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Imaging of keratin dynamics during the cell cycle and in response to phosphatase inhibition

Windoffer R, Leube RE, 2004

The organization of the keratin intermediate filament cytoskeleton is closely linked to epithelial function. To study keratin network plasticity and its regulation at different levels, tools are needed to localize and measure local network dynamics. In this paper, we present image analysis methods designed to determine the speed and direction of keratin filament motion and to identify locations of keratin filament polymerization and depolymerization at subcellular resolution. Using these methods, we have analyzed time-lapse fluorescence recordings of fluorescent keratin 13 in human vulva carcinoma-derived A431 cells.


The fluorescent keratins integrated into the endogenous keratin cytoskeleton, and thereby served as reliable markers of keratin dynamics. We found that increased times after seeding correlated with down-regulation of inward-directed keratin filament movement. Bulk flow analyses further revealed that keratin filament polymerization in the cell periphery and keratin depolymerization in the more central cytoplasm were both reduced. Treating these cells and other human keratinocyte-derived cells with EGF reversed all these processes within a few minutes, coinciding with increased keratin phosphorylation. These results highlight the value of the newly developed tools for identifying modulators of keratin filament network dynamics and characterizing their mode of action, which, in turn, contributes to understanding the close link between keratin filament network plasticity and epithelial physiology.

Time-lapse recording (30 s intervals) of the epifluorescence in the periphery of a PK18-5 cell producing HK18-YFP. Note the continuous inward flow of fluorescent material. The LUT was adjusted in the central square area to highlight details of fluorescence changes.

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Simultaneous fluorescence recording of the distribution of histone H1-EGFP and HK13-EGFP in a dividing AK13-1 cell during cytokinesis. The projection images were obtained from recordings in multiple focal planes and were taken every 2.27 min.


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Recording of keratin HK13-EGFP fluorescence distribution in a single focal plane of an AK13-1 cell (middle) that has entered mitosis. Recording intervals, 2.5 min..

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Projection views of fluorescence images that were obtained in five focal planes of a mitotic AK13-1 cell (middle) synthesizing HK13-EGFP fusions. Recording intervals, 2.5 min.


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Time series of 3D-reconstructions (surface views as anaglyphs) derived from a live cell fluorescence-recording of an AK13-1 cell at the onset of mitosis depicting the distribution of HK13-EGFP hybrids.
The image series should be viewed with red-green glasses for 3D-visualization,. Recording intervals, 2.5 min.

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3D-reconstructions (voxel-reconstructions as anaglyphs) of a time series that was recorded at 2.5 min intervals in an AK13-1 cell upon entry into mitosis delineating the distribution of HK13-EGFP chimeras. The image series should be viewed with red-green glasses for 3D-visualization.


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Surface view of 3D-reconstructions derived from time-lapse fluorescence image stacks that were recorded at 1.6 min intervals in an AK13-1 cell at the end of mitosis depicting altering patterns of HK13-EGFP distribution.

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Time-lapse fluorescence image series (2 min recording intervals) taken during a FRAP experiment that was performed in a hepatocellular PK18-5 cell producing HK18-YFP chimeras.


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