Literature DB >> 20702399

Automated analysis of time-lapse fluorescence microscopy images: from live cell images to intracellular foci.

Oleh Dzyubachyk1, Jeroen Essers, Wiggert A van Cappellen, Céline Baldeyron, Akiko Inagaki, Wiro J Niessen, Erik Meijering.   

Abstract

MOTIVATION: Complete, accurate and reproducible analysis of intracellular foci from fluorescence microscopy image sequences of live cells requires full automation of all processing steps involved: cell segmentation and tracking followed by foci segmentation and pattern analysis. Integrated systems for this purpose are lacking.
RESULTS: Extending our previous work in cell segmentation and tracking, we developed a new system for performing fully automated analysis of fluorescent foci in single cells. The system was validated by applying it to two common tasks: intracellular foci counting (in DNA damage repair experiments) and cell-phase identification based on foci pattern analysis (in DNA replication experiments). Experimental results show that the system performs comparably to expert human observers. Thus, it may replace tedious manual analyses for the considered tasks, and enables high-content screening.
AVAILABILITY AND IMPLEMENTATION: The described system was implemented in MATLAB (The MathWorks, Inc., USA) and compiled to run within the MATLAB environment. The routines together with four sample datasets are available at http://celmia.bigr.nl/. The software is planned for public release, free of charge for non-commercial use, after publication of this article.

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Year:  2010        PMID: 20702399     DOI: 10.1093/bioinformatics/btq434

Source DB:  PubMed          Journal:  Bioinformatics        ISSN: 1367-4803            Impact factor:   6.937


  10 in total

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10.  FoCo: a simple and robust quantification algorithm of nuclear foci.

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  10 in total

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