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Use of live cell microscopy to follow the temporal regulation of gene expression October 6 th, 2009 Michael Halter, Joe Chalfoun, Antonio Cardone, Benjamin.

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Presentation on theme: "Use of live cell microscopy to follow the temporal regulation of gene expression October 6 th, 2009 Michael Halter, Joe Chalfoun, Antonio Cardone, Benjamin."— Presentation transcript:

1 Use of live cell microscopy to follow the temporal regulation of gene expression October 6 th, 2009 Michael Halter, Joe Chalfoun, Antonio Cardone, Benjamin L. Stottrup, Alex Tona, Alden A. Dima, Anne L. Plant, John T. Elliott Cell Systems Science Group, Biochemical Sciences, CSTL, NIST Michael Halter, Joe Chalfoun, Antonio Cardone, Benjamin L. Stottrup, Alex Tona, Alden A. Dima, Anne L. Plant, John T. Elliott Cell Systems Science Group, Biochemical Sciences, CSTL, NIST fraction of cell cycle fluorescence intensity Copyright © 2000 Cell Press. The Hallmarks of Cancer Douglas Hanahan and Robert A. Weinberg

2 Single cell clones from NIH-3T3 cell population transfected with a destabilized EGFP reporter (PEST sequence, reported ~2 hr half-life) Tenascin-C gene reporter cell lines gene promoter sequenceGFP CONCEPT: GFP is produced when gene is active Full Tenascin-C promoter

3 Tenascin-C (TNC) regulation and role in disease Courtesy of Peter Jones, UCHSC Artery Blocked from Hypertension Normal Artery (Chapados et al., Circulation Research. 2006;99:837.) TNC expression associated with: Mechanics ECM/integrins Proliferation Migration… Tenascin-C F-actin

4 Cell Body Stain GFP Fluorescence GFP Intensity= Transcription+Translation+Folding+Degradation Tenascin-C GFP reporter cells Fluorescence Microscopy GFP fluorescence intensity Cell # GFP intensity distributions are stable in culture (gene activity varies over 3-orders of magnitude?) Langenbach et al, BMC-Biotech, 2006 Flow Cytometry Correlations between spread area and GFP intensity Gene expression responses to different ECM conditions What are the dynamics of cell behavior?

5 Challenges to quantifying live cell images Movie: >62 hours, phase contrast on left, GFP fluorescence on right Challenges Cell segmentationCell segmentation Tracking, mitotosis, edge cells (leave the field)Tracking, mitotosis, edge cells (leave the field) 36 fields @ 15 min intervals

6 Live cell segmentation and tracking

7 Single cell GFP intensities over time indicate tenascin-C regulation is coupled to the cell cycle Normalizing the intensity data and averaging over >30 cells suggests that tenascin-C production is upregulated before division and is directly coupled to cell cycle progression Intensity Fraction of cell cycle Averaging Cell Intensity Profiles Averaging over all cells Time (fraction of cell cycle) Relative GFP fluorescence intensity

8 Applications of quantitative live cell image data Quantify GFP intensities changes with time Examine correlation between phenotype (migrate, division time) and gene expression Understand (stem cell) lineage progression and epigenetic gene regulation

9 Acknowledgements: Live Cell Image Analysis Joe Chalfoun (segmentation, tracking) Marcin Kociolek (segmentation) Alden Dima (segmentation, tracking) Antonio Cardone (segmentation, tracking) Ben Stottrup (manual segmentation, Augsburg College, MN) For further information contact: Michael Halter Biochemical Science Division Gaithersburg, MD 20899 michael.halter@nist.gov

10 Understanding cell state with quantitative live cell imaging Copyright © 2000 Cell Press. The Hallmarks of Cancer Douglas Hanahan and Robert A. Weinberg Gain pathway knowledge: mechanistic understanding of disease identification/validation of cellular biomarkers therapeutic intervention, drug discovery, toxicity

11 Copyright © 2000 Cell Press. The Hallmarks of Cancer Douglas Hanahan and Robert A. Weinberg Single cell analysis Average expression Biological variability Subpopulation information

12 non-transfected NIH3T3’s transfected cells avg=610 +/- 240 avg=5 +/- 7.5 flow cytometry Cell intensities

13 ECM response element strain response element serum response element -655 -250 -180 -57 Prx 1,2 Krox NF  b OCT NF-1 d2 EGFP TATA The Tenascin-C promoter Tenascin-C is an extracellular matrix protein Promoter sequence is ~4kBases with a number of transcription factor binding sites Gene activity is upregulated during development, wound healing and in some cancers and is often correlated with cell spreading and proliferation in vitro

14 LED illumination stability LED intensity measured over 7 days

15 (Chapados et al., Circulation Research. 2006;99:837.) Tenascin-C: an ECM protein TNC levels are high during embryogenesis, but almost absent during normal postnatal life with some basal expression detectable in tendons and ligaments only. Tenascin-C expression is upregulated during inflammation, wound healing, and in many cancers Tenascin-C is thought to have anti- adhesive properties and play a role in signaling The expression of TNC is often correlated with cell spreading

16 Movie: 65 hours, phase contrast on left, GFP on right Quantify GFP intensities from live cells Flow Cytometry GFP fluorescence intensity Cell # What gene regulation (or other?) processes give rise to the stable distribution of GFP intensities with large variability? We use live cell imaging and image analysis to quantify the dynamics of GFP expression driven by the tenascin-C promoter

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