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Article type: Research Article
Authors: Kimmig, Rainer; | Wimberger, Pauline | Kapsner, Thomas | Hillemanns, Peter
Affiliations: Department of Obstetrics and Gynecology, Klinikum Grosshadern, Ludwig‐Maximilians‐University, Munich, Germany | Department of Medical Informatics, Biometry and Epidemiology (IBE), Ludwig‐Maximilians‐University, Marchioninistr. 15, D‐81377 Munich, Germany
Note: [] Corresponding author: Rainer Kimmig, MD, Klinik und Poliklinik für Frauenheilkunde und Geburtshilfe der Universität München – Großhadern, D‐81377 Munich, Germany. Tel.: + 49 89 7095 2851/2858; Fax: + 49 89 7095 5851; E‐mail: [email protected]‐muenchen.de.
Abstract: Flow cytometric assessment of DNA‐ploidy and S‐phase fraction in malignant tumors is compromised by the heterogeneity of cell subpopulations derived from the malignant and surrounding connective tissue, e.g., tumor, stromal and inflammatory cells. To evaluate the effect on quality of DNA cell cycle analysis and determination of DNA ploidy, cytokeratin labeling of epithelial cells was used for tumor cell enrichment in breast, ovarian, cervical and endometrial cancer prior to DNA analysis. In a prospective study, tumor cell subpopulations of 620 malignant tumors were labeled by a FITC‐conjugated cytokeratin antibody (CK 5, 6, CK18 and CK 5, 6, 8 and CK 17, respectively) prior to flow cytometric cell cycle analysis. Compared to total cell analysis, detection rate of DNA‐aneuploid tumors following cytokeratin labeling was increased from 62% to 76.5% in breast cancer, from 68% to 77% in ovarian cancer, from 60% to 80% in cervical cancer and from 30% to 53% in endometrial cancer. Predominantly in DNA‐diploid tumors, a significantly improved detection of S‐phase fraction of the tumor cells was shown due to the elimination of contaminating nonproliferating “normal cells”. S‐phase fraction following tumor cell enrichment was increased by 10% (mean) following cytokeratin staining in ovarian and endometrial cancer, by 30% in breast cancer and even by 70% in cervical cancer compared to total cell analysis. Thus, diagnostic accuracy of DNA‐analysis was enhanced by cytokeratin labeling of tumor cells for all tumor entities investigated.
Keywords: Flow cytometry, DNA cell cycle analysis, cytokeratin
Journal: Analytical Cellular Pathology, vol. 22, no. 3, pp. 165-178, 2001
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