Intracellular levels of Na+ and TTX-sensitive Na+ channel current in diabetic rat ventricular cardiomyocytes

Bilginoglu A., KANDİLCİ H. B., TURAN B.

Cardiovascular Toxicology, cilt.13, sa.2, ss.138-147, 2013 (SCI-Expanded) identifier identifier identifier

  • Yayın Türü: Makale / Tam Makale
  • Cilt numarası: 13 Sayı: 2
  • Basım Tarihi: 2013
  • Doi Numarası: 10.1007/s12012-012-9192-9
  • Dergi Adı: Cardiovascular Toxicology
  • Derginin Tarandığı İndeksler: Science Citation Index Expanded (SCI-EXPANDED), Scopus
  • Sayfa Sayıları: ss.138-147
  • Anahtar Kelimeler: Type-I diabetes, Systolic Na+ regulation, Systolic Ca2+ regulation, Systolic H+ regulation, Na+/Ca2+ exchanger, Na+/H+ exchanger, Na+/K+ pump, SODIUM CONCENTRATION, RYANODINE RECEPTOR, PAPILLARY-MUSCLE, CA2+ HOMEOSTASIS, PH REGULATION, OVERLOAD, CARDIOMYOPATHY, INHIBITION, EXCHANGER, ISCHEMIA
  • Lokman Hekim Üniversitesi Adresli: Hayır

Özet

Intracellular Na+ ([Na+] i ) is an important modulator of excitation-contraction coupling via regulating Ca 2+ efflux/influx, and no investigation has been so far performed in diabetic rat heart. Here, we examined whether any change of [Na+] i in paced cardiomyocytes could contribute to functional alterations during diabetes. Slowing down in depolarization phase of the action potential, small but significant decrease in its amplitude with a slight depolarized resting membrane potential was traced in live cardiomyocytes from diabetic rat, being parallel with a decreased TTX-sensitive Na+ channel current (I Na) density. We recorded either [Na+] i or [Ca2+] i by using a fluorescent Na+ indicator (SBFI-AM or Na-Green) or a Ca2+ indicator (Fura 2-AM) in freshly isolated cardiomyocytes. We examined both [Na+] i and [Ca2+] i at rest, and also [Na+] i during pacing with electrical field stimulation in a range of 0.2-2.0 Hz stimulation frequency. In order to test the possible contribution of Na +/H+ exchanger (NHE) to [Na+] i, we examined the free cytoplasmic [H+] i changes from time course of [H+] i recovery in cardiomyocytes loaded with SNARF1-AM by using ammonium prepulse method. Our data showed that [Na +] i in resting cells from either diabetic or control group was not significantly different, whereas the increase in [Na+] i was significantly smaller in paced diabetic cardiomyocytes compared to that of the controls. However, resting [Ca2+] i in diabetic cardiomyocytes was significantly higher than that of the controls. Here, a lower basal pH i in diabetics compared with the controls correlates also with a slightly higher but not significantly different NHE activity and consequently a similar Na+ loading rate at resting state with a leftward shift in pH sensitivity of NHE-dependent H+-flux. NHE protein level remained unchanged, while protein levels of Na +/K+ ATPase and Na+/Ca2+ exchanger were decreased in the diabetic cardiomyocytes. Taken together, the present data indicate that depressed I Na plays an important role in altered electrical activity with less Na+ influx during contraction, and an increased [Ca2+] i load in these cells seems to be independent of [Na+] i . The data with insulin treatment suggest further a recent balance between Na+ influx and efflux proteins associated with the [Na+] i, particularly during diabetes. © 2012 Springer Science+Business Media New York.