Staining of fungal cell walls with fluorescent brighteners: Flow-cytometric analysis

Flow cytometry is a rapid method for measuring the optical properties of individual cells. The technique has found great utility in the study of mammalian cells, but microbiological applications have been more limited. We here show that UV-excited fluorescent whitening agents, in particular Tinopal

## Background: This study was undertaken in mice to develop a reproducible procedure of cell permeabilization, allowing intracellular protein staining by immunofluorescence (i.e., bcl-2) without losing surface labeling especially for lectins (i.e., b220 and peanut agglutinin [pna]). this article re

Background: Flow cytometric analysis is a powerful technique for the single cell assessment of cell surface expression of selected molecules. The major deficiency of flow cytometry has been its relative insensitivity. Only molecules expressed in abundance have been readily observed. Methods: We have

Double fluorescent labeling, with fluorescein isothiocyanate (FIT0labeled F(ab')z specific lor the heavy chain and R-phycoerythrin (R-PE)-labeled F(ab')2 specific for the light chain, wiis demoilstrated :IS ;I convenient means for the accurate evaluation of a heterogeneous non-aIitibody-producing po