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Binding assay procedure

Radioassay is a competitive protein binding assay which employs a natural binding protein instead of an antibody. For example, transcortin is the binding protein for cortisol in nature and also in the radioassay procedure for cortisol. [Pg.58]

A prominent advantage of this assay procedure is the feature that the complex of hapten and labeled antibody was captured on a solid phase (PMP) and separated from the reaction medium before signal determination. This additional step not only reduces interference due to biological specimens but also eliminates the tedious transfer of supernatant, which is essential in conventional immunometric assays. This immunometric assay provided somewhat improved specificity in terms of the cross-reactivities with T2 and reverse T3 (3,3, 5 -L-triiodothyronine). The authors speculated that the dissociation rate of the antibody-cross-reactant complex would be faster than that of an antibody-analyte complex thus the former binding would be preferentially substimted by T2 immobilized on CPG. [Pg.155]

Lectins, or proteins with specific binding sites for carbohydrates, can be used as targeting molecules to localize particular glycoconjugates such as glycoproteins or glycolipids on cell surfaces (Fig. 373). Labeled with gold particles, lectins are important probes for detection of cell surface components and intracellular receptors and in immunological or biochemical assay procedures (Bog-Hansen et al., 1978 Kimura et al., 1979 Nicolson, 1978 Roth, 1983 Benhamou et al., 1988 Nakajima et al., 1988). [Pg.621]

Affinity of MIP towards the target analyte should be examined prior to fabrication of the chemosensor. Batch binding assays are used to test selectivity of suitable MIPs. Especially, affinity of MIP to compounds, which are structurally related to the target analyte, should be tested. If MIP binds similarly with these compounds as the template, then cross-reactivity is manifested [156], This effect was exploited for determination of adenine and its derivatives with the use of MIP templated with 9-ethyladenine. Nevertheless, the cross-reactivity, if undesired, can be avoided by suitable sample pretreatment, e.g. by interferant extraction with a supported liquid membrane (SLM) coupled to the MIP-PZ chemosensor. The Fluoropore membrane filter of submicrometre porosity can serve that purpose. That way, this membrane holds interferants, thus eliminating the matrix effect. The SLM-involving determination procedure is cheaper than traditional laborious sample pretreatment used to remove the interfering substances. For instance, caffeine [143] and vanillin [157] in food samples have been determined using this procedure. [Pg.228]

Bar-Or, 2001 [8] PTCA 54 NA NA Change in albumin-cobalt binding assay value after procedure Prospective enrollment... [Pg.4]

Enzyme-linked Immunosorbent Assay. A promising alternative to the RIA procedure is an enzyme-linked immunosorbent assay (ELISA) which depends upon the conjugation of a functional enzyme to either an antigen or antibody. The amount of enzyme present in a competitive binding assay is quantitated instead of the amount of radiolabeled compound. The concentration of the enzyme can be determined through its subsequent reaction with a substrate which results in a measurable spectroscopic change. [Pg.338]


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See also in sourсe #XX -- [ Pg.179 ]

See also in sourсe #XX -- [ Pg.241 ]




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Assay procedure

Binding assays

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