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采用富集稳定同位素结合多元线性回归对内源性光谱干扰和质量偏差进行硒代谢研究的校正。

Internal correction of spectral interferences and mass bias for selenium metabolism studies using enriched stable isotopes in combination with multiple linear regression.

机构信息

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

出版信息

Anal Bioanal Chem. 2012 Mar;402(9):2749-63. doi: 10.1007/s00216-012-5747-7. Epub 2012 Feb 10.

DOI:10.1007/s00216-012-5747-7
PMID:22349322
Abstract

The analytical methodology for the in vivo study of selenium metabolism using two enriched selenium isotopes has been modified, allowing for the internal correction of spectral interferences and mass bias both for total selenium and speciation analysis. The method is based on the combination of an already described dual-isotope procedure with a new data treatment strategy based on multiple linear regression. A metabolic enriched isotope ((77)Se) is given orally to the test subject and a second isotope ((74)Se) is employed for quantification. In our approach, all possible polyatomic interferences occurring in the measurement of the isotope composition of selenium by collision cell quadrupole ICP-MS are taken into account and their relative contribution calculated by multiple linear regression after minimisation of the residuals. As a result, all spectral interferences and mass bias are corrected internally allowing the fast and independent quantification of natural abundance selenium ((nat)Se) and enriched (77)Se. In this sense, the calculation of the tracer/tracee ratio in each sample is straightforward. The method has been applied to study the time-related tissue incorporation of (77)Se in male Wistar rats while maintaining the (nat)Se steady-state conditions. Additionally, metabolically relevant information such as selenoprotein synthesis and selenium elimination in urine could be studied using the proposed methodology. In this case, serum proteins were separated by affinity chromatography while reverse phase was employed for urine metabolites. In both cases, (74)Se was used as a post-column isotope dilution spike. The application of multiple linear regression to the whole chromatogram allowed us to calculate the contribution of bromine hydride, selenium hydride, argon polyatomics and mass bias on the observed selenium isotope patterns. By minimising the square sum of residuals for the whole chromatogram, internal correction of spectral interferences and mass bias could be accomplished. As a result, the tracer/tracee ratio could be calculated for each selenium-containing species and a time relationship for synthesis and degradation established. Both selenite and selenized yeast labelled with (77)Se were employed for comparative purposes.

摘要

用于研究使用两种富集硒同位素的体内硒代谢的分析方法已被修改,允许对内进行光谱干扰和质量偏差的内部校正,无论是总硒还是形态分析。该方法基于已描述的双同位素程序与基于多元线性回归的新数据处理策略的组合。代谢富集同位素 ((77)Se) 口服给予受试对象,并用第二种同位素 ((74)Se) 进行定量。在我们的方法中,考虑到在通过碰撞池四极杆 ICP-MS 测量硒同位素组成时可能发生的所有多原子干扰,并通过多元线性回归在最小化残差后计算其相对贡献。结果,所有光谱干扰和质量偏差都得到了内部校正,从而可以快速且独立地定量天然丰度硒 ((nat)Se) 和富集的 (77)Se。从这个意义上说,每个样品中的示踪剂/示踪物比的计算非常简单。该方法已应用于研究雄性 Wistar 大鼠中 (77)Se 的时间相关组织掺入,同时保持 (nat)Se 稳态条件。此外,还可以使用所提出的方法研究代谢相关信息,如尿中硒蛋白合成和硒排泄。在这两种情况下,都使用 (74)Se 作为柱后同位素稀释剂。将多元线性回归应用于整个色谱图允许我们计算溴化氢、硒化氢、氩多原子和质量偏差对观察到的硒同位素模式的贡献。通过最小化整个色谱图的残差平方和,可以对内进行光谱干扰和质量偏差的校正。结果,可以为每个含硒物种计算示踪剂/示踪物比,并建立合成和降解的时间关系。使用 ((77)Se 标记的亚硒酸盐和硒酵母进行了比较。

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