Your search keyword '"Pine PS"' showing total 2 results

1. A semiautomated fluorescence-based cell-to-cell fusion assay for gp120-gp41 and CD4 expressing cells.

Author

Pine PS, Weaver JL, Oravecz T, Pall M, Ussery M, and Aszalos A

Subjects

Antibodies, Monoclonal, CD4-Positive T-Lymphocytes immunology, Cell Fusion physiology, Cell Line, Cytochalasin D pharmacology, Fluoresceins pharmacokinetics, Fluorescent Dyes pharmacokinetics, Giant Cells physiology, HIV-1 growth & development, Humans, Image Processing, Computer-Assisted, Nucleic Acid Synthesis Inhibitors pharmacology, Time Factors, Virus Replication drug effects, CD4-Positive T-Lymphocytes cytology, CD4-Positive T-Lymphocytes virology, HIV Envelope Protein gp120 analysis, HIV Envelope Protein gp41 analysis, HIV-1 isolation & purification

Abstract

A novel fluorescence-based method was developed to measure HIV envelope glycoprotein (env)-CD4-mediated cell fusion. This method measures the spread of a fluorescent dye as the cytosolic compartments of adjacent cells become contiguous upon cell-to-cell fusion. Calcein-labeled CD4+ Sup-T1 cells were seeded onto a monolayer of unlabeled TF228.1.16 cells, which stably express env, the gp120-gp41 complex. Changes in the following parameters were measured using a stage-scanning laser microscope: total fluorescent area, average fluorescent area, and average shape factor. Anti-CD4 monoclonal antibodies, anti-Leu3a, and OKT4E were shown to block fusion in a dose-dependent manner, while OKT4 had no effect. Aurin tricarboxylic acid, a compound that interferes with the binding of anti-Leu3a mAb and gp120 to CD4+ human peripheral blood lymphocytes, T20, a peptide that interferes with gp41, and cytochalasin D, a microfilament disrupter, all blocked fusion in a dose-dependent manner. This semiautomated assay can be used to quickly assess the effectiveness of compounds acting at different sites to block CD4 and env initiated cell-to-cell fusion.

Published

1998

2. Laser scanning and confocal microscopy of daunorubicin, doxorubicin, and rhodamine 123 in multidrug-resistant cells.

Author

Weaver JL, Pine PS, Aszalos A, Schoenlein PV, Currier SJ, Padmanabhan R, and Gottesman MM

Subjects

ATP Binding Cassette Transporter, Subfamily B, Member 1, Animals, Cell Line, Daunorubicin analysis, Doxorubicin analysis, Drug Resistance genetics, Humans, KB Cells, Lasers, Membrane Glycoproteins genetics, Mice, Microscopy, Fluorescence methods, Rhodamine 123, Rhodamines analysis, Transfection, Verapamil pharmacology, Daunorubicin metabolism, Doxorubicin metabolism, Drug Resistance physiology, Rhodamines metabolism

Abstract

The multidrug-resistant gene (MDR1) encodes an energy-dependent drug efflux pump (P-glycoprotein) for many anti-cancer drugs. We have studied the intracellular distribution of rhodamine 123 (R123), daunorubicin (DN), and doxorubicin (DOX) in cells expressing a human MDR1 gene. The distribution of these fluorescent drugs was measured by laser scanning microscopy and confocal microscopy. We devised a new method for analysis of fluorescence line scan data to determine the intracellular distribution of fluorescent probes. This method and confocal microscopy showed that R123, DN, and DOX are localized to both plasma membrane and intracellular compartments in multidrug-resistant cells. When the cells are treated with verapamil, an inhibitor of the multidrug transporter, the amount of DOX, DN, and R123 associated with the cell rises. After inhibition, the relative distribution of DOX and DN between the cell surface and intracellular structures does not change dramatically. However, R123 tends to relocalize to intracellular sites from predominantly plasma membrane sites, indicating that this dye behaves differently than the anti-cancer drugs. These results show the subcellular distributions of R123, DN, and DOX in plasma membrane, cytoplasm, and intracellular membrane systems, but do not allow definitive distinctions among existing models of how P-glycoprotein affects the distribution of drugs.

Published

1991