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Quantitative cytofluorimetric determination of cell membrane-associated large tumor antigen on SV40-transformed cells.

作者信息

Hess R D, Kuther M, Haessler C, Paetzold S, Braun D G, Brandner G

机构信息

Abteilung Virologie, Albert-Ludwigs-Universität, Freiburg, Germany.

出版信息

Cytometry. 1995 May 1;20(1):81-5. doi: 10.1002/cyto.990200112.

Abstract

The aim of this study was to quantitate the number of cell membrane-located SV40 large tumor antigen (large T) molecules of SV40-transformed cell lines by cytofluorimetric analysis. Five different SV40-transformed cell lines were labelled by either a biotin- or a fluorescein-conjugated monoclonal antibody, PAb1605, which is specific for the large T carboxyterminus. The conjugated-antibody fluorescence signals of the stained large T molecules of transformed cells were measured via cytofluorimetry. Comparison of the fluorescence signals of calibrated beads bearing a known number of fluorescein molecules to the signals of conjugated PAb1605 antibodies bound on microbeads to a defined number of IgG binding sites made it possible to determine the number of antibody-accessible large T molecules per SV40-transformed cell. The numbers (x10(-4)) found per cell were 1.0 (ELONA, hamster), 3.0 (VLM, mouse), 3.5 (mKSA, mouse), 11 (C57SV, mouse), and 5.5 (SV80, human), respectively. Thus, the technique described allows a precise quantitation of surface-exposed, antibody-accessible viral antigen expression.

摘要

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