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Radioimmunoassay • Radioimmunoassay (RIA) is a very sensitive in vitro assay technique used to measure concentrations of antigens (for example, hormone levels in the blood) by use of antibodies. • RIA technique is extremely sensitive and extremely specific, requiring specialized equipment. History • The technique was introduced in 1960 by Berson and Yalow as an assay for the concentration of insulin in plasma. • It represented the first time that hormone levels in the blood could be detected by an in vitro assay. • The technique of radioimmunoassay has revolutionized research and clinical practice in many areas, e.g., –Blood banking –Diagnosis of allergies –Endocrinology Principle • The technique is based on the ability of an unlabelled form of the substance to inhibit competitively the binding of a radioactively labelled substance by specific antibodies. I125 labeled antigen Ag in serum Ab for the Ag • It is based on a principle of serial dilutions. One starts with a combination of radioactively labelled antigen (corresponding to the hormone to be measured) and antibody to that hormone. • Then, a specific quantity of unlabeled, or cold antigen is added to the mixture. The unlabeled antigen competes with the radioactive antigen for binding to the antibody and displaces a proportional amount of it. The unbound antigen is separated away (by centrifugation, for example) and the amount of radioactivity remaining is measured. • This process is continually repeated, using progressively greater concentrations of unlabeled antigen, and a line graph demonstrating the relationship between concentration of the unlabeled antigen and the radioactivity remaining is constructed. • This process creates a standard binding curve. The competitive binding process is then repeated using the biological sample to be tested and by comparison the radioactivity resulting with the standard binding curve, one can deduce the concentration of the hormone in the sample of interest.
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