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采用顶空 GC-MS 法测定体外代谢模型中甲基硒醇、二甲基硒化物和二甲基二硒化物的形成。

Formation of methylselenol, dimethylselenide and dimethyldiselenide in in vitro metabolism models determined by headspace GC-MS.

机构信息

Department of Pharmaceutics and Analytical Chemistry, Faculty of Pharmaceutical Sciences, University of Copenhagen, Universitetsparken 2, Copenhagen, Denmark.

出版信息

Metallomics. 2010 Feb;2(2):167-73. doi: 10.1039/b914255j. Epub 2010 Jan 7.

Abstract

The aim of this study was to identify the presence of MeSeH in metabolic reactions. An analytical method based on direct headspace GC-MS, eliminating loss of volatile species during sample pretreatment procedures, was developed for this purpose. The in vitro conversion of selenium compounds to the volatile species methylselenol, MeSeH, dimethyl selenide, DMeSe and dimethyl diselenide, DMeDSe was investigated. The analytical method was evaluated by means of standards of dimethyl diselenide, dimethyl selenide. The corresponding sulfides were found unsuitable as internal standards as they interacted with the selenides. The limit of detection was 0.25 μmol L(-1) (20 μg L(-1)) for the selenide as well as the diselenide. Formation of MeSeH was not observed in significant amount when selenomethionine was incubated with the enzyme l-methionine-γ-lyase; instead large amounts of DMeDSe were formed. In aqueous solution, methylseleninic acid, MeSeA reacted spontaneously with glutathione, GSH to form DMeDSe. In strongly reducing environments, however, MeSeH was also observed. When the formed MeSeH was trapped with iodoacetic acid, no DMeDSe was detected indicating that DMeDSe formation was due to spontaneous oxidation of MeSeH. These findings imply that DMeDSe may be a marker for the production of MeSeH in in vitro models. When MeSeA, Se-methylselenocysteine, Se-MeSeCys and SeMet were incubated with Jurkat cells, DMeDSe formation was only observed in the case of MeSeA. Trace amounts of DMeSe was observed in the vial with MeSeA as well as Se-MeSeCys. When DMeSe and DMeDSe were added to plasma, the sensitivity of only DMeDSe decreased significantly, implicating that DMeDSe underwent a reaction with plasma hindering the volatilization. This emphasizes that results from in vitro selenium metabolism studies may not be uncritically interpreted as consistent with the in vivo reality.

摘要

本研究旨在鉴定代谢反应中 MeSeH 的存在。为此,开发了一种基于直接顶空 GC-MS 的分析方法,该方法在样品预处理过程中消除了挥发性物质的损失。研究了硒化合物向挥发性物质甲基硒醇(MeSeH)、二甲基硒化物(DMeSe)、二甲基二硒化物(DMeDSe)转化的体外转化。通过二甲基二硒化物、二甲基硒化物的标准品对分析方法进行了评估。发现相应的硫化物不适合作为内标,因为它们与硒化物相互作用。硒化物和二硒化物的检出限均为 0.25 μmol L(-1)(20 μg L(-1))。当蛋氨酸与酶 l-蛋氨酸-γ-裂合酶孵育时,没有观察到蛋氨酸硒代半胱氨酸大量生成 MeSeH;相反,大量形成 DMeDSe。在水溶液中,甲基亚硒酸(MeSeA)与谷胱甘肽(GSH)自发反应生成 DMeDSe。然而,在强还原环境中,也观察到 MeSeH。当形成的 MeSeH 用碘代乙酸捕获时,没有检测到 DMeDSe,表明 DMeDSe 的形成是由于 MeSeH 的自发氧化。这些发现表明,DMeDSe 可能是体外模型中 MeSeH 产生的标志物。当 MeSeA、硒代蛋氨酸、Se-MeSeCys 和 Met 与 Jurkat 细胞孵育时,只有 MeSeA 才会形成 DMeDSe。在 MeSeA 以及 Se-MeSeCys 的小瓶中观察到痕量的 DMeSe。当 DMeSe 和 DMeDSe 加入到血浆中时,只有 DMeDSe 的灵敏度显著降低,这表明 DMeDSe 与血浆发生反应,阻碍了其挥发。这强调了从体外硒代谢研究中获得的结果可能不能被不加批判地解释为与体内实际情况一致。

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