Zhang Yan-Ping, Oertner Thomas G
Friedrich Miescher Institute, Novartis Research Foundation, Maulbeerstr. 66, WRO-1066.4.04, CH-4058 Basel, Switzerland.
Nat Methods. 2007 Feb;4(2):139-41. doi: 10.1038/nmeth988. Epub 2006 Dec 31.
We have combined millisecond activation of channelrhodopsin-2 (ChR2), a light-gated ion channel, with two-photon calcium imaging to investigate active synaptic contacts in rat hippocampal slice cultures. Calcium influx was larger during light-induced action potentials than during action potentials induced by somatic current injection, leading to highly reproducible synaptic transmission. Pairing of light stimulation with postsynaptic depolarization induced long-term potentiation, making this technique ideal for genetic and pharmacological dissection of synaptic plasticity.
我们将光门控离子通道通道视紫红质-2(ChR2)的毫秒级激活与双光子钙成像相结合,以研究大鼠海马脑片培养物中的活跃突触联系。光诱导动作电位期间的钙内流比体细胞电流注入诱导的动作电位期间更大,从而导致高度可重复的突触传递。光刺激与突触后去极化配对可诱导长时程增强,这使得该技术成为突触可塑性的遗传和药理学剖析的理想选择。
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