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Two-photon imaging of spatially extended neuronal network dynamics with high temporal resolution

机译:具有高时间分辨率的空间扩展神经元网络动力学的双光子成像

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摘要

We describe a simple two-photon fluorescence imaging strategy, called targeted path scanning (TPS), to monitor the dynamics of spatially extended neuronal networks with high spatiotemporal resolution. Our strategy combines the advantages of mirror-based scanning, minimized dead time, ease of implementation, and compatibility with high-resolution low-magnification objectives. To demonstrate the performance of TPS, we monitor the calcium dynamics distributed across an entire juvenile rat hippocampus (>1.5mm), at scan rates of 100Hz, with single cell resolution and single action potential sensitivity. Our strategy for fast, efficient two-photon microscopy over spatially extended regions provides a particularly attractive solution for monitoring neuronal population activity in thick tissue, without sacrificing the signal to noise ratio or high spatial resolution associated with standard two-photon microscopy. Finally, we provide the code to make our technique generally available.
机译:我们描述了一种简单的两光子荧光成像策略,称为目标路径扫描(TPS),以高时空分辨率监视空间扩展的神经元网络的动态。我们的策略结合了基于镜像的扫描,停滞时间最小,易于实现以及与高分辨率低倍物镜兼容的优点。为了证明TPS的性能,我们以100Hz的扫描速率监测了整个幼年大鼠海马(> 1.5mm)中的钙动力学,具有单细胞分辨率和单动作电位敏感性。我们在空间扩展区域上进行快速,高效的双光子显微术的策略为监视厚组织中的神经元群体活动提供了一种特别有吸引力的解决方案,而不会牺牲与标准双光子显微术相关的信噪比或高空间分辨率。最后,我们提供了使我们的技术普遍可用的代码。

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