Although the general cytotoxicity of selenite is well established, the mechanism by which this compound crosses cellular membranes is still unknown. Here, we show that in Saccharomyces cerevisiae, the transport system used opportunistically by selenite depends on the phosphate concentration in the growth medium. Both the high and low affinity phosphate transporters are involved in selenite uptake. When cells are grown at low P i concentrations, the high affinity phosphate transporter Pho84p is the major contributor to selenite uptake. When phosphate is abundant, selenite is internalized through the low affinity P i transporters (Pho87p, Pho90p, and Pho91p). Accordingly, inactivation of the high affinity phosphate transporter Pho84p results in increased resistance to selenite and reduced uptake in low P i medium, whereas deletion of SPL2, a negative regulator of low affinity phosphate uptake, results in exacerbated sensitivity to selenite. Measurements of the kinetic parameters for selenite and phosphate uptake demonstrate that there is a competition between phosphate and selenite ions for both P i transport systems. In addition, our results indicate that Pho84p is very selective for phosphate as compared with selenite, whereas the low affinity transporters discriminate less efficiently between the two ions. The properties of phosphate and selenite transport enable us to propose an explanation to the paradoxical increase of selenite toxicity when phosphate concentration in the growth medium is raised above 1 mM.Although toxic at high concentrations, selenium is required in many cells, because it is translationally incorporated as selenocysteine into selenoproteins that perform specific and essential functions (1). Cells must ensure selenium uptake to sustain this metabolism. However, little is known about selenium transport. Because selenium and sulfur are chalcogen elements that have many chemical properties in common, selenium shares metabolic pathways with sulfur. Accordingly, selenate was shown to be taken up by the yeast Saccharomyces cerevisiae sulfate permeases (2). Similarly, in plants, selenate is taken up by roots via the high affinity sulfate transporters (3).On the other hand, specific selenite transporters have never been identified so far. The sulfate ABC transporter of Escherichia coli mediates selenite uptake in addition to that of selenate (4). However, repression of the expression of that transporter does not quench selenite uptake completely, indicating that an alternative entry pathway exists for selenite (5). In S. cerevisiae, which does not possess selenoproteins, an energy-dependent uptake of selenite, distinct from that of selenate, was reported. Characterization of the kinetics of selenite uptake suggested the existence of two transport systems: a high affinity system at low selenite concentration and a low affinity system at higher concentration (6). Recently, a study of selenite uptake by wheat (Triticum aestivum) roots showed it to be an active process competitively inhibited by phosph...
Results of an international intercomparison study (CCQM-P86) to assess the analytical capabilities of national metrology institutes (NMIs) and selected expert laboratories worldwide to accurately quantitate the mass fraction of selenomethionine (SeMet) and total Se in pharmaceutical tablets of selenised-yeast supplements (produced by Pharma Nord, Denmark) are presented. The study, jointly coordinated by LGC Ltd., UK, and the Institute for National Measurement Standards, National Research Council of Canada (NRCC), was conducted under the auspices of the Comité Consultatif pour la Quantité de Matière (CCQM) Inorganic Analysis Working Group and involved 15 laboratories (from 12 countries), of which ten were NMIs. Apart from a protocol for determination of moisture content and the provision of the certified reference material (CRM) SELM-1 to be used as the quality control sample, no sample preparation/extraction method was prescribed. A variety of approaches was thus used, including single-step and multiple-step enzymatic hydrolysis, enzymatic probe sonication and hydrolysis with methanesulfonic acid for SeMet, as well as microwave-assisted acid digestion and enzymatic probe sonication for total Se. For total Se, detection techniques included inductively coupled plasma (ICP) mass spectrometry (MS) with external calibration, standard additions or isotope dilution MS (IDMS), inductively coupled plasma optical emission spectrometry , flame atomic absorption spectrometry and instrumental neutron activation analysis. For determination of SeMet in the tablets, five NMIs and three academic/institute laboratories (of a total of five) relied upon measurements using IDMS. For species-specific IDMS measurements, an isotopically enriched standard of SeMet (76Se-enriched SeMet) was made available. A novel aspect of this study relies on the approach used to distinguish any errors which arise during analysis of a SeMet calibration solution from those which occur during analysis of the matrix. To help those participants undertaking SeMet analysis to do this, a blind sample in the form of a standard solution of natural abundance SeMet in 0.1 M HCl (with an expected value of 956 mg kg(-1) SeMet) was provided. Both high-performance liquid chromatography (HPLC)-ICP-MS or gas chromatography (GC)-ICP-MS and GC-MS techniques were used for quantitation of SeMet. Several advances in analytical methods for determination of SeMet were identified, including the combined use of double IDMS with HPLC-ICP-MS following extraction with methanesulfonic acid and simplified two-step enzymatic hydrolysis with protease/lipase/driselase followed by HPLC-ICP-IDMS, both using a species-specific IDMS approach. Overall, satisfactory agreement amongst participants was achieved; results averaged 337.6 mg kg(-1) (n = 13, with a standard deviation of 9.7 mg kg(-1)) and 561.5 mg kg(-1) (n = 11, with a standard deviation of 44.3 mg kg(-1)) with median values of 337.6 and 575.0 mg kg(-1) for total Se and SeMet, respectively. Recovery of SeMet from SELM-1 averaged 95...
A new model equation for determining the measurement result in standard addition experiments was derived and successfully applied to the quantitative determination of rhodium in automotive catalysts. Existing equations for standard addition experiments with gravimetric preparation were changed in order to integrate the novel idea of including the uncertainty associated with the standard into the model equation. Using this novel equation combined with the ordinary least squares algorithm for the regression line also yielded a new formula for the associated measurement uncertainty. This uncertainty accounts for the first time for the uncertainty associated with the standard. The derivation for the model equation and the resulting associated measurement uncertainty is shown for gravimetric standard addition experiments both with and without an internal standard.
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