Fast Ca2+-dependent inactivation of the store operated Ca2+ current (ISOC) in liver cells: a role for calmodulin
Date
2004
Authors
Litjens, T.
Harland, M.
Roberts, M.
Barritt, G.
Rychkov, G.
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Journal article
Citation
Journal of Physiology, 2004; 558(1):85-97
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Tom Litjens, M. Lyn Harland, Michael L. Roberts, Gergory J. Barritt and Grigori Y. Rychkov
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Abstract
Store-operated Ca ²+ channels (SOCs) provide a major pathway for Ca ²+ entry in non-excitable cells. SOCs in immortalized liver cells are highly selective for Ca ²+ over other cations and are similar to well studied Ca ²+ release activated Ca ²+ (CRAC) channels in haematopoietic cell lines. In the present work, employing H4IIE liver cells, we investigated fast inactivation of SOC current (Isoc), which occurs at membrane potentials below -60mV. This inactivation was significantly reduced when BAPTA, a faster Ca ²+ buffer, was used instead of EGTA, and was completely abolished if Na+ was used as a charge carrier in the absence of divalent cations in the external medium. These results suggested that fast inactivation of SOCs in H4IIE cells was Ca ²+ dependent and was similar to the fast inactivation of CRAC channels. Experiments showing that the fast inactivation of Isoc was not affected by the disruption of actin by latrunculin B indicate that the cytoskeleton is unlikely to be involved. To elucidate the mechanism of Ca ²+ dependence, a possible role of calmodulin (CaM) in SOCs’ fast inactivation was investigated. The CaM inhibitors Mas-7 and calmidazolium failed to affect Isoc fast inactivation, whereas over-expression of a CaM inhibitor peptide or a mutant CaM lacking functional EF hands significantly altered the inactivation of Isoc. Out of two exponential components normally required to approximate kinetics of Isoc fast inactivation, the faster component was reduced in amplitude by 30%, compared to the control. The results presented suggest that CaM is responsible for at least part of Ca ²+-dependent fast inactivation of Isoc in liver cells. It is hypothesized that CaM is tethered to the channel itself and therefore protected from chemical inhibitors.
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