Inal in the Pathophysiology of Insulin-Secretion: A “Cardiac” Paradigm in a New Cell Type

Abstract

BACKGROUND: enhancement of the sustained component of the sodium current (INaL) is a major factor contributing to myocardial damage. A beneficial effect of the INaL blocker Ranolazine (RAN) on glycemic control was recently described in the MERLIN-TIMI 36 trial in diabetic patients. However, the mechanism underlying this finding hasn't been elucidated yet.AIM: To characterize INaL in insulin-secreting cells (INS-1E) and evaluate its role in glucose-stimulated insulin secretion (GSIS).METHODS: INaL, identified as the steady-state current blocked by 10 μM RAN (IRAN) or 0.5 μM TTX (ITTX), and its impact on membrane potential (Vm) were assessed by patch clamp. Veratridine (VERA) was used as INaL enhancer. INaL-dependent intracellular Ca2+ changes were detected by Fluo-4AM. To simulate hyperglycemic stress (CHG), INS-1E cells were exposed to 33 mM glucose for 24 hrs. GSIS was measured by HTRF assay.RESULTS: Glucose- and tolbutamide-triggered action potentials were suppressed by TTX, but not by RAN. VERA caused depolarization, countered by INaL blockade. The reversal potentials of ITTX and IRAN were negative to Na+ equilibrium potential, but they approached it when K+-channels were blocked. This revealed INaL coupling to Na+-activated K+ current (IKNa); expression of IKNa channels (Slo2.1/2.2) was confirmed by transcript analysis. INaL blockade blunted cytosolic Ca2+ response to depolarization. CHG enhanced INaL. Whereas acute INaL enhancement (VERA) increased GSIS, chronic one (CHG or VERA) depressed GSIS, which was partially restored by RAN.CONCLUSIONS: INaL is expressed in insulin-secreting cells, is coupled to IKNa , affects Ca2+ signalling and, when enhanced acutely, increases GSIS. However, constitutive INaL enhancement, induced by chronic hyperglycemic stress, and leads to GSIS depression instead. Overall, chronic INaL enhancement may represent a mechanism of damage progression common to myocardial and insulin-secreting cells.