Using Cell-ID 1.4 with R for microscope-based cytometry

A. CHERNOMORETZ; A. BUSH; R. YU; A. GORDON; A. COLMNAN-LERNER

Current Protocols in Molecular Biology

Wiley Interscience

Año: 2008 vol. 84 p. 14181 - 141827

1934-3639

This unit describes a method for quantifying various cellular parameters (e.g., volume, total and subcellular fluorescence localization) from sets of microscope images of individual cells. It includes procedures for tracking cells over time. One purposefully defocused transmission image (sometimes referred to as bright-field or BF) is acquired to locate each cell. Fluorescent images (one for each of the color channels to be analyzed) are then acquired by conventional wide-field epifluorescence or confocal microscopy. This method uses the image processing capabilities of Cell-ID (Gordon et al., 2007) and data analysis by the statistical programming framework R (R-Development-Team, 2008), which we have supplemented with a package tailored to analyze Cell-ID output. Both programs are open-source software packages.