Atomic force microscopy as analytical tool to study physico-mechanical properties of intestinal cells

Christa Schimpel; Oliver Werzer; Eleonore Fröhlich; Gerd Leitinger; Markus Absenger-Novak; Birgit Teubl; Andreas Zimmer; Eva Roblegg

doi:10.3762/bjnano.6.151

Atomic force microscopy as analytical tool to study physico-mechanical properties of intestinal cells

Beilstein J Nanotechnol. 2015 Jul 6:6:1457-66. doi: 10.3762/bjnano.6.151. eCollection 2015.

Authors

Christa Schimpel¹, Oliver Werzer¹, Eleonore Fröhlich², Gerd Leitinger³, Markus Absenger-Novak², Birgit Teubl¹, Andreas Zimmer¹, Eva Roblegg⁴

Affiliations

¹ Institute of Pharmaceutical Sciences, Department of Pharmaceutical Technology, NAWI Graz, Karl-Franzens-University of Graz, BioTechMed-Graz, Austria.
² Medical University of Graz, Center for Medical Research, BioTechMed-Graz, Austria.
³ Research Unit Electron Microscopic Techniques, Institute of Cell Biology, Histology and Embryology, Center for Medical Research, Medical University of Graz, BioTechMed-Graz, Austria.
⁴ Institute of Pharmaceutical Sciences, Department of Pharmaceutical Technology, NAWI Graz, Karl-Franzens-University of Graz, BioTechMed-Graz, Austria ; Research Center Pharmaceutical Engineering GmbH, Graz, Austria.

Abstract

The small intestine is a complex system that carries out various functions. The main function of enterocytes is absorption of nutrients, whereas membranous cells (M cells) are responsible for delivering antigens/foreign substances to the mucosal lymphoid tissues. However, to get a fundamental understanding of how cellular structures contribute to physiological processes, precise knowledge about surface morphologies, cytoskeleton organizations and biomechanical properties is necessary. Atomic force microscopy (AFM) was used here as a powerful tool to study surface topographies of Caco-2 cells and M cells. Furthermore, cell elasticity (i.e., the mechanical response of a cell on a tip indentation), was elucidated by force curve measurements. Besides elasticity, adhesion was evaluated by recording the attraction and repulsion forces between the tip and the cell surface. Organization of F-actin networks were investigated via phalloidin labeling and visualization was performed with confocal laser scanning fluorescence microscopy (CLSM) and scanning electron microscopy (SEM). The results of these various experimental techniques revealed significant differences in the cytoskeleton/microvilli arrangements and F-actin organization. Caco-2 cells displayed densely packed F-actin bundles covering the entire cell surface, indicating the formation of a well-differentiated brush border. In contrast, in M cells actins were arranged as short and/or truncated thin villi, only available at the cell edge. The elasticity of M cells was 1.7-fold higher compared to Caco-2 cells and increased significantly from the cell periphery to the nuclear region. Since elasticity can be directly linked to cell adhesion, M cells showed higher adhesion forces than Caco-2 cells. The combination of distinct experimental techniques shows that morphological differences between Caco-2 cells and M cells correlate with mechanical cell properties and provide useful information to understand physiological processes/mechanisms in the small intestine.

Keywords: Caco-2 cells; M cells; atomic force microscopy; elasticity; mechanical properties.