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从谢弗侧支释放锌及其意义。

Zinc release from Schaffer collaterals and its significance.

作者信息

Takeda Atsushi, Nakajima Satoko, Fuke Sayuri, Sakurada Naomi, Minami Akira, Oku Naoto

机构信息

Department of Medical Biochemistry, School of Pharmaceutical Sciences, University of Shizuoka, 52-1 Yada, Suruga-ku, Shizuoka 422-8526, Japan.

出版信息

Brain Res Bull. 2006 Feb 15;68(6):442-7. doi: 10.1016/j.brainresbull.2005.10.001. Epub 2005 Oct 24.

DOI:10.1016/j.brainresbull.2005.10.001
PMID:16459200
Abstract

On the basis of the evidence that approximately 45% of Schaffer collateral boutons are zinc-positive, zinc release from Schaffer collaterals and its action were examined in hippocampal slices. When zinc release from Schaffer collaterals was examined using ZnAF-2, a membrane-impermeable zinc indicator, ZnAF-2 signal in the stratum radiatum of the CA1 was increased by tetanic stimuli at 100 Hz for 1s, suggesting that zinc is released from Schaffer collaterals in a calcium- and impulse-dependent manner. An in vivo microdialysis experiment indicated that the perfusion with 10 microM zinc significantly decreases extracellular glutamate concentration in the CA1. When tetanic stimuli at 100 Hz for 5s were delivered to the dentate granule cells, the increase in calcium signal in the stratum radiatum of the CA1, as well as in the stratum lucidum of the CA3, was attenuated by addition of 10 microM zinc, while enhanced by addition of 1mM CaEDTA, a membrane-impermeable zinc chelator. The increase in calcium signal in the CA1, in which Schaffer collateral synapses exist, during delivery of tetanic stimuli at 100 Hz for 1s to the Schaffer collateral-commissural pathway was also significantly enhanced by addition of 1mM CaEDTA. These results suggest that zinc released from Schaffer collaterals suppressively modulates presynaptic and postsynaptic calcium signaling in the CA1, followed by the suppression of glutamate release.

摘要

基于约45%的谢弗侧支终扣为锌阳性这一证据,研究人员在海马切片中检测了谢弗侧支的锌释放及其作用。当使用膜不透性锌指示剂ZnAF-2检测谢弗侧支的锌释放时,100 Hz持续1秒的强直刺激可使CA1区辐射层中的ZnAF-2信号增强,这表明锌以钙和冲动依赖的方式从谢弗侧支释放。一项体内微透析实验表明,用10微摩尔锌灌注可显著降低CA1区细胞外谷氨酸浓度。当对齿状颗粒细胞施加100 Hz持续5秒的强直刺激时,添加10微摩尔锌可减弱CA1区辐射层以及CA3区透明层中钙信号的增加,而添加1毫摩尔CaEDTA(一种膜不透性锌螯合剂)则可增强钙信号的增加。在对谢弗侧支-连合通路施加100 Hz持续1秒的强直刺激期间,添加1毫摩尔CaEDTA也可显著增强存在谢弗侧支突触的CA1区钙信号的增加。这些结果表明,从谢弗侧支释放的锌对CA1区突触前和突触后钙信号进行抑制性调节,进而抑制谷氨酸释放。

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