PUBLICATION
Extracting fluorescent reporter time courses of cell lineages from high-throughput microscopy at low temporal resolution
- Authors
- Downey, M.J., Jeziorska, D.M., Ott, S., Tamai, T.K., Koentges, G., Vance, K.W., and Bretschneider, T.
- ID
- ZDB-PUB-120106-22
- Date
- 2011
- Source
- PLoS One 6(12): e27886 (Journal)
- Registered Authors
- Tamai, Takako Katherine
- Keywords
- none
- MeSH Terms
-
- Animals
- Biomarkers/metabolism
- Cell Division
- Cell Line
- Cell Lineage*
- Cell Nucleus/metabolism
- Cell Tracking
- Fluorescence
- Genes, Reporter*
- Green Fluorescent Proteins/metabolism
- High-Throughput Screening Assays/methods*
- Imaging, Three-Dimensional
- Mice
- Microscopy/methods*
- Time Factors
- Zebrafish/metabolism
- PubMed
- 22194797 Full text @ PLoS One
Citation
Downey, M.J., Jeziorska, D.M., Ott, S., Tamai, T.K., Koentges, G., Vance, K.W., and Bretschneider, T. (2011) Extracting fluorescent reporter time courses of cell lineages from high-throughput microscopy at low temporal resolution. PLoS One. 6(12):e27886.
Abstract
The extraction of fluorescence time course data is a major bottleneck in high-throughput live-cell microscopy. Here we present an extendible framework based on the open-source image analysis software ImageJ, which aims in particular at analyzing the expression of fluorescent reporters through cell divisions. The ability to track individual cell lineages is essential for the analysis of gene regulatory factors involved in the control of cell fate and identity decisions. In our approach, cell nuclei are identified using Hoechst, and a characteristic drop in Hoechst fluorescence helps to detect dividing cells. We first compare the efficiency and accuracy of different segmentation methods and then present a statistical scoring algorithm for cell tracking, which draws on the combination of various features, such as nuclear intensity, area or shape, and importantly, dynamic changes thereof. Principal component analysis is used to determine the most significant features, and a global parameter search is performed to determine the weighting of individual features. Our algorithm has been optimized to cope with large cell movements, and we were able to semi-automatically extract cell trajectories across three cell generations. Based on the MTrackJ plugin for ImageJ, we have developed tools to efficiently validate tracks and manually correct them by connecting broken trajectories and reassigning falsely connected cell positions. A gold standard consisting of two time-series with 15,000 validated positions will be released as a valuable resource for benchmarking. We demonstrate how our method can be applied to analyze fluorescence distributions generated from mouse stem cells transfected with reporter constructs containing transcriptional control elements of the Msx1 gene, a regulator of pluripotency, in mother and daughter cells. Furthermore, we show by tracking zebrafish PAC2 cells expressing FUCCI cell cycle markers, our framework can be easily adapted to different cell types and fluorescent markers.
Genes / Markers
Expression
Phenotype
Mutations / Transgenics
Human Disease / Model
Sequence Targeting Reagents
Fish
Orthology
Engineered Foreign Genes
Mapping