Ultratrace determination of platinum in biological materials via neutron activation and radiochemical separation

A neutron activation analysis scheme based upon a radiochemical separation of the activation products has been developed. The method utilizes the inherent sensitivity of the activation reaction¹⁹⁸Pt(n, γ)¹⁹⁹Pt and counting of the daughter nuclide¹⁹⁹Au. This nuclide is radiochemically separated from interfering activities by homogeneous precipitation as elemental gold. The remaining interference of the secondary reaction¹⁹⁷Au(n,γ)¹⁹⁸ Au(n,γ)¹⁹⁹Au from gold in the samples is quantitatively assessed and corrected. During this process accurate gold concentrations in the samples are obtained at ultratrace levels. The analysis scheme is applied to gold and platinum determinations in biological Standard Reference Materials and human liver specimens. Gold and platinum are determined at concentrations of 5·10^?11 g/g, and at higher levels.