For industrial purposes cobalt is used to a large extent. About 2,300 persons are occupationally exposed to this carcinogenic metal in Western Germany. As reliable analytic methods for biological monitoring are not available we developed procedures for analyzing cobalt in whole blood and urine by using two independent methods, voltammetry and ETAAS. For ETAAS-analysis of urine the cobalt content is chelatized and extracted in an organic solvent. This clean-up step enables us to calibrate with aqueous standards.--Samples of whole blood are directly injected into the graphite tube after being diluted with a homogeniziser. For their gentle thermal decomposition we use a temperature/time programme containing six steps. Both kinds of sample treatments are uncomplicated and permit routine applications. For voltammetric determination of cobalt in urine and blood the biological material must be completely mineralized. The dry residue is dissolved in a NH4Cl/NH3 solution. Cobalt is chelatized with 2,3-butanedione-dioxime and preconcentrated by adsorption at the hanging mercury electrode. By scanning the potential into negative direction the cobalt complex is reduced. The resulting signal can be used for the quantitative determination. For comparison of both methods we have analyzed blood and urine samples of occupationally exposed persons. We found very good correlations with a statistical significance at the level of 0.01%.