Division of Endocrinology, Diabetes, and Metabolism, University of Vermont, Burlington, Vermont
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ABSTRACT |
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The pancreatic islet ß-cell regulates cellular fuel metabolism and glucose homeostasis through its secretion of insulin. Numerous studies in rodents and humans have shown a tremendous capacity for ß-cell expansion in response to physiological and pathophysiological changes in tissue insulin requirements, i.e., insulin resistance (13). Over the last several years, much has been learned about the molecular regulation of ß-cell development from mice with targeted genetic mutations of transcription factors and cell signaling intermediates. These studies have identified a key role for the insulin/IGF-1 signaling pathway in the adaptive response to insulin resistance, particularly the intermediates insulin receptor substrate-2 (IRS-2) (49), Akt/protein kinase B (PKB) (1013), and the forkhead transcription factor Foxo1 (14) as putative regulators of the gene encoding pancreatic-duodenal homeobox-1 (PDX-1) (15). Although the details are not known about how the ß-cell mass is regulated in response to progressive insulin resistance, a recent study implicates PDX-1 with a key role (16). Although the relative contribution of hyperplasia of existing ß-cells versus new cell development (neogenesis) from pancreatic epithelial precursors of death from apoptosis and hypertrophy of ß-cells is not clear, recent evidence underscores the importance of ß-cell proliferation as a principal mechanism of ß-cell growth and mass maintenance (1618).
We previously investigated ß-cell regeneration following a partial pancreatectomy in normally insulin-sensitive Sprague-Dawley rats (19). We observed that the growth factoractivated kinase Akt, which has been implicated in regulating duct-derived neogenesis and ß-cell proliferation, cell size, differentiation, and survival (1013,2024), was activated in a subset of IRS-2+/PDX-1+ epithelial cells in the common pancreatic duct epithelium (19). This suggested a possible regulatory mechanism whereby enhanced signaling through IRS-2 and Akt may promote duct-derived ß-cell differentiation during islet regeneration. Whether these proteins play a similar role in the ß-cell growth response to insulin resistance is not known.
The Zucker fatty (ZF) (fa/fa) rat is a model of hyperlipidemia, insulin resistance, and obesity because of a mutated leptin receptor gene (2530). These rats physiologically adapt to the insulin resistance through increased ß-cell mass and enhanced ß-cell function such that hyperglycemia is largely prevented. As a result, this model has been used extensively to investigate the biochemical and molecular bases for ß-cell compensation. A study of adult ZF rats has reported a striking increase of ß-cell mass in response to their insulin resistance attributable to enhanced ß-cell hypertrophy and neogenesis (1). This study did not address the mechanisms that initiate or mediate these ß-cell massaugmenting processes. Furthermore, the temporal relationship between the growth of ß-cells and the onset of fully established insulin resistance in these rats has never been determined.
The present study has investigated the time of onset and origin of the cells that mediate ß-cell expansion in ZF rats. We have also screened for potential signaling intermediates. Importantly, we observed that ß-cell mass expansion preceded the onset of obesity and marked insulin resistance. Our results have uncovered potential regulatory mechanisms whereby Akt/PKB signaling promotes enhanced ß-cell mass in an animal that develops severe insulin resistance in adulthood.
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RESEARCH DESIGN AND METHODS |
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For the detection of labile signaling intermediates (phospho-Akt and phospho-BAD) in relation to the transcription factor PDX-1, pancreata from 25-day-old rats (in the postweaning period) (n = 4 each group) were rapidly excised, cut into smaller pieces, and paraformaldehyde fixed for 1 h. They were immediately washed, then equilibrated in 30% sucrose/PBS, embedded in OCT medium (Miles Scientific), and sectioned at 5 µm in a cryostat.
Zucker pup genotyping.
