Circulating platelet-neutrophil aggregates characterize the development of type 1 diabetes in humans and NOD mice
Sarah K. Popp, Federica Vecchio, Debra J. Brown, Riho Fukuda, Yuri Suzuki, Yuma Takeda, Rikako Wakamatsu, Mahalakshmi A. Sarma, Jessica Garrett, Anna Giovenzana, Emanuele Bosi, Antony R.A. Lafferty, Karen J. Brown, Elizabeth E. Gardiner, Lucy A. Coupland, Helen E. Thomas, Beng H. Chong, Christopher R. Parish, Manuela Battaglia, Alessandra Petrelli, Charmaine J. Simeonovic
Sarah K. Popp, Federica Vecchio, Debra J. Brown, Riho Fukuda, Yuri Suzuki, Yuma Takeda, Rikako Wakamatsu, Mahalakshmi A. Sarma, Jessica Garrett, Anna Giovenzana, Emanuele Bosi, Antony R.A. Lafferty, Karen J. Brown, Elizabeth E. Gardiner, Lucy A. Coupland, Helen E. Thomas, Beng H. Chong, Christopher R. Parish, Manuela Battaglia, Alessandra Petrelli, Charmaine J. Simeonovic
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Research Article

Circulating platelet-neutrophil aggregates characterize the development of type 1 diabetes in humans and NOD mice

Abstract

Platelet-neutrophil aggregates (PNAs) facilitate neutrophil activation and migration and could underpin the recruitment of neutrophils to the pancreas during type 1 diabetes (T1D) pathogenesis. PNAs, measured by flow cytometry, were significantly elevated in the circulation of autoantibody-positive (Aab+) children and new-onset T1D children, as well as in pre-T1D (at 4 weeks and 10–12 weeks) and T1D-onset NOD mice, compared with relevant controls, and PNAs were characterized by activated P-selectin+ platelets. PNAs were similarly increased in pre-T1D and T1D-onset NOD isolated islets/insulitis, and immunofluorescence staining revealed increased islet-associated neutrophil extracellular trap (NET) products (myeloperoxidase [MPO] and citrullinated histones [CitH3]) in NOD pancreata. In vitro, cell-free histones and NETs induced islet cell damage, which was prevented by the small polyanionic drug methyl cellobiose sulfate (mCBS) that binds to histones and neutralizes their pathological effects. Elevated circulating PNAs could, therefore, act as an innate immune and pathogenic biomarker of T1D autoimmunity. Platelet hyperreactivity within PNAs appears to represent a previously unrecognized hematological abnormality that precedes T1D onset. In summary, PNAs could contribute to the pathogenesis of T1D and potentially function as a pre-T1D diagnostic.

Authors

Sarah K. Popp, Federica Vecchio, Debra J. Brown, Riho Fukuda, Yuri Suzuki, Yuma Takeda, Rikako Wakamatsu, Mahalakshmi A. Sarma, Jessica Garrett, Anna Giovenzana, Emanuele Bosi, Antony R.A. Lafferty, Karen J. Brown, Elizabeth E. Gardiner, Lucy A. Coupland, Helen E. Thomas, Beng H. Chong, Christopher R. Parish, Manuela Battaglia, Alessandra Petrelli, Charmaine J. Simeonovic

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Figure 3

Histone- and NET-induced damage of islets is prevented by mCBS.

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Histone- and NET-induced damage of islets is prevented by mCBS. (A) BALB...
(A) BALB/c mouse islets treated for 2 hours with 800 μg/mL histones and labeled with PI to identify islet cell death (% PI+ islet area) by confocal microscopy and morphometry. Data show mean ± SEM for islets examined in each group. n = 3 experiments/group, n = 24–30 islets analyzed/group, n = 4–7 focal planes at 30 μm intervals examined from a Z stack for each islet, acquired by confocal microscopy. Nonparametric Kruskal-Wallis test with Dunn’s multiple comparisons test. (B) Confocal images of mouse (top panels) and human (bottom panels) islets labeled with PI (red) to identify damaged/dead islet cells and Calcein-AM (green) to identify viable cells. Scale bar: 50 μm. (C) Human islets treated for 18 hours with 800 μg/mL histones + 100–800 μg/mL mCBS. Data show mean percentage of PI+ islet area ± SEM for islets in each group; n = 3 experiments, n = 30 islets/group, n = 4–7 focal planes were examined, as in A. Nonparametric Kruskal-Wallis test with Dunn’s multiple comparisons test. (D) Fluorescence microscopy of PMA- and CI-treated human neutrophils demonstrate release of NETs labeled with SYTOX Green (top panels); merged images confirm that NETs consisted of extracellular DNA (Hoechst 33342; white), MPO (green), and CitH3 (red). Scale bar: 20 μm. (E) Isolated mouse islets cultured with PMA-NETs, CI-NETs, or histones (His) for 17 hours. Data show mean percentage of PI+ islet area ± SEM; n = 3 experiments, n = 28–30 islets analyzed/group, n = 3–5 focal planes were examined as in A. Nonparametric Kruskal-Wallis test with Dunn’s multiple comparisons test. (F) Confocal images of isolated mouse islets treated with PMA-NETs and CI-NETs for 17 hours and labeled with PI (red) and Calcein-AM (green). Scale bar: 25 μm.