Integrin-based meningioma cell migration is promoted by photon but not by carbon-ion irradiation

Purpose Sublethal doses of photon irradiation (IR) are suspected to increase tumor cell migration and support locoregional recurrence of disease, which has already been shown in other cell lines. This manuscript describes the effect of photon and carbon-ion IR on WHO class I meningioma cell migratio...

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Veröffentlicht in:Strahlentherapie und Onkologie 2015-04, Vol.191 (4), p.347-355
Hauptverfasser: Simon, Florian, Dittmar, Jan-Oliver, Brons, Stephan, Orschiedt, Lena, Urbschat, Steffi, Weber, Klaus-Josef, Debus, Jürgen, Combs, Stephanie E., Rieken, Stefan
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Sprache:eng
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Zusammenfassung:Purpose Sublethal doses of photon irradiation (IR) are suspected to increase tumor cell migration and support locoregional recurrence of disease, which has already been shown in other cell lines. This manuscript describes the effect of photon and carbon-ion IR on WHO class I meningioma cell migration and provides an approach to the underlying cellular mechanisms. Materials and methods Meningioma cells were gained operatively at the university hospital in Homburg/Saar, Germany. For migration, membranes (8-µm pore sizes) were coated with collagen I, with collagen IV, and with fibronectin. Cells were analyzed in migration experiments with or without serum stimulation, with or without photon and carbon IR 24 h prior to experiments, and with or without integrin antibodies. Fluorescence-activated cell sorting (FACS) analyses of the integrins ανβ 1 , ανβ 3 , and ανβ 5 were performed without IR and 6, 12 and 24 h after IR. Enzyme-linked immunosorbent assay (ELISA) analyses of matrix metalloproteinases (MMP)-2 and MMP-9 were realized with and without IR after cells were cultured on collagen I, collagen IV, or fibronectin for 24 h. Cells and supernatants for FACS and ELISA were stored at − 18 °C. The significance level was set at 5 % using both Student’s t test and two-way ANOVA. Results Migration of meningioma cells was serum-inducible ( p  
ISSN:0179-7158
1439-099X
DOI:10.1007/s00066-014-0778-y