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RIPK3 promotes islet amyloid-induced β-cell loss and glucose intolerance in a humanized mouse model of type 2 diabetes.

Citation
Mukherjee, N., et al. “Ripk3 Promotes Islet Amyloid-Induced Β-Cell Loss And Glucose Intolerance In A Humanized Mouse Model Of Type 2 Diabetes.”. Molecular Metabolism, p. 101877.
Center University of Washington
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Author Noyonika Mukherjee, Christopher J Contreras, Li Lin, Kaitlyn A Colglazier, Egan G Mather, Michael A Kalwat, Nathalie Esser, Steven E Kahn, Andrew T Templin
Keywords diabetes, islet amyloid, RIPK3, β-cell cytotoxicity
Abstract

OBJECTIVE: Aggregation of human islet amyloid polypeptide (hIAPP), a β-cell secretory product, leads to islet amyloid deposition, islet inflammation and β-cell loss in type 2 diabetes (T2D), but the mechanisms that underlie this process are incompletely understood. Receptor interacting protein kinase 3 (RIPK3) is a pro-death signaling molecule that has recently been implicated in amyloid-associated brain pathology and β-cell cytotoxicity. Here, we evaluated the role of RIPK3 in amyloid-induced β-cell loss using a humanized mouse model of T2D that expresses hIAPP and is prone to islet amyloid formation.

METHODS: We quantified amyloid deposition, cell death and caspase 3/7 activity in islets isolated from WT, Ripk3, hIAPP and hIAPP; Ripk3 mice in real time, and evaluated hIAPP-stimulated inflammation in WT and Ripk3 bone marrow derived macrophages (BMDMs) in vitro. We also characterized the role of RIPK3 in glucose stimulated insulin secretion (GSIS) in vitro and in vivo. Finally, we examined the role of RIPK3 in high fat diet (HFD)-induced islet amyloid deposition, β-cell loss and glucose homeostasis in vivo.

RESULTS: We found that amyloid-prone hIAPP mouse islets exhibited increased cell death and caspase 3/7 activity compared to amyloid-free WT islets in vitro, and this was associated with increased RIPK3 expression. hIAPP; Ripk3 islets were protected from amyloid-induced cell death compared to hIAPP islets in vitro, although amyloid deposition and caspase 3/7 activity were not different between genotypes. We observed that macrophages are a source of Ripk3 expression in isolated islets, and that Ripk3 BMDMs were protected from hIAPP-stimulated inflammatory gene expression (Tnf, Il1b, Nos2). Following 52 weeks of HFD feeding, islet amyloid-prone hIAPP mice exhibited impaired glucose tolerance and decreased β-cell area compared to WT mice in vivo, whereas hIAPP; Ripk3 mice were protected from these impairments.

CONCLUSIONS: In conclusion, loss of RIPK3 protects from amyloid-induced inflammation and islet cell death in vitro and amyloid-induced β-cell loss and glucose intolerance in vivo. We propose that therapies targeting RIPK3 may reduce islet inflammation and β-cell loss and improve glucose homeostasis in the pathogenesis of T2D.

Year of Publication
2024
Journal
Molecular metabolism
Volume
80
Number of Pages
101877
Date Published
02/2024
ISSN Number
2212-8778
DOI
10.1016/j.molmet.2024.101877
Alternate Journal
Mol Metab
PMID
38218538
PMCID
PMC10830894
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