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Tissue analysis mercury speciation

S. R. Segade, J. F. Tyson, Evaluation of two flow injection systems for mercury speciation analysis in fish tissue samples by slurry sampling cold vapor atomic absorption spectrometry, J. Anal. Atom. Spectrom., 18 (2003), 268-273. [Pg.725]

Earlier methods used to determine mercury in biological tissue and fluids were mainly colorimetric, using dithizone as the com-plexing agent. However, during the past two to three decades, AAS methods - predominantly the cold vapor principle with atomic absorption or atomic fluorescence detection - have become widely used due to their simplicity, sensitivity, and relatively low price. Neutron activation analysis (NAA), either in the instrumental or radiochemical mode, is still frequently used where nuclear reactors are available. Inductively coupled plasma mass spectrometry (ICP-MS) has become a valuable tool in mercury speciation. Gas and liquid chromatography, coupled with various detectors have also gained much importance for separa-tion/detection of mercury compounds (Table 17.1). [Pg.936]

Some of the difficulties in the unbiased determination of certain trace elements in biological materials may be due to problems of speciation. The range of complex organo-metallic species that can be found in nature is very wide (Frausto da Silva and Williams, 1991). In carrying out an analysis for a particular element in any type of biological fluid or tissues, major assumptions are made concerning the precise chemical composition of element species present. Different analytical techniques will have different sensitivities towards particular element species. Much of the early understanding of the special analytical problems posed by element speciation comes from studies of arsenic (Buchet et al., 1980 Buchet et al., 1981) and mercury (Clarkson, 1983). Problems with other metals remain to be resolved and may require considerable analytical sophistication such as in the analysis of chromium speciation (Urasa and Nam, 1989). [Pg.217]

Certified references are available mostly in powder form for tissues like hair, liver and muscle. For speciation analysis of tissue samples, it may be necessary to cold digest the tissue sample e.g. methyl mercury in hair samples will be destroyed if microwave digested." ... [Pg.391]


See other pages where Tissue analysis mercury speciation is mentioned: [Pg.359]    [Pg.6094]    [Pg.70]    [Pg.760]    [Pg.6093]    [Pg.572]    [Pg.300]    [Pg.391]   
See also in sourсe #XX -- [ Pg.228 , Pg.239 ]




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