Biotin-Avidin Mediated Homogeneous Enzyme-Linked Binding Assays for Riboflavin and Riboflavin Binding Protein Using Alkaline Phosphatase as the Labelt

A detailed model describing particle growth and morphology in polyolefins synthesized using supported metallocene catalysts is presented. The multigrain model (MGM) is extended to consider metal extraction and the effects of polymer particle compressibility, in addition to monomer sorption and mass and heat transfer considerations. The effects of active metal extraction into the polymer phase and the pores of the particle on the kinetics of polymerization and morphological features of the polymer particle are studied. The effects of greater compressibility of polymer particles on morphological features such as particle porosity are studied. Model predictions for porosity and morphology are shown to reproduce similar trends as have been reported in experimental studies. © 2001 John Wiley & Sons, Inc. J Appl Polym Sci 79: 2565–2579, 2001

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Local Modulation of the Redox State of p‐Nitrothiophenol Self‐Assembled Monolayers Using the Direct Mode of Scanning Electrochemical Microscopy

Schwamborn

Stoica

Neugebauer

et al. 2009

ChemPhysChem

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Labeling Digoxin Antibody with Colloidal Gold and Ferrocene for Its Use in a Membrane Immunostrip and Immunosensor

Choi

Kim

Choi

et al. 1999

Microchemical Journal

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Enzyme-Linked Competitive Binding Assays Based on the Biotin/Avidin Interaction

et al. 1999

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The strong interaction between biotin and avidin is utilized for the development of enzyme-linked competitive binding assays not only for biotin itself, but also for other biomolecules. Alkaline phosphatase, a single substrate enzyme typically used for heterogeneous types of competitive binding assays, is employed also for homogeneous types. For the biotin assay, the heterogeneous protocol offers a much improved detection capability when compared to the homogeneous type. A simple approach of simulating dose-response curves is introduced. An effective analyte concentration attached to an enzyme label is determined by using the same binder, but with a different enzyme label. The analyte system adapted to the biotin/avidin-mediated homogeneous protocol is digoxin and a monoclonal anti-digoxin antibody. The detection capabilities of these assays, particularly the homogeneous types, are shown to be limited by the detectability of the enzyme conjugate employed.

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Biotin-Avidin Mediated Homogeneous Enzyme-Linked Binding Assays for Riboflavin and Riboflavin Binding Protein Using Alkaline Phosphatase as the Labelt

Cited by 3 publications

References 11 publications

Local Modulation of the Redox State of p‐Nitrothiophenol Self‐Assembled Monolayers Using the Direct Mode of Scanning Electrochemical Microscopy

Local Modulation of the Redox State of p‐Nitrothiophenol Self‐Assembled Monolayers Using the Direct Mode of Scanning Electrochemical Microscopy

Labeling Digoxin Antibody with Colloidal Gold and Ferrocene for Its Use in a Membrane Immunostrip and Immunosensor

Enzyme-Linked Competitive Binding Assays Based on the Biotin/Avidin Interaction

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