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亚细胞群体成像工具揭示了海马体CA3区稳定的顶端树突。

Sub-cellular population imaging tools reveal stable apical dendrites in hippocampal area CA3.

作者信息

Moore Jason J, Rashid Shannon K, Bicker Emmett, Johnson Cara D, Codrington Naomi, Chklovskii Dmitri B, Basu Jayeeta

机构信息

Neuroscience Institute, New York University Langone Health, New York, NY, 10016, USA.

Center for Computational Neuroscience, Flatiron Institute, Simons Foundation, New York, NY, 10010, USA.

出版信息

Nat Commun. 2025 Jan 28;16(1):1119. doi: 10.1038/s41467-025-56289-9.

Abstract

Apical and basal dendrites of pyramidal neurons receive anatomically and functionally distinct inputs, implying compartment-level functional diversity during behavior. To test this, we imaged in vivo calcium signals from soma, apical dendrites, and basal dendrites in mouse hippocampal CA3 pyramidal neurons during head-fixed navigation. To capture compartment-specific population dynamics, we developed computational tools to automatically segment dendrites and extract accurate fluorescence traces from densely labeled neurons. We validated the method on sparsely labeled preparations and synthetic data, predicting an optimal labeling density for high experimental throughput and analytical accuracy. Our method detected rapid, local dendritic activity. Dendrites showed robust spatial tuning, similar to soma but with higher activity rates. Across days, apical dendrites remained more stable and outperformed in decoding of the animal's position. Thus, population-level apical and basal dendritic differences may reflect distinct compartment-specific input-output functions and computations in CA3. These tools will facilitate future studies mapping sub-cellular activity and their relation to behavior.

摘要

锥体神经元的顶端和基底树突接收在解剖学和功能上不同的输入,这意味着在行为过程中存在隔室水平的功能多样性。为了验证这一点,我们在小鼠头部固定导航过程中,对海马体CA3锥体神经元的胞体、顶端树突和基底树突的体内钙信号进行了成像。为了捕捉特定隔室的群体动态,我们开发了计算工具,用于自动分割树突,并从密集标记的神经元中提取准确的荧光轨迹。我们在稀疏标记的标本和合成数据上验证了该方法,预测了高实验通量和分析准确性的最佳标记密度。我们的方法检测到了快速的局部树突活动。树突显示出强大的空间调谐,类似于胞体,但活动率更高。在不同的日子里,顶端树突保持更稳定,并且在解码动物位置方面表现更优。因此,群体水平的顶端和基底树突差异可能反映了CA3中不同的特定隔室输入-输出功能和计算。这些工具将有助于未来绘制亚细胞活动及其与行为关系的研究。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f7b6/11775317/e078b7b946cb/41467_2025_56289_Fig1_HTML.jpg

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