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Laser-scanning Photostimulation of Optogenetically Targeted Forebrain Circuits

机译:激光扫描光致目标前脑电路的光刺激。

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摘要

The sensory forebrain is composed of intricately connected cell types, of which functional properties have yet to be fully elucidated. Understanding the interactions of these forebrain circuits has been aided recently by the development of optogenetic methods for light-mediated modulation of neuronal activity. Here, we describe a protocol for examining the functional organization of forebrain circuits in vitro using laser-scanning photostimulation of channelrhodopsin, expressed optogenetically via viral-mediated transfection. This approach also exploits the utility of cre-lox recombination in transgenic mice to target expression in specific neuronal cell types. Following transfection, neurons are physiologically recorded in slice preparations using whole-cell patch clamp to measure their evoked responses to laser-scanning photostimulation of channelrhodopsin expressing fibers. This approach enables an assessment of functional topography and synaptic properties. Morphological correlates can be obtained by imaging the neuroanatomical expression of channelrhodopsin expressing fibers using confocal microscopy of the live slice or post-fixed tissue. These methods enable functional investigations of forebrain circuits that expand upon more conventional approaches.
机译:感觉前脑由错综复杂的细胞类型组成,这些细胞的功能特性尚未完全阐明。最近,通过光遗传学调节神经元活动的光遗传学方法的发展,帮助理解了这些前脑回路的相互作用。在这里,我们描述了一种协议,该协议使用激光扫描光刺激的视紫红质(通过病毒介导的转基因表达)体外检查前脑回路的功能组织。这种方法还利用了转基因小鼠中cre-lox重组的效用,以靶向特定神经元细胞类型的表达。转染后,使用全细胞膜片钳将神经元生理记录在切片制品中,以测量其对表达视紫红质表达纤维的激光扫描光刺激的诱发反应。这种方法可以评估功能性地形和突触特性。形态相关性可以通过使用活切片或固定后组织的共聚焦显微镜对表达视紫红质表达纤维的神经解剖表达进行成像来获得。这些方法可以对前脑电路进行功能研究,从而扩展到更多常规方法上。

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