Tail genomic DNA was isolated from Zucker pups using Qiagens DNeasy Tissue Kit and following manufacturers instructions (Qiagen). The introduction of an MspI site by the fa mutation was detected by PCR using a previously described protocol (29). Briefly, PCR primers spanning the fa mutation were designed to amplify a 1.8-kb fragment. PCR was performed in 20 µl containing 100 ng of genomic DNA mixed with 1X Taq buffer (HotStarTaq DNA polymerase buffer; Qiagen), 500 nmol/l of primers (forward: 5'-GTTTGCGTATGGAAGTCACAG-3', reverse: 5'-ACCAGCAGAGATGTATCCGAG-3'), 250 µmol/l dNTPs, and 1 unit of HotStarTaq DNA Polymerase (Qiagen). PCR amplication protocol began with one cycle of 92°C for 15 min, followed by 35 cycles at 92°C for 30 s, 54°C for 1 min, 68°C for 5 min, and finished with an extension step at 72°C for 10 min. A total of 20 µl of PCR product was digested with MspI for 1 h at 37°C and analyzed on a 1% agarose gel. MspI restriction enzyme digestion of the 1.8-kb product from wild-type Zucker pups produced fragments of 1,100 and 700 bp, whereas the fa mutation produced fragments of 950, 700, and 130 bp.
Plasma glucose and insulin measurements.
Fed glucose levels were determined in whole blood using a glucose meter (Freestyle; TheraSense) at 9:00 A.M., and the plasma was subsequently analyzed for insulin employing a rat insulin standard-range enzyme immunoassay kit (Alpco Diagnostics).
ß-Cell mass measurements.
Five-micrometer paraffin sections throughout the entire pancreas were mounted as ribbons on microscope slides to facilitate section counting. At 200-µm intervals in the young rats or 400-µm intervals in the adult rats, sections were rehydrated, blocked, and immunostained with guinea pig anti-insulin IgG (Linco Research) followed by donkey antiguinea pig IgG-alkaline phosphatase (Jackson Immunoresearch). Following development with Vector Red substrate (Vector Laboratories), sections were counterstained with hematoxylin, cleared, and mounted in Permount (Fisher Scientific).
The proportion of islet ß-cell surface area versus surface area of the whole pancreas was determined planimetrically by digitally imaging 1420 (young rats) or 5060 (adult rats) nonoverlapping 3.63-mm2 fields per pancreas on a Zeiss Universal microscope coupled to a Spot RT color charge-coupled device camera (Diagnostics Instruments). Single and small clusters of ß-cells were presumed to be neogenic and were below the threshold for accurate surface area measurements; hence, we measured these cells in different assays (see below). Therefore, only islets >5 cell diameters were included for islet ß-cell surface area measurements. Image files were analyzed using NIH Image version 1.62 with the "Area-Measure" tool, then tabulated (in pixel values) and entered into Microsoft Excel for statistical analyses (significance determined by Students t test where P
0.05 was considered significant). This planimetric method also allowed us to estimate relative islet numbers and compare islet sizes. The possibility of measuring large islets twice was minimized due to the wide sampling interval between sections. ß-Cell mass was estimated for each animal by determining the average ß-cell surface area per animal multiplied by their pancreatic weight.
ß-Cell and duct proliferation.
At least two slides per adult pancreas were immunohistochemically stained for BrdU and insulin. Hydrated tissue sections were subjected to pretreatment with 0.125% trypsin solution (Zymed) for 10 min at 37°C or a 10-min boil in 10 mmol/l citrate buffer, pH 6.0, followed by denaturation in 2N HCl for 20 min. After blocking, sections were incubated overnight in mouse antiBrdU-biotin (1:20; Zymed), washed, and then incubated in Z-avidinhorseradish peroxidase (1:300; Zymed Laboratories) for 1 h. In other experiments examining young ZF ß-cell and duct proliferation, slides were immunostained for the proliferation marker Ki-67 and insulin. This alternative strategy was used due to inconsistencies in BrdU labeling in these young rats that are known to occur in certain situations (31), including paraformaldehyde fixation (32). Since BrdU labeling marks the "S" phase of the cell cycle and Ki-67 marks a cycling cell, these two markers are not interchangeable but are related. Therefore, in young Zucker pups, the values for proliferation were expressed as Ki-67+ ß-cells (%) and were much higher than the values for BrdU incorporation. Hydrated tissue sections were subjected to pretreatment as above and then were incubated overnight in mouse antiKi-67 (1:500; Transduction Laboratories), washed, and then incubated in donkey antimouse-IgG-biotin (Jackson Immunoresearch) followed by streptavidinhorseradish peroxidase (1:300; Zymed). Following development in DAB/H2O2, sections were then stained for insulin as described above and finally counterstained with hematoxylin. The number of Ki-67+ nuclei per 1,0001,500 islet ß-cells or per 300 common duct cells was counted for each animal.
ß-Cell size measurements.
