Phenotypic biomonitoring using multivariate flow cytometric analysis of multi-stained microorganisms

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

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

The expression of different proliferation associated nuclear antigens was analyzed using a washless double-staining method and flow cytometry. It is a simple and rapid two-step procedure which can be performed on low cell numbers. A series of hematopoietic cell lines and fresh lymphoma cells were te

We have developed a "one-tube" triple staining procedure that allows the identification of intratumor phenotypic subpopulations by FCM. Solid tumors were dissociated by a combined mechanid enzymatic method. Ovarian ascites tumor cell aggregates were enzymatically dissociated using trypsin. A n antik