Spectral analysis of doxorubicin accumulation and the indirect quantification of its DNA intercalation
Language English Country Netherlands Media print-electronic
Document type Journal Article, Research Support, Non-U.S. Gov't
PubMed
20638475
DOI
10.1016/j.ejpb.2010.07.008
PII: S0939-6411(10)00191-8
Knihovny.cz E-resources
- MeSH
- Cell Nucleus metabolism MeSH
- 3T3 Cells MeSH
- DNA metabolism MeSH
- Doxorubicin analogs & derivatives metabolism pharmacology MeSH
- Spectrometry, Fluorescence MeSH
- Hydrophobic and Hydrophilic Interactions MeSH
- Drug Delivery Systems * MeSH
- Humans MeSH
- Lymphoma, T-Cell drug therapy metabolism MeSH
- Mice MeSH
- Tumor Cells, Cultured MeSH
- Polymers metabolism MeSH
- Antibiotics, Antineoplastic metabolism pharmacology MeSH
- Flow Cytometry MeSH
- Animals MeSH
- Check Tag
- Humans MeSH
- Mice MeSH
- Animals MeSH
- Publication type
- Journal Article MeSH
- Research Support, Non-U.S. Gov't MeSH
- Names of Substances
- 7,8-dehydro-9,10-desacetyldoxorubicinone MeSH Browser
- DNA MeSH
- Doxorubicin MeSH
- Polymers MeSH
- Antibiotics, Antineoplastic MeSH
There is a wide range of techniques utilizing fluorescence of doxorubicin (Dox) commonly used for analysis of intracellular accumulation and destiny of various drug delivery systems containing this anthracycline antibiotic. Unfortunately, results of these studies can be significantly influenced by doxorubicin degradation product, 7,8-dehydro-9,10-desacetyldoxorubicinone (D*) forming spontaneously in aqueous environment, whose fluorescence strongly interfere with that of doxorubicin. Here, we define two microscopy techniques enabling to distinguish and separate Dox and D* emission based either on its spectral properties or on fluorescence lifetime analysis. To analyze influx and nuclear accumulation of Dox (free or polymer-bound) by flow cytometry, we propose using an indirect method based on its DNA intercalation competition with Hoechst 33342 rather than a direct measurement of doxorubicin fluorescence inside the cells.
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