gms | German Medical Science

64. Jahrestagung der Deutschen Gesellschaft für Neurochirurgie (DGNC)

Deutsche Gesellschaft für Neurochirurgie (DGNC) e. V.

26. - 29. Mai 2013, Düsseldorf

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Inhibition of mitotic Aurora B led to disturbed chromosomal segregation and mitotic catastrophe in glioma cells irrespective of 53 status

Meeting Abstract

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  • Ralf Wiedemuth - Klinik und Poliklinik für Neurochirurgie, Universitätsklinikum Carl Gustav Carus, TU Dresden
  • Gabriele Schackert - Klinik und Poliklinik für Neurochirurgie, Universitätsklinikum Carl Gustav Carus, TU Dresden
  • Achim Temme - Klinik und Poliklinik für Neurochirurgie, Universitätsklinikum Carl Gustav Carus, TU Dresden

Deutsche Gesellschaft für Neurochirurgie. 64. Jahrestagung der Deutschen Gesellschaft für Neurochirurgie (DGNC). Düsseldorf, 26.-29.05.2013. Düsseldorf: German Medical Science GMS Publishing House; 2013. DocP 145

doi: 10.3205/13dgnc562, urn:nbn:de:0183-13dgnc5625

Veröffentlicht: 21. Mai 2013

© 2013 Wiedemuth et al.
Dieser Artikel ist ein Open Access-Artikel und steht unter den Creative Commons Lizenzbedingungen (http://creativecommons.org/licenses/by-nc-nd/3.0/deed.de). Er darf vervielfältigt, verbreitet und öffentlich zugänglich gemacht werden, vorausgesetzt dass Autor und Quelle genannt werden.

Gliederung

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Objective: Inhibition of Aurora kinase B by RNA interference or small chemical compounds has been shown to block solid tumor growth in many different tumor entities even in gliomas. In this study we sought to elucidate the role of the tumor suppressor protein p53 in the cell cycle regulation and chromosomal segregation of U87-MG glioma cells treated with the specific Aurora B inhibitor Barasertib (AZD1152-HQPA).

Method: The tumor suppressor p53 was stably knocked down in U87-MG glioma cells by a retroviral vector encoding the small hairpin shRNA targeting p53. Cells were either incubated with Aurora B Inhibitor (AZD1152-HQPA) or DMSO and subjected to cell cycle analysis, apoptosis assays, Western blot analysis, flow cytometry and proliferation analysis.

Results: Aurora B inhibition resulted in wild type and p53-deficient (shp53) U87-MG cells in a significant increase in the amount of polyploid cells with defective mitosis compared to control cells (DMSO). However, an induction of p21waf/cip on the steady state protein level was only observed in U87-MG wild type cells expressing functional p53. Determination of proliferation by BrdU-incorporation analysis and clonal survival experiments indicated an impaired cell growth of wild type and p53-deficient U87-MG cells after Barasertib treatment. But even polyploid cells irrespective of p53 wt expression or p53-deficiency showed BrdU incorporation in cells having a DNA content >4N indicating further intrinsic cell cycle progression. SubG1 analysis revealed a twofold increase in the fraction of dead cells in those cells treated with Aurora B inhibitor compared to controls. Yet, western blot analysis showed no increase in cleaved caspase 3, suggesting that cell death caused by aurora B inhibition occurs rather by mitotic catastrophe than organized apoptosis.

Conclusions: Our results suggest that Aurora B inhibition severely affects proliferation and survival of glioma cells irrespective of p53 status. Therapies targeting Aurora B might represent a promising avenue for adjuvant local treatment of secondary and primary glioblastoma.