Preparation of polysaccharide-enzyme conjugates for competitive binding assays

The use of two enzyme labels in a dual analyte simultaneous heterogeneous enzyme-linked competitive binding assay is examined. Reaction conditions for monitoring glucosed-phosphate dehydrogenase (G6PDH) and Pgalactosidase (@gal) activities are found which enable the independent measurement of each e

A new solid-phase enzyme-linked assay for riboflavin (vitamin B2) is described. The assay is based on the competition between analyte vitamin molecules and a glucose-6-phosphate dehydrogenase-3-carboxymethylriboflavin conjugate for a limited number of riboflavin-binding protein sites immobilized on

A simple method has been developed to assay the immunological reactivity of antigenenzyme conjugates by rate nephelometry. Unlike immunodiffusion or immunoelectrophoresis, the procedure is independent of molecular hydrodynamics and is based on precipitin rate curves obtained by light-scattering meas

## Abstract Tubulin is an attractive and established target for anticancer therapy. To date, the only method to determine the binding of inhibitor to tubulin has been competitive radioligand binding assays. We developed a non‐radioactive mass spectrometry (MS) binding assay to study the tubulin bin

The competitive ELISA test was compared with competitive RIA, complement fixation, and indirect fluorescent antibody test for the detection of antibody to varicella-zoster virus (VZV). ELISA and RIA were the most sensitive tests, being tenfold as sensitive as indirect immunofluorescence and 20 times

## Abstract A single step, separation free competitive binding reaction between the fluorescent antibiotic mithramycin and actinomycin‐D for common binding sites on DNA coated 10 μm diameter microspheres is described. The fluorescence of the microspheres is measured with a flowcytometer. In the pre