Direct enzyme linked assay

Diphenylhydantoin (via drinking-water for six months) was tested in genetically predisposed mice (C57BL/6-lpr/lpr strain) and found to depress levels of autoantibodies (Bloksma et al., 1994). In another study (Okada et al., 2001), a slight shift towards a Th2 response was demonstrated by showing an increase in the keyhole limpet haemocyanin (KLH)-induced production of IL-4 and IgE as measured by direct enzyme-linked immunosorbent assay (ELISA) in a four-week exposure study. 

Multiple enzyme systems, where one enzyme produces an electrochemically inactive product that is consumed as a substrate by another enzyme to form an active product, have been successfully used to extend enzyme selectivity. The selectivity of immunochemical systems has been employed by implementation of enzyme-linked assays. Direct coupling of redox relay centers of enzymes to conductive electrodes has been achieved by a technique known as molecular wiring and avoids the indirect analysis of products of enzyme-substrate reactions. This fast and sensitive technique measures current flow and is commercially available. 

Oxime carbamates are not directly amenable to gas chromatography (GC) because of their high thermal instability, which often leads to their breakdown at the injection port or in the column during analysis. Analysis of oxime carbamates by GC with sulfur detection or flame photometric detection involves oxidation of the intact insecticides or alkaline hydrolysis to form the more volatile but stable oxime compound. Enzymatic techniques have been reported for the analysis of these compounds. Enzyme-linked immunosorbent assay (ELISA) has been used to determine aldicarb and its sulfone and sulfoxide metabolites and methomyl in water, soil, and sediment samples. 

Berkowitz FE, Levin MJ. Use of an enzyme-linked immunosorbent assay performed directly on fixed infected cell monolayers for evaluating drugs against varicella-zoster virus. Antimicrob. Agents Chemother. 1985 28 207-210. 

In a direct immunoassay the immobilized antibody binds to the corresponding antigen. The competitive immunoassay relies upon the competition of the analyte with a labelled analyte for antibody binding. These formats are widely used for high throughput affinity arrays. A sandwich immunoassay is based on the trapping or capture of the analyte by another antibody. In ELISA (enzyme linked immunosorbent assays) the second antibody is conjugated with an enzyme. The bound enzyme labelled antibody is detected by its ability to break down its substrate to a colored product. 

Enzyme-linked immunosorbent assay (ELISA) is comparable to the immuno-radiometric assay except that an enzyme tag is attached to the antibody instead of a radioactive label. ELISAs have the advantage of nonradioactive materials and produce an end product that can be assessed with a spectrophotometer. The molecule of interest is bound to the enzyme-labeled antibody, and the excess antibody is removed for immunoradiometric assays. After excess antibody has been removed or the second antibody containing the enzyme has been added (two-site assay), the substrate and cofactors necessary are added in order to visualize and record enzyme activity. The level of molecule of interest present is directly related to the level of enzymatic activity. The sensitivity of the ELISAs can be enhanced by increasing the incubation time for producing substrate. 

Enzyme-linked immunosorbent assay (ELISA) is based on the specific reaction between an antibody and an antigen. One of the reagents in the reaction is labeled with an enzyme that generates a colorimetric product that can be measured with a spectrophotometric device. The color intensity correlates with the concentration of specific antibody and the respective antigen. The reaction can be formatted in various ways in a multiwell plate (microtiter plate) with the common formats being the sandwich assay, the competitive assay, and the direct assay. (See Figure 11.1.)... 

Enzyme-Linked Immunosorbent Assays (ELISA). Three methods are commonly used direct competition, double antibody sandwish and antibody inhibition. 

B6. Buscarlet, L., Grass , J., Creminon, C., Pradelles, R, Dupret-Carruel, J., Jolivet, M., and Mons, S., Cross-linking of 17/i-estradiol to monoclonal antibodies by direct UV irradiation Application to an enzyme immunometric assay. Anal. Chem. 71, 1002-1008 (1999). 

Wolbers R, Landrey G (1987) The use of direct reactive fluorescent dyes for the characterization of binding media in cross sectional examinations. Preprints of 15th Annual Meeting of the American Institute for Conservation and Artistic Works, Vancouver, 168-202. Heginbotham A, Millay V, Quick M (2006) The use of immunofluorescence microscopy and enzyme-linked immunosorbent assay as complementary techniques for protein identification in artist s materials. J Am Inst Conserv 45 89-105. 

Enzyme-linked immunosorbent assays. An indirect application of enzymes in analysis is as a marker or label in enzyme-linked immunosorbent assays (ELISA). In ELISA, the enzyme does not react with the analyte instead, an antibody is raised against the analyte (antigen or hapten) and labelled with easily assayed enzyme, usually a phosphatase or a peroxidase. The enzyme activity is proportional to the amount of antibody in the system, which in turn is proportional, directly or indirectly depending on the arrangement used, to the amount of antigen present (Morris and Clifford, 1984). 

Among the many immunological assay methods, the enzyme-linked immunosorbent assay methods (ELISA) are the most popular methods. ELISA can detect both antigen molecules and antibody molecules with only a slight modification of the procedure. The direct-binding and sandwich methods that are used for the... 

Sulfadiazine Swine bile and Direct assay Direct competitive enzyme-linked 32-36 67... 

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