Islet ß-cell size was determined by double immunofluorescence labeling and confocal imaging of insulin and either GLUT2 (Alpha Diagnostics; young rats and 5-week groups) or pan-cadherin (Zymed) (10-week group) to mark ß-cell surface boundaries. A nuclear counterstain was also used in an effort to maximize the number of cells optically sectioned through the middle of the cell. Only those ß-cells with a clearly defined nucleus were measured. Pseudocolored images were merged using Adobe Photoshop, and ß-cell boundaries were outlined and the surface area measured (µm2) using NIH Image.
Islet number and size measurements.
Using the primary data obtained for the ß-cell mass measurements, the relative islet number for each animal (calculated as average number per microscopic field in 400-µm intervals) was determined. With this same primary data set, we also determined the relative sizes, or cross-sectional surface area of individual islets, by converting pixel values to micrometers squared and tabulating for each animal.
Analysis of neogenesis.
Single and small clusters of cells too small to be considered definitive islets and thus not accounted for in the islet mass measurements for the 10-, 20-, 28-, and 31-day and 10-week-old rats were tallied in each group (n = 45 each group). Using the same insulin-stained sections that were used for islet ß-cell mass measurements, the total number of ß-cells as singles and clusters as doublets, triplets, quadruplets, and up to five cell diameters (very small islets) were counted for each animal. Single and clustered ß-cells, regardless of their location, show no signs of replication and therefore were considered neogenic and may aggregate to form new islets.
Multiple-labeling immunofluorescence.
Hydrated sections of pancreas were blocked in 5% normal donkey serum + 1% BSA and then incubated overnight at 4°C in an antibody mixtures of sheep anti-amylase (Biogenesis), guinea pig anti-insulin or C-peptide (Linco), rabbit or guinea pig anti-glucagon (Linco), sheep anti-somatostatin (Cortex), and rabbit or guinea pig antipancreatic polypeptide (Linco). For staining of PDX-1, a rabbit antiserum was used at 1:1,000 (gift from Dr. Chris Wright, Vanderbilt University). Staining for PDX-1 required antigen retrieval as detailed previously. Labeling of phospho-Akt and phospho-BAD required rapidly fixed and processed frozen sections that were stained with antiserum specific for activated Akt using a mouse monoclonal antiphospho-S473Akt (Cell Signaling Technology) or a sheep antiphospho-S473Akt (Upstate), and mouse antiphospho-BAD (Cell Signaling Technology). Polyclonal antibody to Bcl-2 was obtained from Santa Cruz Biotechnology.
Following washing, sections were incubated in a secondary antibody mixture that contained "ML-" grade donkey antispecies-specific IgG conjugated to CY2 (1:300), CY3 (1:2000), or CY5 (1:500; all from Jackson ImmunoResearch), counterstained in 0.5 µg/ml Hoecsht 33258, and mounted in Aqua Polymount (Polysciences). Alternate sections were stained with nonimmune serum from the appropriate species. Controls for secondary antibody specificity were performed as previously detailed (19). Images were acquired using the aforementioned color charge-coupled device camera for conventional epifluorescence or by confocal microscopy.
Immunoblot analyses.
Purified islets were lysed in ice-cold buffer consisting of 50 mmol/l HEPES (pH 7.5), 1% (vol/vol) Nonidet P-40, 2 mmol/l sodium orthovanadate, 100 mmol/l sodium fluoride, 10 mmol/l sodium pyrophosphate, 4 mmol/l EDTA, 1 mmol/l PMSF, and protease inhibitors. The lysate was sonicated, spun, and the protein concentration determined. Protein was separated by SDS-PAGE, transferred to polyvinylidine fluoride membranes, and probed with the relevant antibodies followed by enhanced chemiluminescence detection. Antibodies used to probe for total protein, and activated (phosphorylated) forms of Akt and BAD were obtained from Cell Signaling. Bcl-2 antibody was purchased from Santa Cruz Biotechnology. These were the same antibodies used for the immunostaining experiments.
Analysis of apoptosis for ß-cells in situ and in vitro.
