| Literature DB >> 27341785 |
Alberto Moreno-Cencerrado1, Jagoba Iturri1, Ilaria Pecorari2, Maria D M Vivanco3, Orfeo Sbaizero2, José L Toca-Herrera1.
Abstract
Cell adhesion forces are typically a mixture of specific and nonspecific cell-substrate and cell-cell interactions. In order to resolve these phenomena, Atomic Force Microscopy appears as a powerful device which can measure cell parameters by means of manipulation of single cells. This method, commonly known as cell-probe force spectroscopy, allows us to control the force applied, the area of interest, the approach/retracting speed, the force rate, and the time of interaction. Here, we developed a novel approach for in situ cantilever cell capturing and measurement of specific cell interactions. In particular, we present a new setup consisting of two different half-surfaces coated either with recrystallized SbpA bacterial cell surface layer proteins (S-layers) or integrin binding Fibronectin, on which MCF-7 breast cancer cells are incubated. The presence of a clear physical boundary between both surfaces benefits for a quick detection of the region under analysis. Thus, quantitative results about SbpA-cell and Fibronectin-cell adhesion forces as a function of the contact time are described. Additionally, the importance of the cell spreading in cell-cell interactions has been studied for surfaces coated with two different Fibronectin concentrations: 20 μg/mL (FN20) and 100 μg/mL (FN100), which impact the number of substrate receptors. Microsc. Res. Tech. 80:124-130, 2017.Entities:
Keywords: S-layer proteins; atomic force microscopy; cell adhesion; force spectroscopy; single-cell probe
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Year: 2016 PMID: 27341785 DOI: 10.1002/jemt.22706
Source DB: PubMed Journal: Microsc Res Tech ISSN: 1059-910X Impact factor: 2.769