Flow cytometric analysis of in vivo polyamine deprivation in Lewis lung carcinoma (3LL) cells using the monoclonal antibody SPM8‐2

Flow cytometric analysis of in vivo polyamine deprivation in Lewis lung carcinoma (3LL) cells using the monoclonal antibody SPM8‐2

It has previously been shown that the monoclonal antibody SPM8‐2 recognizes free spermine and spermidine as well as polyamines bound by an amide bond. In the present work it is demonstrated that this antibody also interacts with spermidine, spermine, and to a lesser extent N1‐ and N8‐acetyl spermidi...

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Veröffentlicht in:Cytometry (New York, N.Y.) N.Y.), 1997-03, Vol.27 (3), p.255-261
Hauptverfasser: Delcros, Jean‐Guy, Lœuillet, Laurence, Chamaillard, Laura, Royou, Anne, Bouillé, Nathalie, Seiler, Nikolaus, Moulinoux, Jacques‐Philippe
Format: Artikel
Sprache:eng
Schlagworte:
Animals
Antibodies, Monoclonal - immunology
Antibodies, Monoclonal - metabolism
Antibodies, Monoclonal - pharmacology
antipolyamine antibody
Carcinoma, Lewis Lung - immunology
Carcinoma, Lewis Lung - metabolism
Cell Separation
Enzyme-Linked Immunosorbent Assay
flow cytometry
Flow Cytometry - methods
Mice
Mice, Inbred C57BL
Mice, Inbred DBA
polyamine
Polyamines - chemistry
Polyamines - immunology
Polyamines - metabolism
Tumor Cells, Cultured
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Zusammenfassung:It has previously been shown that the monoclonal antibody SPM8‐2 recognizes free spermine and spermidine as well as polyamines bound by an amide bond. In the present work it is demonstrated that this antibody also interacts with spermidine, spermine, and to a lesser extent N1‐ and N8‐acetyl spermidine in an ELISA test where the polyamines are bound by reaction with formaldehyde. 3LL Lewis lung carcinoma cells from tumor‐grafted mice were labeled with fluorescein‐conjugated monoclonal antibody SPM8‐2 and analyzed by flow cytometry. Both viable cells and formaldehyde‐fixed and subsequently permeabilized cells showed fluorescent staining. However, most polyamines present in the cells are not directly available for antibody binding. Treatment of fixed cells with DNase or RNase greatly increased fluorescent staining, suggesting that some polyamines are co‐localized with DNA and RNA. Antibody labeling of the cells was prevented by addition of free spermine. 3LL cells from tumors of mice treated by a polyamine depleting regimen had decreased intracellular spermidine levels and bound less antibody when compared to untreated controls. After digestion with RNase, the cells from treated mice bound considerably less fluorescent antibody than tumor cells from untreated mice, while their RNA content was similar. In contrast, fluorescent staining after DNase digestion was only slightly affected by the treatment with a polyamine depleting regimen. This suggests that the pools of polyamines which are co‐localized with RNA are depleted more readily than those associated with DNA. Since only a small proportion of the intracellular polyamines is accessible to the bulky antibodies, treatment with hydrolytic enzymes (DNase, RNase) is necessary to reveal specific compartments of the polyamines and to demonstrate qualitative and semiquantitative differences of their distribution within cells. Cytometry 27:255–261, 1997. © 1997 Wiley‐Liss, Inc.
ISSN:0196-4763
1097-0320
DOI:10.1002/(SICI)1097-0320(19970301)27:3<255::AID-CYTO7>3.0.CO;2-D