For determination of the apoptotic ß-cells in young rats (1035 days), a modified TUNEL staining protocol was used to fluorescently mark cells with fragmented DNA strands (33). A Dead-End TUNEL Kit (Promega) was used with the initial steps of the protocol followed by the manufacturers suggestions. Modification of the kit (TdT-based end labeling with biotin-UTP as the labeled nucleotide) included incubation with streptavidin-CY3 (1:2,000, Jackson ImmunoResearch) in the final labeling step. Pancreas or islet sections were immunofluorescently stained for insulin (CY2) and finally counterstained with 0.5 µg/ml Hoechst. Verification of TUNEL labeling included staining adjacent slides with rabbit anti-cleaved caspase 3 (R&D Systems) or propidium iodide to label apoptotic nuclei. TUNEL labeling of short-term cultured islets was accomplished by isolating islets from 4.5-week-old rats (ZLC, n = 3; ZF, n = 6; mean islets per rat, 15) using standard methods and incubating in RPMI-1640 + 10% fetal bovine serum at 37°C for 1 h before fixing and processing for frozen sections.
Confocal imaging.
Sections were imaged using a Bio-Rad MRC 1024 scanning confocal head coupled to an upright Olympus BX50 microscope with an Ar-Kr laser utilizing the 488-, 568-, and 647-nm excitation lines (UVM Microscopy Imaging Facility). Images were acquired with the Bio-Rad LaserSharp software merged and formatted on a Power Macintosh running Adobe Photoshop.
Quantitative imaging for Bcl-2 and PDX-1.
Semiquantitative comparisons of Bcl-2 immunofluorescence intensity for islet ß-cells from young pups were accomplished by batch staining and sampling by confocal microscopy for Bcl-2 (CY3), insulin (CY5), and a nuclear counterstain (YO-PRO1; Molecular Probes). The approach allowed us to measure the relative levels of immunoreactive Bcl-2 within individual ß-cells without potential signal from the nonß-cells, an inherent pitfall in whole-islet analyses. Samples were imaged with the confocal microscope using a 60x PlanApo objective lens (N.A. = 1.4) and the 568-, 488-, and 647-nm excitation lines, respectively, of an ArKr laser. For each field, the microscope was focused to maximize the number of cells optically sectioned through the middle of the nucleus. All confocal imaging parameters were identical for each imaged field with four nonoverlapping fields of 170 x 170 µm captured for each animal analyed. Grayscale images (512 x 512 pixels) were transferred to a Power Macintosh running NIH Image for analyses. For each field studied, the Area-Measure tool was used to determine the mean pixel intensity (range 0255 grayscale levels) of Bcl-2 immunofluorescence in randomly picked 20-pixel areas of the perinuclear region of ß-cells. The final corrected intensity values were calculated for each cell after subtraction of the field background fluorescence values.
Using an imaging strategy similar to method above, semiquantitative comparisons of duct nuclear PDX-1 immunofluorescence intensity were obtained from sections of the common pancreatic duct epithelium from 10-week-old ZF and ZLC rats (n = 5 per group).
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RESULTS |
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ß-Cell mass studies of ZF pups.
Before this study, ß-cell mass measurements and growth parameters of ZF rats <5 weeks of age had not been reported. We investigated 10-, 20-, 28-, and 31-day-old ZLC and ZF pups and observed a subtle increase in ß-cell mass of the ZF pups at 20 days of age (1.4-fold over lean littermate controls; P = 0.029) (Fig. 3A). This early ß-cell growth preceded any differences in body weight or insulinemia compared with the ZLC pups (Figs. 3B and C and Table 1). Also, blood glucose levels were not different between the ZF and ZLC pups at any time point (Fig. 3D).
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Survival potential is enhanced in islets from young ZF rats.
The rarity of TUNEL+ ß-cells in tissue sections made cell survival potential determinations between the groups untenable, possibly due to efficient apoptotic clearance mechanisms in Zucker rat pancreata. To circumvent this problem, we performed TUNEL staining on frozen sections of isolated islets from 4.5-week-old rats (ZLC, n = 3; ZF, n = 6) that were then cultured for 1 h before fixation. Accordingly, we found that islets from ZF rats exhibited a significantly reduced fraction (P = 0.009) of TUNEL+ ß-cells compared with the ZLC islets (Fig. 3F).
