Corrections for instrumental errors in measurement of fluorescence and polarization of fluorescence

## Background: The pulses of light scatter and fluorescence measured in flow cytometers exhibit varying degrees of polarization. Flow cytometers are heterogeneously sensitive to this polarization, depending on the light source(s), the optical layout, and the types of mirrors and filters used. There

A simple and direct method for the simultaneous correction of steady-state polarized fluorescence intensities, depolarized (or scrambled) by the effects of applied hydrostatic pressure, is described. In the method discussed here, it is not necessary to first determine the scrambling factors from a s

Synthesis of Immunocomponents for the Measurement of Lead (Pb) by Fluorescence Polarization Immunoassay. -The development of an immunoassay for lead, based on the inhibition of 5-aminolevulinic acid dehydratase and its indication by fluorescence polarization (FPIA), is described. Five fluorescent t

## Background: The Cellscan mark-S (CS-S) scanning cytometer was used for tracing enzymatic reactions in the same individual cells under various physiological conditions over periods of minutes. On-line reagent addition and changes in the experimental conditions (buffers, ions, substrates and inhib

A theory describing the shapes of polarized fluorescence photobleaching recovery ( PFPR ) curves for a population of fluorophores undergoing restricted rotational diffusion in twodimensional systems such as planar membranes has been developed. In this model, restricted rotational diffusion of the fl

Background: Numerous applications of fluorescence microscopy require quantitation of signal intensity in reproducible units. Two problems must be overcome to achieve this goal. First, due to various instrumental factors, the same sample imaged on two microscopes or even on the same microscope at dif