2005
DOI: 10.2337/diabetes.54.suppl_2.s108
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Mechanisms of β-Cell Death in Type 2 Diabetes

Abstract: A decrease in the number of functional insulin-producing ␤-cells contributes to the pathophysiology of type 2 diabetes. Opinions diverge regarding the relative contribution of a decrease in ␤-cell mass versus an intrinsic defect in the secretory machinery. Here we review the evidence that glucose, dyslipidemia, cytokines, leptin, autoimmunity, and some sulfonylureas may contribute to the maladaptation of ␤-cells. With respect to these causal factors, we focus on Fas, the ATP-sensitive K ؉ channel, insulin rece… Show more

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Cited by 401 publications
(319 citation statements)
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References 92 publications
(76 reference statements)
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“…Using both methods, IL-1β and iNOS were immunohistochemically undetectable. Thus, and in contrast to Donath and collaborators [6,8,9], we were unable to find any evidence for hyperglycaemia-induced IL-1β or iNOS immunostaining at the protein level, either in pancreatic beta cells or in immune cells in the Psammomys pancreas [12]. As we analysed islets from gerbils that had been on a high-energy diet both for 1 and for 3 weeks, we can also exclude a transient increase in expression of IL-1β.…”
Section: Discussioncontrasting
confidence: 70%
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“…Using both methods, IL-1β and iNOS were immunohistochemically undetectable. Thus, and in contrast to Donath and collaborators [6,8,9], we were unable to find any evidence for hyperglycaemia-induced IL-1β or iNOS immunostaining at the protein level, either in pancreatic beta cells or in immune cells in the Psammomys pancreas [12]. As we analysed islets from gerbils that had been on a high-energy diet both for 1 and for 3 weeks, we can also exclude a transient increase in expression of IL-1β.…”
Section: Discussioncontrasting
confidence: 70%
“…In these infiltrated type 1 diabetes islets the immune cells showed a dense immunostaining for IL-1β and iNOS [12,16]. To exclude the possibility that low contents of IL-1β and iNOS could have been masked by fixation in the immunohistochemical staining procedure, we used both 4% paraformaldehyde fixed pancreatic tissue [12,16], as used by Donath and collaborators [6], and cryostat sections of unfixed pancreas tissue of Psammomys obesus. Using both methods, IL-1β and iNOS were immunohistochemically undetectable.…”
Section: Discussionmentioning
confidence: 99%
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