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Abstract
High-content screening (HCS) uses microscopy images to generate phenotypic profiles of cell morphological data in high-dimensional feature space. While HCS provides detailed cytological information at single-cell resolution, these complex datasets are usually aggregated into summary statistics that do not leverage patterns of biological variability within cell populations. Here we present a broad-spectrum HCS analysis system that measures image-based cell features from 10 cellular compartments across multiple assay panels. We introduce quality control measures and statistical strategies to streamline and harmonize the data analysis workflow, including positional and plate effect detection, biological replicates analysis and feature reduction. We also demonstrate that the Wasserstein distance metric is superior over other measures to detect differences between cell feature distributions. With this workflow, we define per-dose phenotypic fingerprints for 65 mechanistically diverse compounds, provide phenotypic path visualizations for each compound and classify compounds into different activity groups.
A high-content screening assay based on a comprehensive set of cytological features, together with a robust statistical analysis workflow for profiling broad-based cellular phenotypic responses to small molecules or genetic perturbations.
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1 New York University Abu Dhabi, Center for Genomics and Systems Biology, Abu Dhabi, UAE (GRID:grid.440573.1) (ISNI:0000 0004 1755 5934)
2 New York University Abu Dhabi, Center for Genomics and Systems Biology, Abu Dhabi, UAE (GRID:grid.440573.1) (ISNI:0000 0004 1755 5934); New York University, Department of Biology and Center for Genomics and Systems Biology, New York, USA (GRID:grid.137628.9) (ISNI:0000 0004 1936 8753)