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三维亚细胞信号定位的详细分析。

A detailed analysis of 3D subcellular signal localization.

作者信息

Pinidiyaarachchi Amalka, Zieba Agata, Allalou Amin, Pardali Katerina, Wählby Carolina

机构信息

The Centre for Image Analysis, Uppsala University, Uppsala, Sweden.

出版信息

Cytometry A. 2009 Apr;75(4):319-28. doi: 10.1002/cyto.a.20663.

Abstract

Detection and localization of fluorescent signals in relation to other subcellular structures is an important task in various biological studies. Many methods for analysis of fluorescence microscopy image data are limited to 2D. As cells are in fact 3D structures, there is a growing need for robust methods for analysis of 3D data. This article presents an approach for detecting point-like fluorescent signals and analyzing their subnuclear position. Cell nuclei are delineated using marker-controlled (seeded) 3D watershed segmentation. User-defined object and background seeds are given as input, and gradient information defines merging and splitting criteria. Point-like signals are detected using a modified stable wave detector and localized in relation to the nuclear membrane using distance shells. The method was applied to a set of biological data studying the localization of Smad2-Smad4 protein complexes in relation to the nuclear membrane. Smad complexes appear as early as 1 min after stimulation while the highest signal concentration is observed 45 min after stimulation, followed by a concentration decrease. The robust 3D signal detection and concentration measures obtained using the proposed method agree with previous observations while also revealing new information regarding the complex formation.

摘要

在各种生物学研究中,检测荧光信号并确定其与其他亚细胞结构的位置关系是一项重要任务。许多荧光显微镜图像数据分析方法仅限于二维。由于细胞实际上是三维结构,因此对稳健的三维数据分析方法的需求日益增长。本文提出了一种检测点状荧光信号并分析其亚核位置的方法。使用标记控制(种子)三维分水岭分割来勾勒细胞核。将用户定义的对象和背景种子作为输入,梯度信息定义合并和分割标准。使用改进的稳定波检测器检测点状信号,并使用距离壳确定其相对于核膜的位置。该方法应用于一组研究Smad2-Smad4蛋白复合物相对于核膜定位的生物学数据。Smad复合物在刺激后1分钟就出现,而在刺激后45分钟观察到最高信号浓度,随后浓度下降。使用所提出的方法获得的稳健的三维信号检测和浓度测量结果与先前的观察结果一致,同时还揭示了有关复合物形成的新信息。

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