In the absence of finding any detectable differences in islet ß-cell death in situ, we predicted that the early ß-cell mass expansion in young ZF rats was initially because of enhanced neogenesis. This was supported by our finding of significant increases in the number of small ß-cell clusters at 2028 days of age that, unexpectedly, transiently wane at 31 days (Fig. 4A). Since no differences were seen in the numbers of clusters between the groups at 10 days of age before the ß-cell mass increase (Fig. 4A), there appears to be a temporal correlation with the increased ß-cell mass and increased prevalence of ß-cell clusters from 20 days of age onward. These ß-cells consistently lacked any indications of proliferation (not shown). Upon closer analysis, these clusters were composed of insulin+/PDX-1+ cells that were associated with both ducts and acini (Figs. 4B and C), and may serve as the source of new islets. This was followed by a transient rise in proliferation at 31 days that preceded a substantial ß-cell mass increase at 35 days of age.
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DISCUSSION |
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At the outset of these experiments, we had anticipated that the ß-cell mass of ZF rats would grow in concordance with their progressive insulin resistance and peak when severe insulin resistance is established. We were unable to establish the dominant mechanisms of ß-cell mass expansion in adult ZF rats due to the fact that a steady-state increase in mass was already established by the time of adulthood. In fact, we found that the ß-cell mass of ZF rats was substantially elevated by 5 weeks of age. Although several studies on ZF rats have considered the 10- to 12-week-old age period when insulin resistance is fully established, mild insulin resistance in skeletal muscle has been detected as early as 30 days of age (44). This early period of mild insulin resistance temporally correlates well with our finding of increased ß-cell mass and proliferation. Our investigation of earlier time points has shown that ZF pups are not born with enhanced ß-cell mass; instead, a significant increase was observed just before weaning (at 20 days), which clearly precedes major changes in energy metabolism after 23 days that result in hyperphagia, hyperinsulinemia, and significant weight gain (29). Thus, our results demonstrate an apparent temporal disparity between the ß-cell expansion and ensuing metabolic alterations that merits further study.
We thus focused on ZF rat pups before 5 weeks of age and have demonstrated that the key insulin signaling molecule, Akt, is activated in ducts, acini, and ß-cells. Downstream of IRS-2/PI3-kinase signaling, Akt, and in particular, the Akt-2 isoform (13) appears to be a crucial element in compensatory ß-cell expansion (10,11). Activated (phospho-) Akt staining levels in the duct epithelium were dramatically enhanced in ZF rats in the postweaning period. Furthermore, the most intense PDX-1+ cells consistently costained for phospho-Akt. This observation is significant, since studies of mouse models harboring mutations of genes encoding key insulin signaling intermediates indicate that the link between the insulin signaling pathway and ß-cell mass compensation to insulin resistance is through the stimulation of pdx-1 expression via nuclear exclusion of the forkhead protein transcription factor Foxo1 in ß-cells, an established target of Akt (14,15). Thus, the phospho-Akt+/PDX-1+ cells we have identified in ducts and centroacinar regions of young ZF rats may represent a novel insulin/IGF-responsive progenitor for ß-cell neogenesis, although this remains to be proven.
In addition to the exocrine duct epithelium and centroacinar region, we also observed increased phospho-Akt immunoreactivity in islet ß-cells of ZF rats. In ß-cells, Akt has been proposed to function in mediating proliferation (10,22,24,45), size (10,11), and survival (11,12,21,23,24). Enhanced ß-cell proliferation in ZF rats was limited to a restricted time (31 days of age) that preceded the onset of the largest ß-cell mass increase (3.8-fold at 35 days of age). Since Akt has been ascribed with roles associated with enhanced ß-cell proliferation in vivo (10), future studies are necessary to determine whether it may be serving such a role in the young ZF rat.
The Bcl-2 family member BAD, a well-established substrate of Akt that is inhibited upon phosphorylation, functions as a proapoptotic factor by antagonizing Bcl-2 activity, a related prosurvival protein (46). Both BAD and Bcl-2 are expressed in ß-cells and have been implicated in the coordinate control of ß-cell apoptosis/survival, respectively (46). We detected both increased phospho-BAD and Bcl-2 staining in ß-cells of ZF pups by immunostaining that is consistent with the notion of an enhanced survival potential of ß-cells of ZF rats. Elevated Bcl-2 staining might also represent increased compartmentalization of the protein to cellular membranes. We speculate from these findings in young rats that activated Akt in ß-cells may be targeted to mitochondrial BAD, thus inhibiting its function and promoting ß-cell survival. We failed to detect decreased apoptosis in the ZF rat pancreas based on in situ apoptosis assays, but the rarity of these profiles (<0.1% in all rats and time points), probably from their rapid engulfment from phagocytes or neighboring ß-cells (47), made this approach ineffective to demonstrate changes in apoptosis. However, we quantified apoptosis in ß-cells from 4.5-week-old ZF and ZLC pups using another strategy. Hence, we observed increased survival potential in isolated, short-term cultured islets from young ZF rats based on decreased TUNEL staining. Relatedly, a recent study of pdx-1+/ haploinsufficient mice has ascribed PDX-1 with a pro-survival role in islets (48). Although the mechanisms involved are unresolved, a similar role for PDX-1 could be operating in the pancreas of young ZF rats, although this has yet to be explored.
