Short term culture of breast cancer tissues to study the activity of the anticancer drug taxol in an intact tumor environment

BACKGROUND: Sensitivity of breast tumors to anticancer drugs depends upon dynamic interactions between epithelial tumor cells and their microenvironment including stromal cells and extracellular matrix. To study drug-sensitivity within different compartments of an individual tumor ex vivo, culture m...

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Autores principales: van der Kuip, Heiko, Mürdter, Thomas E, Sonnenberg, Maike, McClellan, Monika, Gutzeit, Susanne, Gerteis, Andreas, Simon, Wolfgang, Fritz, Peter, Aulitzky, Walter E
Formato: Texto
Lenguaje:English
Publicado: BioMed Central 2006
Materias:
Technical Advance
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC1456977/
https://www.ncbi.nlm.nih.gov/pubmed/16603054
http://dx.doi.org/10.1186/1471-2407-6-86
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author van der Kuip, Heiko
Mürdter, Thomas E
Sonnenberg, Maike
McClellan, Monika
Gutzeit, Susanne
Gerteis, Andreas
Simon, Wolfgang
Fritz, Peter
Aulitzky, Walter E
author_facet van der Kuip, Heiko
Mürdter, Thomas E
Sonnenberg, Maike
McClellan, Monika
Gutzeit, Susanne
Gerteis, Andreas
Simon, Wolfgang
Fritz, Peter
Aulitzky, Walter E
author_sort van der Kuip, Heiko
collection PubMed
description BACKGROUND: Sensitivity of breast tumors to anticancer drugs depends upon dynamic interactions between epithelial tumor cells and their microenvironment including stromal cells and extracellular matrix. To study drug-sensitivity within different compartments of an individual tumor ex vivo, culture models directly established from fresh tumor tissues are absolutely essential. METHODS: We prepared 0.2 mm thick tissue slices from freshly excised tumor samples and cultivated them individually in the presence or absence of taxol for 4 days. To visualize viability, cell death, and expression of surface molecules in different compartments of non-fixed primary breast cancer tissues we established a method based on confocal imaging using mitochondria- and DNA-selective dyes and fluorescent-conjugated antibodies. Proliferation and apoptosis was assessed by immunohistochemistry in sections from paraffin-embedded slices. Overall viability was also analyzed in homogenized tissue slices by a combined ATP/DNA quantification assay. RESULTS: We obtained a mean of 49 tissue slices from 22 breast cancer specimens allowing a wide range of experiments in each individual tumor. In our culture system, cells remained viable and proliferated for at least 4 days within their tissue environment. Viability of tissue slices decreased significantly in the presence of taxol in a dose-dependent manner. A three-color fluorescence viability assay enabled a rapid and authentic estimation of cell viability in the different tumor compartments within non-fixed tissue slices. CONCLUSION: We describe a tissue culture method combined with a novel read out system for both tissue cultivation and rapid assessment of drug efficacy together with the simultaneous identification of different cell types within non-fixed breast cancer tissues. This method has potential significance for studying tumor responses to anticancer drugs in the complex environment of a primary cancer tissue.
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spelling pubmed-14569772006-05-04 Short term culture of breast cancer tissues to study the activity of the anticancer drug taxol in an intact tumor environment van der Kuip, Heiko Mürdter, Thomas E Sonnenberg, Maike McClellan, Monika Gutzeit, Susanne Gerteis, Andreas Simon, Wolfgang Fritz, Peter Aulitzky, Walter E BMC Cancer Technical Advance BACKGROUND: Sensitivity of breast tumors to anticancer drugs depends upon dynamic interactions between epithelial tumor cells and their microenvironment including stromal cells and extracellular matrix. To study drug-sensitivity within different compartments of an individual tumor ex vivo, culture models directly established from fresh tumor tissues are absolutely essential. METHODS: We prepared 0.2 mm thick tissue slices from freshly excised tumor samples and cultivated them individually in the presence or absence of taxol for 4 days. To visualize viability, cell death, and expression of surface molecules in different compartments of non-fixed primary breast cancer tissues we established a method based on confocal imaging using mitochondria- and DNA-selective dyes and fluorescent-conjugated antibodies. Proliferation and apoptosis was assessed by immunohistochemistry in sections from paraffin-embedded slices. Overall viability was also analyzed in homogenized tissue slices by a combined ATP/DNA quantification assay. RESULTS: We obtained a mean of 49 tissue slices from 22 breast cancer specimens allowing a wide range of experiments in each individual tumor. In our culture system, cells remained viable and proliferated for at least 4 days within their tissue environment. Viability of tissue slices decreased significantly in the presence of taxol in a dose-dependent manner. A three-color fluorescence viability assay enabled a rapid and authentic estimation of cell viability in the different tumor compartments within non-fixed tissue slices. CONCLUSION: We describe a tissue culture method combined with a novel read out system for both tissue cultivation and rapid assessment of drug efficacy together with the simultaneous identification of different cell types within non-fixed breast cancer tissues. This method has potential significance for studying tumor responses to anticancer drugs in the complex environment of a primary cancer tissue. BioMed Central 2006-04-07 /pmc/articles/PMC1456977/ /pubmed/16603054 http://dx.doi.org/10.1186/1471-2407-6-86 Text en Copyright © 2006 van der Kuip et al; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License ( (http://creativecommons.org/licenses/by/2.0) ), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Technical Advance
van der Kuip, Heiko
Mürdter, Thomas E
Sonnenberg, Maike
McClellan, Monika
Gutzeit, Susanne
Gerteis, Andreas
Simon, Wolfgang
Fritz, Peter
Aulitzky, Walter E
Short term culture of breast cancer tissues to study the activity of the anticancer drug taxol in an intact tumor environment
title Short term culture of breast cancer tissues to study the activity of the anticancer drug taxol in an intact tumor environment
title_full Short term culture of breast cancer tissues to study the activity of the anticancer drug taxol in an intact tumor environment
title_fullStr Short term culture of breast cancer tissues to study the activity of the anticancer drug taxol in an intact tumor environment
title_full_unstemmed Short term culture of breast cancer tissues to study the activity of the anticancer drug taxol in an intact tumor environment
title_short Short term culture of breast cancer tissues to study the activity of the anticancer drug taxol in an intact tumor environment
title_sort short term culture of breast cancer tissues to study the activity of the anticancer drug taxol in an intact tumor environment
topic Technical Advance
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC1456977/
https://www.ncbi.nlm.nih.gov/pubmed/16603054
http://dx.doi.org/10.1186/1471-2407-6-86
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