首页> 外文期刊>Brain research >Manganese suppresses ATP-dependent intercellular calcium waves in astrocyte networks through alteration of mitochondrial and endoplasmic reticulum calcium dynamics.
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Manganese suppresses ATP-dependent intercellular calcium waves in astrocyte networks through alteration of mitochondrial and endoplasmic reticulum calcium dynamics.

机译:锰通过改变线粒体和内质网钙动力学来抑制星形胶质细胞网络中ATP依赖的细胞间钙波。

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The neurotoxicity of manganese [Mn] is due in part to glutamate excitotoxicity. Release of ATP by astrocytes is a critical modulator of glutamatergic neurotransmission, which is regulated by calcium (Ca(2+)) waves that propagate through astrocytic networks in response to synaptic activity. It was postulated that Mn alters ATP-dependent intracellular Ca(2+) dynamics in astrocytes, thereby suppressing Ca(2+) wave activity. Confluent primary cultures of cortical astrocytes were loaded with the Ca(2+)-sensitive dye fluo-4 and examined by fluorescence microscopy for Ca(2+) wave activity following micropipet mechanical stimulation of a single cell. Mitochondrial Ca(2+) was evaluated by fluorescence microscopy following addition of ATP using the mitochondrial-specific Ca(2+) dye rhod-2-AM. Imaging studies revealed that pretreatment of astrocytes with 1-10 muM Mn significantly reduced the rate, area, and amplitude of mechanically induced Ca(2+) waves. This attenuation was not a result of inhibited mitochondrial calcium uptake because robust calcium waves were still observed following pretreatment of astrocytes with Ru360, an inhibitor of mitochondrial Ca(2+) uptake, either in coupling or uncoupling conditions. However, determination of endoplasmic reticulum (ER) Ca(2+) levels in cells using the sarco/endoplasmic reticulum Ca(2+)-ATPase inhibitor thapsigargin indicated that Mn reduced the available pool of releasable ER Ca(2+) at concentrations as low as 1 muM. Examination of ATP-stimulated changes in mitochondrial Ca(2+) indicated that, in cells pretreated with Mn, mitochondria retained high levels of Ca(2+). It is concluded that exposure of astrocytes to low concentrations of Mn(2+) results in sequestration of Ca(2+) within the mitochondria that reduces the available pool of releasable Ca(2+) within the ER, thereby inhibiting calcium wave activity.
机译:锰[Mn]的神经毒性部分归因于谷氨酸的兴奋性毒性。星形胶质细胞释放的ATP是谷氨酸能神经传递的关键调节剂,其受钙(Ca(2+))波调节,钙波通过星形细胞网络传播以响应突触活动。据推测,锰改变星形胶质细胞中ATP依赖的细胞内Ca(2+)动态,从而抑制Ca(2+)波的活动。融合的皮质星形胶质细胞的原代培养物中装有Ca(2+)敏感染料fluo-4,并通过微移液管机械刺激单个细胞后,通过荧光显微镜检查Ca(2+)波的活性。线粒体Ca(2+)的荧光显微镜评估后添加ATP,使用线粒体特异性Ca(2+)染料rhod-2-AM。影像学研究表明,以1-10μMMn预处理星形胶质细胞可显着降低机械诱导的Ca(2+)波的速率,面积和幅度。这种衰减不是抑制线粒体钙摄取的结果,因为在星形胶质细胞用Ru360(线粒体Ca(2+)摄取的抑制剂)预处理星形胶质细胞后,无论在偶联还是非偶联条件下,都仍然观察到强大的钙波。但是,使用肌浆/内质网Ca(2 +)-ATPase抑制剂thapsigargin测定细胞中内质网(ER)Ca(2+)的水平表明,Mn降低了可释放ER Ca(2+)的可用浓度低至1毫米。 ATP刺激的线粒体Ca(2+)变化表明,在用Mn预处理的细胞中,线粒体保留了高水平的Ca(2+)。结论是,星形胶质细胞暴露于低浓度的Mn(2+)导致线粒体中Ca(2+)螯合,从而减少了ER中的可释放Ca(2+)的可用池,从而抑制了钙波活性。

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