α Cell dysfunction in islets from nondiabetic, glutamic acid decarboxylase autoantibody–positive individuals
Nicolai M. Doliba, … , Doris A. Stoffers, for the HPAP Consortium
Nicolai M. Doliba, … , Doris A. Stoffers, for the HPAP Consortium
Published June 1, 2022
Citation Information: J Clin Invest. 2022;132(11):e156243. https://doi.org/10.1172/JCI156243.
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α Cell dysfunction in islets from nondiabetic, glutamic acid decarboxylase autoantibody–positive individuals

Abstract

BACKGROUND Multiple islet autoantibodies (AAbs) predict the development of type 1 diabetes (T1D) and hyperglycemia within 10 years. By contrast, T1D develops in only approximately 15% of individuals who are positive for single AAbs (generally against glutamic acid decarboxylase [GADA]); hence, the single GADA+ state may represent an early stage of T1D.METHODS Here, we functionally, histologically, and molecularly phenotyped human islets from nondiabetic GADA+ and T1D donors.RESULTS Similar to the few remaining β cells in the T1D islets, GADA+ donor islets demonstrated a preserved insulin secretory response. By contrast, α cell glucagon secretion was dysregulated in both GADA+ and T1D islets, with impaired glucose suppression of glucagon secretion. Single-cell RNA-Seq of GADA+ α cells revealed distinct abnormalities in glycolysis and oxidative phosphorylation pathways and a marked downregulation of cAMP-dependent protein kinase inhibitor β (PKIB), providing a molecular basis for the loss of glucose suppression and the increased effect of 3-isobutyl-1-methylxanthine (IBMX) observed in GADA+ donor islets.CONCLUSION We found that α cell dysfunction was present during the early stages of islet autoimmunity at a time when β cell mass was still normal, raising important questions about the role of early α cell dysfunction in the progression of T1D.FUNDING This work was supported by grants from the NIH (3UC4DK112217-01S1, U01DK123594-02, UC4DK112217, UC4DK112232, U01DK123716, and P30 DK019525) and the Vanderbilt Diabetes Research and Training Center (DK20593).

Authors

Nicolai M. Doliba, Andrea V. Rozo, Jeffrey Roman, Wei Qin, Daniel Traum, Long Gao, Jinping Liu, Elisabetta Manduchi, Chengyang Liu, Maria L. Golson, Golnaz Vahedi, Ali Naji, Franz M. Matschinsky, Mark A. Atkinson, Alvin C. Powers, Marcela Brissova, Klaus H. Kaestner, Doris A. Stoffers, for the HPAP Consortium

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Figure 2

Insulin and glucagon secretion in islets from healthy and T1D donors.

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Insulin and glucagon secretion in islets from healthy and T1D donors. (A...
(A) The dynamics of insulin secretion in response to different stimuli. (B) Total insulin secretion during 16 mM glucose stimulation. (C) Total insulin secretion during IBMX potentiation. The basal and maximal insulin secretion in T1D islets was 1/60 that of normal islets. Notably, T1D islets had similar insulin response patterns at low glucose, high glucose, and with IBMX treatment compared with control islets. (D) Glucagon secretion profiles. (E) Magnified view of a selected section (53–100 min) of the experiment presented in D to highlight the difference in glucose suppression of glucagon secretion between normal and T1D islets. (F) Total glucagon secretion during AAM stimulation. (G) Total glucagon secretion during IBMX potentiation. *P < 0.05 and ***P < 0.001. Ctrl, control.