Competitive binding systems

The 25-OH-D Is further metabolized In the kidney to 1,25 dlhydroxycholecalclferol (1,25(OH)2D) which Is considered to be the major physiologically Important, tissue-active metabolite of vitamin D. It circulates In extremely low concentrations (< 100 pg/ml of serum). Assay of 1,25(OH)2D Is extremely tedious. It Is done by competitive binding technique using a combined Intestinal cell cytosol and chromatin binding system, biosynthetic 3h-1,25(OH)2D3 as labeled ligand and synthetic 1,25(0H)2D3 as standard (31). 

W. Huang, A. Feltus, A. Witkowski, and S. Daunert, Homogeneous bioluminescence competitive binding assay for folate based on a coupled glucose-6-phosphate dehydrogenase-bacterial luciferase enzyme system. Anal. Chem. 68, 1646-1650 (1996). 

The most common of these systems is the enzyme-multiplied immunoassay technique or EMIT, which is particularly suited to the measurement of small molecules (haptens) such as drugs. EMIT is a trade mark of the Syva Corporation of Palo Alto, California. Although it does not involve the separation of bound fraction from free it is nevertheless a competitive assay system. The antigen is labelled with an enzyme in such a way that the enzyme retains its catalytic activity. When the antigen binds to the antibody the enzyme becomes inhibited, probably by an induced conformational change or by steric hindrance of the enzyme active site (Figure 7.15). 

As the investigation of the interactions between H DAC inhibitors and the enzymes are an important issue, competition assay systems are helpful implements in facilitating the characterization of inhibitor binding. Such a competition binding assay that has been developed for histone deacetylases is based on fluorescence resonance energy transfer (FRET) between tryptophan residues of the histone deacetylase and a fluorescent HDAC inhibitor [38]. In competition with other... 

Their efficacy in many illnesses is explained by the competitive binding of )3-adrenore-ceptors in the autonomic nervous system by basically any of the employed drags of the l-aryloxy-3-aminopropanol-2 class, which result in reduction of heart rate and strength of cardiac beats, slowing of atrioventricular conductivity, reduction of the level of renin in the plasma, and reduction of blood pressure. The main effects of 8-adrenoblockers are expressed at the level of the vasomotor center in the hypothalamus, which result in a slowing of the release of sympathetic, tonic impulses. Included in the main group of... 

Mixing different cross-linkers (19b and 19c) yielded systems with a strong gel-weak gel transition, rather than a distinct sol-gel shift. When the concentration of each of the cross-linkers was above the critical percolation threshold, the kinetically slower cross-linker (19c) dictated the gel properties. Upon addition of enough of a competitive binding additive, such as DMAP, to drop the concentration of the active cross-linking units below their individual percolation thresholds but still allowing the total amount of both active cross-linkers (19b and 19c) to be above the percolation threshold results in a gel whose properties are now controlled by the kinetically faster cross-linker (19c). 

Sklar, L. A., Sayre, J., McNeil, V. M., and Finney, D. A. (1985). Competitive binding kinetics in ligand-receptor-competitor systems. Rate parameters for unlabeled ligands for the formyl peptide receptor. Mol. Pharmacol. 28, 323-330. 

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