Workflow for high-content, individual cell quantification of fluorescent markers from universal microscope data, supported by open source software

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Workflow for high-content, individual cell quantification of fluorescent markers from universal microscope data, supported by open source software

Stockwell, SR; Mittnacht, S; (2014) Workflow for high-content, individual cell quantification of fluorescent markers from universal microscope data, supported by open source software. Journal of Visualized Experiments (94) , Article e51882. 10.3791/51882. Green open access

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Abstract

Advances in understanding the control mechanisms governing the behavior of cells in adherent mammalian tissue culture models are becoming increasingly dependent on modes of single-cell analysis. Methods which deliver composite data reflecting the mean values of biomarkers from cell populations risk losing subpopulation dynamics that reflect the heterogeneity of the studied biological system. In keeping with this, traditional approaches are being replaced by, or supported with, more sophisticated forms of cellular assay developed to allow assessment by high-content microscopy. These assays potentially generate large numbers of images of fluorescent biomarkers, which enabled by accompanying proprietary software packages, allows for multi-parametric measurements per cell. However, the relatively high capital costs and overspecialization of many of these devices have prevented their accessibility to many investigators. Described here is a universally applicable workflow for the quantification of multiple fluorescent marker intensities from specific subcellular regions of individual cells suitable for use with images from most fluorescent microscopes. Key to this workflow is the implementation of the freely available Cell Profiler software(1) to distinguish individual cells in these images, segment them into defined subcellular regions and deliver fluorescence marker intensity values specific to these regions. The extraction of individual cell intensity values from image data is the central purpose of this workflow and will be illustrated with the analysis of control data from a siRNA screen for G1 checkpoint regulators in adherent human cells. However, the workflow presented here can be applied to analysis of data from other means of cell perturbation (e.g., compound screens) and other forms of fluorescence based cellular markers and thus should be useful for a wide range of laboratories.

Type:	Article
Title:	Workflow for high-content, individual cell quantification of fluorescent markers from universal microscope data, supported by open source software
Location:	United States
Open access status:	An open access version is available from UCL Discovery
DOI:	10.3791/51882
Publisher version:	http://dx.doi.org/10.3791/51882
Language:	English
Additional information:	Copyright © 2014 Creative Commons Attribution-NonCommercial License
UCL classification:	UCL UCL > Provost and Vice Provost Offices UCL > Provost and Vice Provost Offices > School of Life and Medical Sciences UCL > Provost and Vice Provost Offices > School of Life and Medical Sciences > Faculty of Medical Sciences UCL > Provost and Vice Provost Offices > School of Life and Medical Sciences > Faculty of Medical Sciences > Cancer Institute UCL > Provost and Vice Provost Offices > School of Life and Medical Sciences > Faculty of Medical Sciences > Cancer Institute > Research Department of Cancer Bio
URI:	https://discovery.ucl.ac.uk/id/eprint/1468474

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