DEVELOPMENT OF A DIRECT RADIOIMMUNOASSAY FOR SERUM PROGESTERONE

A direct radioimmunoassay for the measurement of progesterone in human serum is described. Progesterone 11 alpha-hemisuccinate was conjugate d to tyrosine methyl ester (TME) by the mix anhydride method and then iodinated using chloramine-T. The radiochemical purity of different ba tches of I-125-progesterone was greater than 95% and showed 70-75% bin ding with excess antibody. Progesterone 11 alpha-hemisuccinate was cou pled with BSA and injected to rabits. Antisera collected after three b ooster injections and having a K value of 1 . 10(9) l/M was selected F or the assay. Significant reduction in binding with antibody was seen when hormone free serum was used in the assay system. Various blocking agents were tried to reduce the serum effects and none of them were f ound satisfactory. From a series of optimization experiments, an assay was developed without the use of blocking agents. This assay used a m uch higher concentration of antibody along with lower amount of serum sample (50 mu l). The optimized assay has a sensitivity of 0.5 nj/ml a nd a working range of 0.5 to 100 ng/ml. Serum samples were analyzed us ing the present system and with a kit obtained from Diagnostic Product s Corporation (DPC). Regression analysis showed good correlation betwe en the results obtained from the present system and the DPC kit. (Y = 0.93X + 0.5, r = 0.93 for n = 25).