钙在啮齿动物和人类星形胶质细胞的保护性和毒性(非线性)反应中的作用。

N Debbie Slamon, Carole Mead, Chris Morgan, Andy Mitchell, Vic W Pentreath
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引用次数: 5

摘要

在C6和1321N1细胞的培养中,研究了[Ca(2+)](i)在暴露于不同化学物质时星形胶质细胞反应性变化中的作用。细胞暴露于多达三次连续脉冲的分化剂dBcAMP中,诱导细胞的激活型变化。其他细胞,不管有没有dBcAMP治疗,都用不同浓度的抗抑郁药阿米替林和氟西汀以及神经胶质毒性药物丙烯酰胺和氯喹进行治疗。在一些实验中,使用l型电压钙通道阻滞剂硝苯地平。使用Fura-2AM和荧光显微镜上的电荷耦合器件(CCD)相机测量细胞群中的[Ca(2+)](i)。dBcAMP诱导了[Ca(2+)](i)的剂量和时间依赖性变化,[Ca(2+)](i)的振荡和平均值[Ca(2+)](i)的增加(例如,在C6细胞中,18分钟的平均值[Ca(2+)](i)在单次dBcAMP脉冲后为318 +/- 20nM,在两次连续脉冲后为489 +/- 17nM (p < 0.001),在三次脉冲后为275 +/- 30nM(不显著))。氟西汀和阿米替林治疗剂量引起钙振荡和平均钙浓度的增加(当[Ca(2+)](i)为411 +/- 35nM时,C6细胞中记录的最大平均增幅为0.02 mmol氟西汀10min,对照组为254 +/- 25nM, p = 0.01)。两种抗抑郁药的高剂量(非治疗性)可显著降低。氯喹和丙烯酰胺也引起[Ca(2+)](i)的剂量依赖性双相型改变,在较低的亚细胞毒性剂量下显着减少,随后在较高浓度下显着增加,接近导致细胞损伤的剂量。硝苯地平治疗引起dBcAMP、抗抑郁药或有毒物质引起的钙变化的一些降低,但这种物质也引起细胞毒性改变。研究结果表明,C6和1321N1细胞对不同化学试剂的激活型变化(通常与保护能力增加有关)和毒性反应都与[Ca(2+)]的剂量依赖性改变有关(i)。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
The involvement of calcium in the protective and toxic (nonlinear) responses of rodent and human astroglial cells.

The involvement of [Ca(2+)](i) in the reactive changes of astrocytes which accompany exposure to different chemicals were studied in cultures of C6 and 1321N1 cells. Cells were exposed to up to three serial pulses of the differentiating agent dBcAMP, which induces activation-type changes in the cells. Other cells, with or without the dBcAMP treatments, were treated with a range of concentrations of the antidepressants amitriptyline and fluoxetine and the glial toxicants acrylamide and chloroquine. In some experiments the L-type voltage calcium channel blocker Nifedipine was employed. [Ca(2+)](i) was measured in populations of the cells using Fura-2AM and a charge coupled device (CCD) camera attached to a fluorescence microscope. dBcAMP induced both dose- and time-dependent changes in [ Ca(2+)](i) with increases in both the [Ca(2+)](i) oscillations and mean [Ca(2+)](i) (e.g. in C6 cells at 18 min mean [Ca(2+)](i) was 318 +/- 20nM following the single differentiating dBcAMP pulses, 489 +/- 17nM (p < 0.001) following two serial pulses, and 275 +/- 30nM (not significant) following three pulses). Therapeutic doses of fluoxetine and amitriptyline caused increases in the calcium oscillations and the mean calcium concentrations ( maximum recorded mean increase was in the C6 cells at 10min by 0.02 muM fluoxetine when [Ca(2+)](i) was 411 +/- 35nM c.f. control 254 +/- 25nM, p = 0.01). Higher (non-therapeutic) doses of both antidepressants caused significant reductions. Chloroquine and acrylamide also caused dose-dependent bi-phasic types of alterations in [Ca(2+)](i), with significant reductions at lower, sub-cytotoxic doses followed by significant increases at higher concentrations, approaching those which cause cell damage. Nifedipine treatment caused some reductions in the dBcAMP, antidepressant or toxicant-induced calcium changes, but this substance also initiated cytotoxic alterations. The findings show that both the activation-type changes (which are frequently associated with increased protective capacities) and toxic responses of C6 and 1321N1 cells to different chemical agents are associated with dose-dependent alterations in [Ca(2+)](i).

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