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一种用于评估化学硒或食物硒向谷胱甘肽过氧化物酶中差异掺入的缺硒Caco-2细胞模型。

A selenium-deficient Caco-2 cell model for assessing differential incorporation of chemical or food selenium into glutathione peroxidase.

作者信息

Zeng Huawei, Botnen James H, Johnson Luann K

机构信息

Agricultural Research Service, Grand Forks Human Nutrition Research Center, US Department of Agriculture, Grand Forks, ND, 58202-9034, USA.

出版信息

Biol Trace Elem Res. 2008 Summer;123(1-3):98-108. doi: 10.1007/s12011-008-8097-8. Epub 2008 Feb 12.

DOI:10.1007/s12011-008-8097-8
PMID:18265950
Abstract

Assessing the ability of a selenium (Se) sample to induce cellular glutathione peroxidase (GPx) activity in Se-deficient animals is the most commonly used method to determine Se bioavailability. Our goal is to establish a Se-deficient cell culture model with differential incorporation of Se chemical forms into GPx, which may complement the in vivo studies. In the present study, we developed a Se-deficient Caco-2 cell model with a serum gradual reduction method. It is well recognized that selenomethionine (SeMet) is the major nutritional source of Se; therefore, SeMet, selenite, or methylselenocysteine (SeMSC) was added to cell culture media with different concentrations and treatment time points. We found that selenite and SeMSC induced GPx more rapidly than SeMet. However, SeMet was better retained as it is incorporated into proteins in place of methionine; compared with 8-, 24-, or 48-h treatment, 72-h Se treatment was a more sensitive time point to measure the potential of GPx induction in all tested concentrations. Based on induction of GPx activity, the cellular bioavailability of Se from an extract of selenobroccoli after a simulated gastrointestinal digestion was comparable with that of SeMSC and SeMet. These in vitro data are, for the first time, consistent with previous published data regarding selenite and SeMet bioavailability in animal models and Se chemical speciation studies with broccoli. Thus, Se-deficient Caco-2 cell model with differential incorporation of chemical or food forms of Se into GPx provides a new tool to study the cellular mechanisms of Se bioavailability.

摘要

评估硒(Se)样品在缺硒动物中诱导细胞谷胱甘肽过氧化物酶(GPx)活性的能力是测定硒生物利用度最常用的方法。我们的目标是建立一种缺硒细胞培养模型,该模型能使不同化学形式的硒差异地掺入GPx中,这可能会补充体内研究。在本研究中,我们采用血清逐步降低法建立了一种缺硒的Caco-2细胞模型。众所周知,硒代蛋氨酸(SeMet)是硒的主要营养来源;因此,将不同浓度和处理时间点的SeMet、亚硒酸盐或甲基硒代半胱氨酸(SeMSC)添加到细胞培养基中。我们发现亚硒酸盐和SeMSC比SeMet更快速地诱导GPx。然而,SeMet能更好地保留下来,因为它会取代蛋氨酸掺入蛋白质中;与8小时、24小时或48小时的处理相比,72小时的硒处理是在所有测试浓度下测量GPx诱导潜力的更敏感时间点。基于GPx活性的诱导,经模拟胃肠道消化后的硒西兰花提取物中硒的细胞生物利用度与SeMSC和SeMet相当。这些体外数据首次与先前发表的关于动物模型中亚硒酸盐和SeMet生物利用度以及西兰花硒化学形态研究的数据一致。因此,能使不同化学或食物形式的硒差异地掺入GPx的缺硒Caco-2细胞模型为研究硒生物利用度的细胞机制提供了一种新工具。

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