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Independent optical excitation of distinct neural populations

机译:不同神经群体的独立光激发

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摘要

Optogenetic tools enable examination of how specific cell types contribute to brain circuit functions. A long-standing question is whether it is possible to independently activate two distinct neural populations in mammalian brain tissue. Such a capability would enable the study of how different synapses or pathways interact to encode information in the brain. Here we describe two channelrhodopsins, Chronos and Chrimson, discovered through sequencing and physiological characterization of opsins from over 100 species of alga. Chrimson's excitation spectrum is red shifted by 45 nm relative to previous channelrhodopsins and can enable experiments in which red light is preferred. We show minimal visual system-mediated behavioral interference when using Chrimson in neurobehavioral studies in Drosophila melanogaster. Chronos has faster kinetics than previous channelrhodopsins yet is effectively more light sensitive. Together these two reagents enable two-color activation of neural spiking and downstream synaptic transmission in independent neural populations without detectable cross-talk in mouse brain slice.
机译:光遗传学工具可以检查特定细胞类型如何促进脑电路功能。一个长期存在的问题是,是否有可能在哺乳动物脑组织中独立激活两个不同的神经种群。这种能力将使人们能够研究不同的突触或途径如何相互作用以在大脑中编码信息。在这里,我们描述了两种通道视紫红质,Chronos和Chrimson,它们是通过对100多种藻类视蛋白的测序和生理表征发现的。相对于以前的通道视紫红质,Chrimson的激发光谱红移了45 nm,并且可以进行优选红光的实验。当在果蝇的神经行为研究中使用Chrimson时,我们显示最小的视觉系统介导的行为干扰。计时比以前的通道视紫红质动力学更快,但实际上对光更敏感。这两种试剂结合在一起,可以在独立的神经种群中实现神经突刺和下游突触传递的双色激活,而在小鼠脑片中却没有可检测到的串扰。

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