Thymol-evoked Ca 2+ Mobilization and Ion Currents in Pituitary GH 3 Cells

In this study, an attempt was made to elucidate the effects of thymol, a monocyclic phenolic compound, on Ca 2+ mobilization and ion currents in pituitary GH 3 cells with the aid of fura-2 fluorimetry and the whole-cell voltage-clamp technique. Thymol increased intracellular Ca 2+ concentrations ([C...

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Published inNatural product communications Vol. 4; no. 6
Main Authors Shen, Ai-Yu, Huang, Mei-Han, Wang, Trey-Shy, Wu, Hui-Ming, Kang, Ya-Fei, Chen, Chi-Lan
Format Journal Article
LanguageEnglish
Published 01.06.2009
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Abstract In this study, an attempt was made to elucidate the effects of thymol, a monocyclic phenolic compound, on Ca 2+ mobilization and ion currents in pituitary GH 3 cells with the aid of fura-2 fluorimetry and the whole-cell voltage-clamp technique. Thymol increased intracellular Ca 2+ concentrations ([Ca 2+ ] i ) in GH 3 cells loaded with Ca 2+ -sensitive dye fura-2. Removing extracellular Ca 2+ reduced the thymol-induced [Ca 2+ ] i rise. In Ca 2+ -free solution, thymol-evoked [Ca 2+ ] i rise was unchanged by depleting the Ca 2+ store with thapsigargin (1 μM), while the thapsigargin-induced [Ca 2+ ] i rise was reduced by pretreatment with thymol. These results imply that the Ca 2+ stores depleted by thymol comprise thapsigargin-sensitive and thapsigargin-insensitive pools. In addition, after depletion of the internal Ca 2+ store with 100 μM thymol in Ca 2+ -free solution, a subsequent application of Ca 2+ greatly induced a [Ca 2+ ] i increase. The results indicate that, similar to thapsigargin, 100 μM thymol may activate the capacitative calcium entry (CCE) channel. However, thymol (100 μM) had a slight depressant action in L-type calcium current ( I CaL ). The stimulatory actions of thymol on Ca 2+ signaling may partly be responsible for the underlying cellular mechanisms through which it affects neuroendocrine functions.
AbstractList In this study, an attempt was made to elucidate the effects of thymol, a monocyclic phenolic compound, on Ca 2+ mobilization and ion currents in pituitary GH 3 cells with the aid of fura-2 fluorimetry and the whole-cell voltage-clamp technique. Thymol increased intracellular Ca 2+ concentrations ([Ca 2+ ] i ) in GH 3 cells loaded with Ca 2+ -sensitive dye fura-2. Removing extracellular Ca 2+ reduced the thymol-induced [Ca 2+ ] i rise. In Ca 2+ -free solution, thymol-evoked [Ca 2+ ] i rise was unchanged by depleting the Ca 2+ store with thapsigargin (1 μM), while the thapsigargin-induced [Ca 2+ ] i rise was reduced by pretreatment with thymol. These results imply that the Ca 2+ stores depleted by thymol comprise thapsigargin-sensitive and thapsigargin-insensitive pools. In addition, after depletion of the internal Ca 2+ store with 100 μM thymol in Ca 2+ -free solution, a subsequent application of Ca 2+ greatly induced a [Ca 2+ ] i increase. The results indicate that, similar to thapsigargin, 100 μM thymol may activate the capacitative calcium entry (CCE) channel. However, thymol (100 μM) had a slight depressant action in L-type calcium current ( I CaL ). The stimulatory actions of thymol on Ca 2+ signaling may partly be responsible for the underlying cellular mechanisms through which it affects neuroendocrine functions.
Author Chen, Chi-Lan
Shen, Ai-Yu
Wu, Hui-Ming
Kang, Ya-Fei
Huang, Mei-Han
Wang, Trey-Shy
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