A method for the extraction and gas chromatographic determination of methylmercury in biological matrices is presented. By combining the advantages of two extraction techniques-microwave-assisted extraction (MAE) and solid-phase microextraction (SPME)--the separation of methylmercury from biological samples is possible. Specifically, the procedure involves microwave extraction with 3 M hydrochloric acid, followed by aqueous-phase derivatization with sodium tetraphenylborate and headspace SPME with a silica fibre coated with polydimethylsiloxane (PDMS). For optimization of the derivatization-SPME procedure, a central composite experimental design with alpha = 1.682 and two central points was used to model gas-chromatographic peak areas as functions of pH, extraction temperature and sorption time. A desirability function was then used for the simultaneous optimization for methylmercury and Hg(II). The optimal derivatization-SPME conditions identified were close to pH 5, temperature 100 degrees C, and sorption time 15 min. The identification and quantification of the extracted methylmercury is carried out by gas chromatography with microwave-induced plasma atomic emission spectrometry detection. The validity of the new procedure is shown by the results of analyses of certified reference materials.