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      Automated Method for the Rapid and Precise Estimation of Adherent Cell Culture Characteristics from Phase Contrast Microscopy Images

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          Abstract

          The quantitative determination of key adherent cell culture characteristics such as confluency, morphology, and cell density is necessary for the evaluation of experimental outcomes and to provide a suitable basis for the establishment of robust cell culture protocols. Automated processing of images acquired using phase contrast microscopy (PCM), an imaging modality widely used for the visual inspection of adherent cell cultures, could enable the non-invasive determination of these characteristics. We present an image-processing approach that accurately detects cellular objects in PCM images through a combination of local contrast thresholding and post hoc correction of halo artifacts. The method was thoroughly validated using a variety of cell lines, microscope models and imaging conditions, demonstrating consistently high segmentation performance in all cases and very short processing times (<1 s per 1,208 × 960 pixels image). Based on the high segmentation performance, it was possible to precisely determine culture confluency, cell density, and the morphology of cellular objects, demonstrating the wide applicability of our algorithm for typical microscopy image processing pipelines. Furthermore, PCM image segmentation was used to facilitate the interpretation and analysis of fluorescence microscopy data, enabling the determination of temporal and spatial expression patterns of a fluorescent reporter. We created a software toolbox (PHANTAST) that bundles all the algorithms and provides an easy to use graphical user interface. Source-code for MATLAB and ImageJ is freely available under a permissive open-source license. Biotechnol. Bioeng. 2014;111: 504–517. © 2013 Wiley Periodicals, Inc.

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          Most cited references50

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          NIH Image to ImageJ: 25 years of image analysis.

          For the past 25 years NIH Image and ImageJ software have been pioneers as open tools for the analysis of scientific images. We discuss the origins, challenges and solutions of these two programs, and how their history can serve to advise and inform other software projects.
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            Conversion of embryonic stem cells into neuroectodermal precursors in adherent monoculture.

            Mouse embryonic stem (ES) cells are competent for production of all fetal and adult cell types. However, the utility of ES cells as a developmental model or as a source of defined cell populations for pharmaceutical screening or transplantation is compromised because their differentiation in vitro is poorly controlled. Specification of primary lineages is not understood and consequently differentiation protocols are empirical, yielding variable and heterogeneous outcomes. Here we report that neither multicellular aggregation nor coculture is necessary for ES cells to commit efficiently to a neural fate. In adherent monoculture, elimination of inductive signals for alternative fates is sufficient for ES cells to develop into neural precursors. This process is not a simple default pathway, however, but requires autocrine fibroblast growth factor (FGF). Using flow cytometry quantitation and recording of individual colonies, we establish that the bulk of ES cells undergo neural conversion. The neural precursors can be purified to homogeneity by fluorescence activated cell sorting (FACS) or drug selection. This system provides a platform for defining the molecular machinery of neural commitment and optimizing the efficiency of neuronal and glial cell production from pluripotent mammalian stem cells.
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              Evaluation: from precision, recall and f-measure to roc, informedness, markedness & correlation

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                Author and article information

                Journal
                Biotechnol Bioeng
                Biotechnol. Bioeng
                bit
                Biotechnology and Bioengineering
                Blackwell Publishing Ltd (Oxford, UK )
                0006-3592
                1097-0290
                March 2014
                05 October 2013
                : 111
                : 3
                : 504-517
                Affiliations
                [1 ]Department of Biochemical Engineering, University College London Torrington Place, London, WC1E 7JE, United Kingdom
                [2 ]Centre for Mathematics and Physics in the Life Sciences and Experimental Biology, University College London London, United Kingdom
                [3 ]Department of Computer Science, University College London London, United Kingdom
                Author notes
                Correspondence to: N. Szita

                Contract grant sponsor: British Heart Foundation

                Contract grant number: SP/08/004

                Contract grant sponsor: UCL-BE Peter Dunnill Scholarship

                Contract grant sponsor: UCL Overseas Research Scholarship

                Article
                10.1002/bit.25115
                4260842
                24037521
                0eb26e91-50ff-4a50-99ba-59d3bf1bdea9
                © 2013 The Authors. Biotechnology and Bioengineering Published by Wiley Periodicals, Inc.

                This is an open access article under the terms of the Creative Commons Attribution License, which permits use, distribution and reproduction in any medium, provided the original work is properly cited.

                History
                : 08 March 2013
                : 23 July 2013
                : 09 September 2013
                : 13 September 2013
                Categories
                Articles

                Biotechnology
                confluency,morphology,cell density,adherent cells,phase contrast microscopy,image-processing,on-line monitoring

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