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Measurement of the Isotope Enrichment of Stable Isotope-Labeled Proteins Using High-Resolution Mass Spectra of Peptides

机译:使用肽的高分辨率质谱测定稳定同位素标记的蛋白质的同位素富集

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Stable isotope-enriched molecules are used as internal standards and as tracers of in vivo substrate metabolism. The accurate conversion of measured ratios in the mass spectrometer to mole ratios is complicated because a polyatomic molecule containing enriched atoms will result in a combinatorial distribution of isotopomers depending on the enrichment and number of "labeled" atoms. This effect could potentially cause a large error in the mole ratio measurement depending on which isotope peak or peaks were used to determine the ratio. We report a computational method that predicts isotope distributions over a range of enrichments and compares the predicted distributions to experimental peptide isotope distributions obtained by Fourier transform ion cyclotron resonance mass spectrometry. Our approach is accurate with measured enrichments within 1.5percent of expected isotope distributions. The method is also precise with 4.9, 2.0, and 0.8percent relative standard deviations for peptides containing 59, 79, and 99 atom percent excess ~(15)N, respectively. The approach is automated making isotope enrichment calculations possible for thousands of peptides in a single (mu)LC-FTICR-MS experiment.
机译:稳定的富含同位素的分子被用作内标和体内底物代谢的示踪剂。质谱仪中测得的比率到摩尔比率的准确转换非常复杂,因为包含富集原子的多原子分子将根据“标记”原子的富集和数量导致同位素异构体的组合分布。这种影响可能会在摩尔比测量中引起较大的误差,具体取决于哪个同位素峰或多个峰用于确定该比率。我们报告了一种计算方法,该方法可预测富集范围内的同位素分布,并将预测的分布与通过傅立叶变换离子回旋共振质谱法获得的实验肽同位素分布进行比较。我们的方法是准确的,测得的富集度在预期同位素分布的1.5%之内。对于分别含有59、79和99个原子百分比过量〜(15)N的肽,该方法的相对标准偏差也分别为4.9%,2.0%和0.8%。该方法是自动化的,使得在单个(μ)LC-FTICR-MS实验中数千种肽的同位素富集计算成为可能。

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