An outwardly rectifying Cl (ORCl) current of mu'/> Synergetic activation of outwardly rectifying Cl− currents by hypotonic stress and external Ca2+ in murine osteoclasts
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Synergetic activation of outwardly rectifying Cl− currents by hypotonic stress and external Ca2+ in murine osteoclasts

机译:低渗应激和小鼠破骨细胞中外部Ca2 +协同向外激活Cl-电流的激活

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摘要

class="enumerated" style="list-style-type:decimal">An outwardly rectifying Cl (ORCl) current of murine osteoclasts was activated by hypotonic stimulation. The current was characterized by rapid activation, little inactivation, strong outward rectification, blockage by DIDS and permeability to organic acids (pyruvate and glutamate).The hypotonically activated ORCl current was inhibited by intracellular dialysis with an ATP-free pipette solution, but not by replacement of ATP with a poorly hydrolysable ATP analogue adenosine 5′-O-(3-thiotriphosphate). The current amplitude was reduced when intracellular alkalinity increased over the pH range 6.6–8.0.Intracellular application of cytochalasin D occasionally activated the ORCl current without hypotonic stress, but inhibited activation of the ORCl current by hypotonic stimulation. The hypotonically activated ORCl current was unaffected by a non-actin-depolymerizing cytochalasin, chaetoglobosin C, but partially inhibited by deoxyribonuclease I.Removal of extracellular Ca2+ inhibited activation of the ORCl current by hypotonic shock, but did not reduce the current once activated. The hypotonically activated ORCl current was partially decreased by intracellular dialysis with 20 mm EGTA.With 10 mm Ca2+ in the extracellular medium, the ORCl current was activated in response to more minor decreases in osmolarity than with 1 mm Ca2+. The increased sensitivity to hypotonicity was mimicked by increasing the intracellular Ca2+ level (pCa 6.5).These results suggest that hypotonic stimulation and a rise in the extracellular Ca2+ level synergistically activate the ORCl channel of murine osteoclasts, and that the activating process is modified by multiple intracellular factors (pH, ATP and actin cytoskeletal organization).
机译:class =“ enumerated” style =“ list-style-type:decimal”> <!-list-behavior =枚举前缀-word = mark-type = decimal max-label-size = 0-> 低渗刺激激活了鼠破骨细胞的向外整流Cl -(ORC1)电流。该电流具有活化快,失活少,向外整流作用强,被DIDS阻断和对有机酸(丙酮酸和谷氨酸)的渗透性的特点。游离移液溶液,但不能用水解性差的ATP类似物腺苷5'-O-(3-硫代三磷酸)代替ATP。在pH范围为6.6–8.0时,当细胞内碱度增加时,电流幅度减小。低渗激活的ORCl电流不受非肌动蛋白解聚的细胞松弛素Chaetoglobosin C的影响,但部分被脱氧核糖核酸酶I抑制。 去除细胞外Ca 2 + 抑制了激活ORCl电流受到低渗冲击,但一旦激活,电流并未降低。低渗激活的ORCl电流通过20 mm EGTA的细胞内透析而部分降低。 在细胞外培养基中使用10 mm Ca 2 + 时,ORCl电流被激活。与1 mm Ca 2 + 相比,渗透压降低较小。对低渗敏感性的增加可以通过增加细胞内Ca 2 + 水平(pCa 6.5)来模拟。 这些结果表明低渗刺激和细胞外Ca 的升高2 + 水平协同激活鼠破骨细胞的ORCl通道,且激活过程受到多种细胞内因子(pH,ATP和肌动蛋白细胞骨架组织)的修饰。

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