Activation analysis of Se in biological samples through75Se and77mSe

A method is described to separate trace amounts of selenium in biological samples without using a carrier. This method is based on the adsorption on active carbon of the complex ion formed with APDC /ammonium salt of l-pyrrolidine carbodithioic acid/ at pH 1. The efficiency of the radiochemical separation described is measured by using carrier-free⁷⁵Se labelled solutions of sodium selenite at selenium concentrations from 3.5×10^–8 to 3.5×10^–11 g ml^–1. The results were between 95% and 98% with statistical variations from 2% to 10%. The determination of selenium can be made following this separation either through⁷⁵Se in the traditional way, or through^77mSe if the separation is performed prior to irradiation. The detection limits on the available conditions were 0.01 ppm for⁷⁵Se and 0.1 ppm for^77mSe. When the analysis is performed through⁷⁵Se /t=120 d/, the statistical error is notably smaller because the counting time may be considerable, whereas through^77mSe/t=17.5 s/it is higher than 20%, depending on the concentration and the available neutron flux. However, the advantages of gaining time and the fact of performing the trace separation from a non radioactive material, make both procedures competitive as useful tools for the research on the function of Se in vertebrates.