TY - JOUR
T1 - Chronic continuous exenatide infusion does not cause pancreatic inflammation and ductal hyperplasia in non-human primates
AU - Fiorentino, Teresa Vanessa
AU - Owston, Michael
AU - Abrahamian, Gregory
AU - La Rosa, Stefano
AU - Marando, Alessandro
AU - Perego, Carla
AU - Di Cairano, Eliana S.
AU - Finzi, Giovanna
AU - Capella, Carlo
AU - Sessa, Fausto
AU - Casiraghi, Francesca
AU - Paez, Ana
AU - Adivi, Ashwin
AU - Davalli, Alberto
AU - Fiorina, Paolo
AU - Guardado Mendoza, Rodolfo
AU - Comuzzie, Anthony G.
AU - Sharp, Mark
AU - Defronzo, Ralph A.
AU - Halff, Glenn
AU - Dick, Edward J.
AU - Folli, Franco
N1 - Publisher Copyright:
© 2015 American Society for Investigative Pathology Published by Elsevier Inc. All rights reserved.
PY - 2015/1/1
Y1 - 2015/1/1
N2 - In this study, we aimed to evaluate the effects of exenatide (EXE) treatment on exocrine pancreas of nonhuman primates. To this end, 52 baboons (Papio hamadryas) underwent partial pancreatectomy, followed by continuous infusion of EXE or saline (SAL) for 14 weeks. Histological analysis, immunohistochemistry, Computer Assisted Stereology Toolbox morphometry, and immunofluorescence staining were performed at baseline and after treatment. The EXE treatment did not induce pancreatitis, parenchymal or periductal inflammatory cell accumulation, ductal hyperplasia, or dysplastic lesions/pancreatic intraepithelial neoplasia. At study end, Ki-67-positive (proliferating) acinar cell number did not change, compared with baseline, in either group. Ki-67-positive ductal cells increased after EXE treatment (P = 0.04). However, the change in Ki-67-positive ductal cell number did not differ significantly between the EXE and SAL groups (P = 0.13). M-30-positive (apoptotic) acinar and ductal cell number did not change after SAL or EXE treatment. No changes in ductal density and volume were observed after EXE or SAL. Interestingly, by triple-immunofluorescence staining, we detected c-kit (a marker of cell transdifferentiation) positive ductal cells co-expressing insulin in ducts only in the EXE group at study end, suggesting that EXE may promote the differentiation of ductal cells toward a β-cell phenotype. In conclusion, 14 weeks of EXE treatment did not exert any negative effect on exocrine pancreas, by inducing either pancreatic inflammation or hyperplasia/dysplasia in nonhuman primates.
AB - In this study, we aimed to evaluate the effects of exenatide (EXE) treatment on exocrine pancreas of nonhuman primates. To this end, 52 baboons (Papio hamadryas) underwent partial pancreatectomy, followed by continuous infusion of EXE or saline (SAL) for 14 weeks. Histological analysis, immunohistochemistry, Computer Assisted Stereology Toolbox morphometry, and immunofluorescence staining were performed at baseline and after treatment. The EXE treatment did not induce pancreatitis, parenchymal or periductal inflammatory cell accumulation, ductal hyperplasia, or dysplastic lesions/pancreatic intraepithelial neoplasia. At study end, Ki-67-positive (proliferating) acinar cell number did not change, compared with baseline, in either group. Ki-67-positive ductal cells increased after EXE treatment (P = 0.04). However, the change in Ki-67-positive ductal cell number did not differ significantly between the EXE and SAL groups (P = 0.13). M-30-positive (apoptotic) acinar and ductal cell number did not change after SAL or EXE treatment. No changes in ductal density and volume were observed after EXE or SAL. Interestingly, by triple-immunofluorescence staining, we detected c-kit (a marker of cell transdifferentiation) positive ductal cells co-expressing insulin in ducts only in the EXE group at study end, suggesting that EXE may promote the differentiation of ductal cells toward a β-cell phenotype. In conclusion, 14 weeks of EXE treatment did not exert any negative effect on exocrine pancreas, by inducing either pancreatic inflammation or hyperplasia/dysplasia in nonhuman primates.
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U2 - 10.1016/j.ajpath.2014.09.009
DO - 10.1016/j.ajpath.2014.09.009
M3 - Article
C2 - 25447052
AN - SCOPUS:84918828271
SN - 0002-9440
VL - 185
SP - 139
EP - 150
JO - American Journal of Pathology
JF - American Journal of Pathology
IS - 1
ER -