is supported by a fellowship from the Canadian Diabetes Association in honor of Herbert L. and Francis Nussbaum. Dr. Rosenberg is a senior clinician–scientist of the Fond de la Recherche Scientifique du Quebec (FRSQ).
We thank D. Agapitos, N. Malek, and A. Torrisi for expert technical assistance.
Received for publication September 4, 1998; accepted November 10, 1998.
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Literature Cited |
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