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Population-scale three-dimensional reconstruction and quantitative profiling of microglia arbors

机译:小胶质乔木的种群规模三维重建和定量分析

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>Motivation: The arbor morphologies of brain microglia are important indicators of cell activation. This article fills the need for accurate, robust, adaptive and scalable methods for reconstructing 3-D microglial arbors and quantitatively mapping microglia activation states over extended brain tissue regions.>Results: Thick rat brain sections (100–300 µm) were multiplex immunolabeled for IBA1 and Hoechst, and imaged by step-and-image confocal microscopy with automated 3-D image mosaicing, producing seamless images of extended brain regions (e.g. 5903 × 9874 × 229 voxels). An over-complete dictionary-based model was learned for the image-specific local structure of microglial processes. The microglial arbors were reconstructed seamlessly using an automated and scalable algorithm that exploits microglia-specific constraints. This method detected 80.1 and 92.8% more centered arbor points, and 53.5 and 55.5% fewer spurious points than existing vesselness and LoG-based methods, respectively, and the traces were 13.1 and 15.5% more accurate based on the DIADEM metric. The arbor morphologies were quantified using Scorcioni’s L-measure. Coifman’s harmonic co-clustering revealed four morphologically distinct classes that concord with known microglia activation patterns. This enabled us to map spatial distributions of microglial activation and cell abundances.>Availability and implementation: Experimental protocols, sample datasets, scalable open-source multi-threaded software implementation (C++, MATLAB) in the electronic supplement, and website (). >Contact: >Supplementary information: are available at Bioinformatics online.
机译:>动机:脑小胶质细胞的乔木形态是细胞激活的重要指标。本文满足了对精确的,鲁棒的,自适应的和可扩展的方法的需求,这些方法可用于重建3-D小胶质树胶体并定量绘制扩展的脑组织区域上的小胶质细胞活化状态。>结果:大鼠脑部较厚(100-300) (μm)对IBA1和Hoechst进行了多重免疫标记,并通过具有自动3-D图像拼接功能的步进图像共聚焦显微镜成像,从而生成了脑部扩展区域(例如5903××9874××229体素)的无缝图像。对于小胶质细胞过程的图像特定局部结构,学习了一个基于字典的完整模型。使用自动和可扩展的算法,利用小胶质细胞特定的约束,无缝地重建了小胶质树皮。与现有的基于血管和基于LoG的方法相比,此方法检测到的中心心轴点分别增加了80.1和92.8%,伪点减少了53.5和55.5%,基于DIADEM度量,迹线的精确度分别为13.1和15.5%。乔木形态使用Scorcioni的L度量进行了量化。 Coifman的谐波共聚显示出与已知的小胶质细胞激活模式一致的四个形态学上不同的类别。这使我们能够绘制小胶质细胞活化和细胞丰度的空间分布。>可用性和实现:实验协议,样本数据集,可扩展的开源多线程软件实现(C ++,MATLAB)在电子增刊中,和网站()。 >联系方式: >补充信息:可从生物信息学在线获得。

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