Multi-scale approaches for high-speed imaging and analysis of large neural populations

被引:23
|
作者
Friedrich, Johannes [1 ,2 ,3 ]
Yang, Weijian [4 ]
Soudry, Daniel [1 ,2 ,7 ]
Mu, Yu [3 ]
Ahrens, Misha B. [3 ]
Yuste, Rafael [4 ,5 ]
Peterka, Darcy S. [4 ,6 ]
Paninski, Liam [1 ,2 ,4 ,5 ,6 ]
机构
[1] Columbia Univ, Grossman Ctr Stat Mind, Dept Stat, New York, NY 10027 USA
[2] Columbia Univ, Ctr Theoret Neurosci, New York, NY 10027 USA
[3] Howard Hughes Med Inst, Janelia Res Campus, Ashburn, VA 20147 USA
[4] Columbia Univ, Dept Biol Sci, NeuroTechnol Ctr, New York, NY 10027 USA
[5] Columbia Univ, Kavli Inst Brain Sci, New York, NY 10027 USA
[6] Columbia Univ, Zuckerman Mind Brain Behav Inst, New York, NY 10027 USA
[7] Technion, Dept Elect Engn, Haifa, Israel
基金
瑞士国家科学基金会; 美国国家卫生研究院;
关键词
LIGHT-SHEET MICROSCOPY; NONNEGATIVE MATRIX FACTORIZATION; TENSOR FACTORIZATIONS; VOLTAGE INDICATORS; NEURONAL-ACTIVITY; FIELD MICROSCOPY; CALCIUM SIGNALS; IN-VIVO; BRAIN; DECONVOLUTION;
D O I
10.1371/journal.pcbi.1005685
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Progress in modern neuroscience critically depends on our ability to observe the activity of large neuronal populations with cellular spatial and high temporal resolution. However, two bottlenecks constrain efforts towards fast imaging of large populations. First, the resulting large video data is challenging to analyze. Second, there is an explicit tradeoff between imaging speed, signal-to-noise, and field of view: with current recording technology we cannot image very large neuronal populations with simultaneously high spatial and temporal resolution. Here we describe multi-scale approaches for alleviating both of these bottlenecks. First, we show that spatial and temporal decimation techniques based on simple local averaging provide order-of-magnitude speedups in spatiotemporally demixing calcium video data into estimates of single-cell neural activity. Second, once the shapes of individual neurons have been identified at fine scale (e.g., after an initial phase of conventional imaging with standard temporal and spatial resolution), we find that the spatial/temporal resolution tradeoff shifts dramatically: after demixing we can accurately recover denoised fluorescence traces and deconvolved neural activity of each individual neuron from coarse scale data that has been spatially decimated by an order of magnitude. This offers a cheap method for compressing this large video data, and also implies that it is possible to either speed up imaging significantly, or to "zoom out" by a corresponding factor to image order-of-magnitude larger neuronal populations with minimal loss in accuracy or temporal resolution.
引用
收藏
页数:24
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