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通过笼锁钙的闪光光解揭示海马神经元树突中钙的空间受限扩散。

Spatially confined diffusion of calcium in dendrites of hippocampal neurons revealed by flash photolysis of caged calcium.

作者信息

Korkotian Eduard, Segal Menahem

机构信息

Department of Neurobiology, The Weizmann Institute, Rehovot, Israel.

出版信息

Cell Calcium. 2006 Nov-Dec;40(5-6):441-9. doi: 10.1016/j.ceca.2006.08.008. Epub 2006 Oct 24.

DOI:10.1016/j.ceca.2006.08.008
PMID:17064764
Abstract

The extent of diffusion of a locally evoked calcium surge in dendrites of cultured hippocampal neurons was studied by flash photolysis of caged EGTA. Cells were transfected with pDsRed for visualization, preincubated with caged NP-EGTA (AM) and Fluo-4 (AM) at room temperature and imaged in a PASCAL confocal microscope. Pulses of UV laser light within an active sphere of about 1 micro m(2) produced a rise of Fluo-4 fluorescence transients in dendrites which peaked at 1 ms and decayed exponentially with a fast (8-10 ms) time constant. A slower decay component was uncovered following incubation with thapsigargin. Lateral diffusion of [Ca(2+)]i did not vary significantly among different size dendrites being symmetric and reaching about 3-3.5 micro mm at a diffusion rate of 0.8 micro mm/ms on both sides of the photolysis center. Fluo-4 was also replaced by the membrane-bound Fluo-NOMO (AM) or by the 'heavy' Calcium Green dextran (CGd) loaded through a patch pipette. Similar rates of diffusion were found in these cases, indicating that the diffusion is not of the dye complexed to calcium but of genuine free calcium ions. Interestingly, presence of a dendritic spine at the focus of photolysis significantly reduced [Ca(2+)]i spread while the focal transient remained unaffected. Finally, [Ca(2+)]i diffused about twice as far from the photolysis sphere in glass tubes of a similar diameter to that of a dendrite, indicating that intrinsic calcium uptake mechanisms in the dendrite determine the diffusion of calcium away from its original site of rise.

摘要

通过笼状乙二醇双(2-氨基乙醚)四乙酸(EGTA)的闪光光解,研究了培养的海马神经元树突中局部诱发的钙激增的扩散范围。细胞用pDsRed转染以进行可视化,在室温下用笼状NP-EGTA(AM)和Fluo-4(AM)预孵育,并在PASCAL共聚焦显微镜下成像。在约1μm²的活性球体内的紫外激光脉冲在树突中产生Fluo-4荧光瞬变的升高,其在1毫秒达到峰值并以快速(8 - 10毫秒)的时间常数指数衰减。在用毒胡萝卜素孵育后发现了一个较慢的衰减成分。不同大小的树突之间,[Ca²⁺]i的横向扩散没有显著差异,是对称的,在光解中心两侧以0.8μm/毫秒的扩散速率达到约3 - 3.5μm。Fluo-4也被膜结合的Fluo-NOMO(AM)或通过膜片吸管加载的“重”钙绿葡聚糖(CGd)所取代。在这些情况下发现了相似的扩散速率,表明扩散的不是与钙络合的染料,而是真正的游离钙离子。有趣的是,在光解焦点处存在树突棘显著减少了[Ca²⁺]i的扩散,而焦点瞬变不受影响。最后,[Ca²⁺]i在直径与树突相似的玻璃管中从光解球扩散的距离约为两倍,表明树突中的内在钙摄取机制决定了钙从其原始升高部位的扩散。

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