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Measurements of the DNA double-strand break response

Sammanfattning
Radiotherapy and some chemotherapeutic drugs kill cancer cells by induction of the extremely toxic DNA double-strand breaks (DSBs). Measurements of the DSB response in patients during therapy could allow personalized dosing to improve tumor response and minimize side effects. DSBs induce a strong cellular response via phosphorylation of H2AX, P-H2AX and the formation of foci. P-H2AX can be measured by flow cytometry or counted in separate cell nuclei by immunofluorescence microscopy. The overall aim of my research has been to develop and validate methods to measure P-H2AX in mononuclear cells from cancer patients undergoing radiotherapy. Initially, we wanted to characterize DNA damage induced by the chemotherapeutic drug etoposide that induces TopoII-linked DSBs and to test its ability to activate the P-H2AX response using a flow cytometry-based P-H2AX assay. We found that only 0.3% of etoposide-induced DSBs activated the H2AX response and toxicity. We concluded that the P-H2AX response was a good measure of the toxic effects of etoposide. Next, we wanted to optimize the flow cytometry assay for mononuclear cells from cancer patients undergoing radiation therapy. The P-H2AX response was measured before and after 5Gy pelvic irradiation and in in vitro-irradiated controls. We found a fraction of cells with high P-H2AX signals that corresponded to the 5Gy in vitro-irradiated blood controls. This study indicated that flow cytometry may be well suited for measurements of the P-H2AX response in mononuclear cells following local radiotherapy. To be able to implement the P-H2AX assay in clinical practice and use it in relation to clinical outcome and side effects we have also developed stable and reliable calibrators based on phosphopeptide-coated beads and fixed cells. Using these calibrators it could be possible to use the P-H2AX flow cytometry assay in the clinic in a controlled manner. Finally, using immunostaining in solution before cells are mounted on microscopic slides for quantification of single P-H2AX foci by immunofluorescence, we have the possibility to analyze 16 patient samples within few hours, which makes this method suitable for clinical use.
Delarbeten
I. Numerical analysis of etoposide induced DNA breaks. Muslimović A, Nyström S, Gao Y, Hammarsten O. ::PMID::19516899
 
II. An optimized method for measurement of gamma-H2AX in blood mononuclear and cultured cells. Muslimovic A, Ismail IH, Gao Y, Hammarsten O. ::PMID::18600224
 
III. Calibrators for clinical measurements of phosphorylated H2AX in patient cells by flow cytometry. Muslimovic A, Johansson P, Ruetschi U, Hammarsten O. Submitted manuscript.
 
IV. In-solution staining and arraying method for the immunofluorescence detection of γH2AX foci optimized for clinical applications. Johansson P, Muslimovic A, Hultborn R, Fernström E, Hammarsten O. ::PMID:: 21906040
 
Examinationsnivå
Doctor of Philosophy (Medicine)
Universitet
University of Gothenburg. Sahlgrenska Academy
Institution
Institute of Biomedicine. Department of Clinical Chemistry and Transfusion Medicine
Disputation
Fredagen den 19 oktober 2012, kl. 13.00, Hörsal Arvid Carlsson, Academicum, Medicinaregatan 3, Göteborg
Datum för disputation
2012-10-19
E-post
aida.muslimovic@clinchem.gu.se
URL:
http://hdl.handle.net/2077/30410
Samlingar
  • Doctoral Theses / Doktorsavhandlingar Institutionen för biomedicin
  • Doctoral Theses from Sahlgrenska Academy
  • Doctoral Theses from University of Gothenburg / Doktorsavhandlingar från Göteborgs universitet
Fil(er)
Thesis frame (3.898Mb)
Cover (2.280Mb)
Abstract (1.266Mb)
Datum
2012-09-25
Författare
Muslimovic, Aida
Nyckelord
DSB response
cancer patients
H2AX phosphorylation
Publikationstyp
Doctoral thesis
ISBN
978-91-628-8504-5
Språk
eng
Metadata
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