| Literature DB >> 35998625 |
Lianhe Chu1, Michishige Terasaki1, Charlotte L Mattsson1, Romain Teinturier1, Jérémie Charbord1, Ercument Dirice2, Ka-Cheuk Liu1, Michael G Miskelly3, Qiao Zhou4, Nils Wierup3, Rohit N Kulkarni5, Olov Andersson6.
Abstract
Analogs of the incretin hormones Gip and Glp-1 are used to treat type 2 diabetes and obesity. Findings in experimental models suggest that manipulating several hormones simultaneously may be more effective. To identify small molecules that increase the number of incretin-expressing cells, we established a high-throughput in vivo chemical screen by using the gip promoter to drive the expression of luciferase in zebrafish. All hits increased the numbers of neurogenin 3-expressing enteroendocrine progenitors, Gip-expressing K-cells, and Glp-1-expressing L-cells. One of the hits, a dual-specificity tyrosine phosphorylation-regulated kinase (DYRK) inhibitor, additionally decreased glucose levels in both larval and juvenile fish. Knock-down experiments indicated that nfatc4, a downstream mediator of DYRKs, regulates incretin+ cell number in zebrafish, and that Dyrk1b regulates Glp-1 expression in an enteroendocrine cell line. DYRK inhibition also increased the number of incretin-expressing cells in diabetic mice, suggesting a conserved reinforcement of the enteroendocrine system, with possible implications for diabetes.Entities:
Keywords: DYRK; GIP; GLP-1; chemical screen; diabetes; enteroendocrine cells; incretin hormones; mouse; zebrafish
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Year: 2022 PMID: 35998625 PMCID: PMC9557248 DOI: 10.1016/j.chembiol.2022.08.001
Source DB: PubMed Journal: Cell Chem Biol ISSN: 2451-9448 Impact factor: 9.039