| Literature DB >> 35108513 |
Xiao-Qing Dai1, Joan Camunas-Soler2, Linford J B Briant3, Theodore Dos Santos1, Aliya F Spigelman1, Emily M Walker4, Rafael Arrojo E Drigo5, Austin Bautista6, Robert C Jones7, Dana Avrahami8, James Lyon6, Aifang Nie1, Nancy Smith1, Yongneng Zhang9, Janyne Johnson1, Jocelyn E Manning Fox1, Evangelos D Michelakis9, Peter E Light1, Klaus H Kaestner10, Seung K Kim11, Patrik Rorsman3, Roland W Stein5, Stephen R Quake12, Patrick E MacDonald13.
Abstract
In diabetes, glucagon secretion from pancreatic α cells is dysregulated. The underlying mechanisms, and whether dysfunction occurs uniformly among cells, remain unclear. We examined α cells from human donors and mice using electrophysiological, transcriptomic, and computational approaches. Rising glucose suppresses α cell exocytosis by reducing P/Q-type Ca2+ channel activity, and this is disrupted in type 2 diabetes (T2D). Upon high-fat feeding of mice, α cells shift toward a "β cell-like" electrophysiological profile in concert with indications of impaired identity. In human α cells we identified links between cell membrane properties and cell surface signaling receptors, mitochondrial respiratory chain complex assembly, and cell maturation. Cell-type classification using machine learning of electrophysiology data demonstrated a heterogenous loss of "electrophysiologic identity" in α cells from donors with type 2 diabetes. Indeed, a subset of α cells with impaired exocytosis is defined by an enrichment in progenitor and lineage markers and upregulation of an immature transcriptomic phenotype, suggesting important links between α cell maturation state and dysfunction.Entities:
Keywords: alpha cells; diabetes; exocytosis; glucagon; human; islets of Langerhans; modeling; patch-seq
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Year: 2022 PMID: 35108513 PMCID: PMC8852281 DOI: 10.1016/j.cmet.2021.12.021
Source DB: PubMed Journal: Cell Metab ISSN: 1550-4131 Impact factor: 27.287