A radioimmunoassay for serum 11-deoxy-17-ketosteroids

Abstract

A simplified method for evaluating serum 11-deoxy-17-ketosteroids (11-deoxy-17-KS) equivalent to dehydroepiandrosterone sulfate (DHEAS) has been developed without solvolysis and chromatography. 5μl of serum or plasma was added to 1 ml of ethanol, mixed, and centrifuged. 10 or 20 μ1 of the supernatant was evaporated to dryness and incubated with anti-11-deoxy-17-KS antiserum obtained by immunizing a rabbit with DHEA-3·O·CO-BSA which was prepared from DHEA-3·O·COC1 and containing DHEAS-7α 3H, pepsin-treated human immune serum globulin and bovine serum albumin. Ammonium sulfate was used to separate free from bound DHEAS-7α 3H. The accuracy, precision and sensitivity were satisfactory. The blank values could not be differentiated from zero. As the antiserum reacted not only on DHEAS but also on androsterone sulfate and etiocholanolone sulfate, serum 11-deoxy-17KS obtained by the radioimmunoassay expressed nearly the sum of 100% of DHEAS, 45% of androsterone sulfate and 35% of etiocholanolone sulfate in the serum. A good correlation was found between serum 11-deoxy-17-KS and DHEAS obtained by the radioimmunoassay described in a preveous paper (1). The present radioimmunoassay is the simplest method for the evaluation of the concentrations of C 19 steroids in the serum.