Akt/PKB has been proposed to regulate ß-cell size (10,11) and may also be playing such a role in the ß-cells of ZF rats. Transgenic overexpression of Akt in mouse ß-cells results not only in a several-fold enhancement in ß-cell mass, but also increased ß-cell size, as well as their heightened survival potential (11). A global knockout of the gene encoding for the ribosomal protein p70S6-kinase 1, a downstream target in the Akt-mTOR pathway, results in glucose intolerance and atrophied ß-cells (49). Collectively, Akt in ß-cells may control size through regulation of p70S6-kinase activation, hence, increasing protein translation and cellular growth. We have determined that ß-cell size, as measured by surface area, is enhanced 33% in 5-week-old ZF rats with over a 3.5-fold enhancement in ß-cell mass. The magnitude of this growth is actually more striking when the volume of the ß-cell is considered. This augmentation in ß-cell size and overall mass is sustained throughout adulthood. Although not studied here, enhanced Akt signaling in adult ZF ß-cells likely impacts their growth through S6-kinase activation.
We have also demonstrated that strongly phospho-Akt immunopositive, but insulin-negative cells in the islet periphery of young Zucker rats also stain intensely for nuclear PDX-1. About 50% of these cells lack a typical islet peptide hormone phenotype, but half are somatostatin+ -cells. A lineal relationship of
- and ß-cells has been reported during both embryonic development (50) as well as during islet regeneration in the adult (42). Hence, these islet-borne PDX-1+/phospho-Akt+/somatostatin+/ cells may represent a ß-cell precursor and might also contribute to the ß-cell mass increase in ZF rats.
In summary, we have presented evidence suggesting that at almost all examined time points, ß-cell differentiation from progenitor cells (neogenesis) is significantly enhanced in ZF rats, as judged by significantly increased numbers of ß-cell clusters and single ß-cells associated with the exocrine compartment. Additional support for ß-cell neogenesis was a significant increase in ductal nuclear PDX-1 staining. Increased ductal PDX-1 expression in regeneration models has been correlated with the acquisition of a "de-differentiated" phase analogous to an embryonic state that, in turn, may lead to new ß-cell development (2). Although these criteria serve as only indirect evidence of neogenesis, we surmise that these cells may migrate and aggregate to form new islets, although this remains to be proven. Unexpectedly, islet ß-cell replication rates between the ZF and control rats differ only at a single time point tested, at 4.5 weeks of age. These results are in contrast to recent reports highlighting ß-cell replication as the principal contributor to ß-cell growth in the adult (1618).
We have established several key features regarding the onset and the nature of early ß-cell mass compensation in young Zucker rat pups and have provided data supporting a central role for Akt kinase. We have identified putative Akt targets that likely function in growth, differentiation, and enhanced survival of ß-cells. Furthermore, we have obtained data suggesting that the survival potential of islet ß-cells is enhanced in young ZF rats. Accordingly, it appears that Akt, a key insulin signaling intermediate, orchestrates both new ß-cell development as well as heightened survival (anti-apoptosis) potential of existing ß-cells. Importantly, we have also localized activated (phospho-) Akt to specific PDX+ cells of ducts, acini, and islets of young ZF rats. Thus, in the leptin-signaling deficient ZF rats, mechanisms of ß-cell mass expansion are clearly in play early in life to insure a sufficient insulin supply for the greatly increased insulin requirements later in adulthood.
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ACKNOWLEDGMENTS |
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Address correspondence and reprint requests to T.L. Jetton, University of Vermont College of Medicine, Department of Medicine, Given C331, Burlington, VT 05405. E-mail: thomas.jetton{at}.uvm.edu
Received for publication October 15, 2004 and accepted in revised form May 4, 2005
Key Words: IRS-2, insulin receptor substrate-2 PDX-1, pancreatic/duodenal homeobox-1 PKB, protein kinase B
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REFERENCES |
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