Speciation of selenium-containing small molecules in urine and cell lysate by CE-ICPMS with in-capillary enrichment.

IF 5.6 1区 化学 Q1 CHEMISTRY, ANALYTICAL
Talanta Pub Date : 2025-01-01 Epub Date: 2024-09-21 DOI:10.1016/j.talanta.2024.126929
Yi Lu, Xue Men, Chengxin Wu, Xing Wei, Mingli Chen, Jianhua Wang
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引用次数: 0

Abstract

The quantitative speciation of selenium in biological systems is highly important for evaluating health status and elucidating transformations of Se species in physiological and pathological processes. Hyphenation of capillary electrophoresis with inductively coupled plasma mass spectrometry (CE-ICPMS) is promising for this purpose. However, the unfavorable or insufficient sensitivity for selenium analysis with CE-ICPMS seriously limits its practical applications in biological analysis, e.g., cell analysis. Therefore, it is crucial to improve the detection sensitivity for Se species. In this study, CE-ICPMS sensitivities for five selenium species (selenocystamine (SeA), methyl-2-acetamido-2-deoxy-1-seleno-β-d-galactopyranoside (SeSug 1), selenomethionine (SeMet), Se-Methylselenocysteine (MeSeCys) and selenocystine (SeCys)) were improved by in-capillary stacking via pH gradient between the zones of sample-leading buffer and the incorporation of isopropanol. The improvement on sensitivity of up to 9.9 folds was achieved in different biological samples, with LODs of 0.29-0.52 μg L-1. This approach was further applied for Se speciation in cell lysate, urine and culture medium. It showed that SeMet was more readily reduced in the medium and favorably accumulated by HepG2, HuH-7 and HCCLM3 cells with respect to SeSug 1 and MeSeCys. In cells, all the three Se species were largely transformed into other Se species. Furthermore, more than 70 % of SeMet reduced in medium was transformed into unknown Se species after 48-h interaction with cells.

利用毛细管内富集的 CE-ICPMS 对尿液和细胞裂解物中的含硒小分子进行定性。
生物系统中硒的定量分型对于评估健康状况以及阐明生理和病理过程中硒物种的转化非常重要。毛细管电泳与电感耦合等离子体质谱联用(CE-ICPMS)在这方面前景广阔。然而,用 CE-ICPMS 分析硒的灵敏度不高或不足,严重限制了其在生物分析(如细胞分析)中的实际应用。因此,提高硒的检测灵敏度至关重要。本研究采用毛细管内堆积法,在样品前缓冲液区之间进行 pH 梯度调节,并加入异丙醇,提高了对五种硒(硒囊胺(SeA)、甲基-2-乙酰氨基-2-脱氧-1-硒-β-d-吡喃半乳糖苷(SeSug 1)、硒蛋氨酸(SeMet)、硒甲基硒半胱氨酸(MeSeCys)和硒胱氨酸(SeCys))的检测灵敏度。不同生物样品的灵敏度提高了 9.9 倍,最低检测限为 0.29-0.52 μg L-1。这种方法还被进一步应用于细胞裂解物、尿液和培养基中的硒离子。结果表明,与 SeSug 1 和 MeSeCys 相比,SeMet 更容易在培养基中被还原,并有利于 HepG2、HuH-7 和 HCCLM3 细胞的积累。在细胞中,所有三种 Se 在很大程度上都转化成了其他 Se。此外,与细胞作用 48 小时后,培养基中减少的 SeMet 有超过 70% 转化为未知的 Se 物种。
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来源期刊
Talanta
Talanta 化学-分析化学
CiteScore
12.30
自引率
4.90%
发文量
861
审稿时长
29 days
期刊介绍: Talanta provides a forum for the publication of original research papers, short communications, and critical reviews in all branches of pure and applied analytical chemistry. Papers are evaluated based on established guidelines, including the fundamental nature of the study, scientific novelty, substantial improvement or advantage over existing technology or methods, and demonstrated analytical applicability. Original research papers on fundamental studies, and on novel sensor and instrumentation developments, are encouraged. Novel or improved applications in areas such as clinical and biological chemistry, environmental analysis, geochemistry, materials science and engineering, and analytical platforms for omics development are welcome. Analytical performance of methods should be determined, including interference and matrix effects, and methods should be validated by comparison with a standard method, or analysis of a certified reference material. Simple spiking recoveries may not be sufficient. The developed method should especially comprise information on selectivity, sensitivity, detection limits, accuracy, and reliability. However, applying official validation or robustness studies to a routine method or technique does not necessarily constitute novelty. Proper statistical treatment of the data should be provided. Relevant literature should be cited, including related publications by the authors, and authors should discuss how their proposed methodology compares with previously reported methods.
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