Exendin-4 affects calcium signalling predominantly during activation and activity of beta cell networks in acute mouse pancreas tissue slices

Eva Paradiž Leitgeb; Jasmina Kerčmar; Lidija Križančić Bombek; Vilijem Pohorec; Maša Skelin Klemen; Marjan Slak Rupnik; Marko Gosak; Jurij Dolenšek; Andraž Stožer

doi:10.3389/fendo.2023.1315520

Exendin-4 affects calcium signalling predominantly during activation and activity of beta cell networks in acute mouse pancreas tissue slices

Front Endocrinol (Lausanne). 2024 Jan 16:14:1315520. doi: 10.3389/fendo.2023.1315520. eCollection 2023.

Authors

Affiliations

¹ Institute of Physiology, Faculty of Medicine, University of Maribor, Maribor, Slovenia.
² Center for Physiology and Pharmacology, Medical University of Vienna, Vienna, Austria.
³ Alma Mater Europaea-European Center Maribor, Maribor, Slovenia.
⁴ Faculty of Natural Sciences and Mathematics, University of Maribor, Maribor, Slovenia.

Abstract

Tight control of beta cell stimulus-secretion coupling is crucial for maintaining homeostasis of energy-rich nutrients. While glucose serves as a primary regulator of this process, incretins augment beta cell function, partly by enhancing cytosolic [Ca²⁺] dynamics. However, the details of how precisely they affect beta cell recruitment during activation, their active time, and functional connectivity during plateau activity, and how they influence beta cell deactivation remain to be described. Performing functional multicellular Ca²⁺ imaging in acute mouse pancreas tissue slices enabled us to systematically assess the effects of the GLP-1 receptor agonist exendin-4 (Ex-4) simultaneously in many coupled beta cells with high resolution. In otherwise substimulatory glucose, Ex-4 was able to recruit approximately a quarter of beta cells into an active state. Costimulation with Ex-4 and stimulatory glucose shortened the activation delays and accelerated beta cell activation dynamics. More specifically, active time increased faster, and the time required to reach half-maximal activation was effectively halved in the presence of Ex-4. Moreover, the active time and regularity of [Ca²⁺]_IC oscillations increased, especially during the first part of beta cell response. In contrast, subsequent addition of Ex-4 to already active cells did not significantly enhance beta cell activity. Network analyses further confirmed increased connectivity during activation and activity in the presence of Ex-4, with hub cell roles remaining rather stable in both control experiments and experiments with Ex-4. Interestingly, Ex-4 demonstrated a biphasic effect on deactivation, slightly prolonging beta cell activity at physiological concentrations and shortening deactivation delays at supraphysiological concentrations. In sum, costimulation by Ex-4 and glucose increases [Ca²⁺]_IC during beta cell activation and activity, indicating that the effect of incretins may, to an important extent, be explained by enhanced [Ca²⁺]_IC signals. During deactivation, previous incretin stimulation does not critically prolong cellular activity, which corroborates their low risk of hypoglycemia.

Keywords: beta cell; calcium imaging; connectivity; exendin-4; incretin effect; pancreas; tissue slice.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Calcium
Calcium, Dietary
Exenatide / pharmacology
Glucose / pharmacology
Incretins* / pharmacology
Insulin-Secreting Cells*
Mice

Substances

Exenatide
Incretins
Calcium
Glucose
Calcium, Dietary

Grants and funding

The author(s) declare financial support was received for the research, authorship, and/or publication of this article. The work presented in this study was financially supported by the Slovenian Research Agency (research core funding nos. P3-0396 and I0-0029, as well as research projects nos. J3-9289, N3-0170, J3-2525, J3-3077 and N3-0133).