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N-15/N-14 position-specific isotopic analyses of polynitrogenous amino acids

机译:多氮氨基酸的N-15 / N-14位置特异性同位素分析

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N-15/N-14 isotope ratios are widely used to study processes and systems involving amino acids. Nitrogen isotope fractionation in biological processes occurs primarily at sites of bond-breaking and formation; the finest discrimination for "isotopic fingerprinting" and studies of isotopic fluxes is thus obtained at the position-specific level. While there are numerous reports of natural intramolecular carbon isotope variability, there are no literature reports of 15N/14N position-specific isotopic analysis (N-PSIA) of biologically relevant molecules. We report a methodology for high-precision N-PSIA of four polynitrogenous alpha-amino acids (asparagine, glutamine, lysine, histidine) and the first survey of natural intramolecular 15N/14N in these biomolecules. Selective liberation of N-atoms from multiple commercial standards of each parent amino acid was achieved by an appropriate enzymatic reaction or by acid hydrolysis. 15N/14N measurements were performed on N-ethoxycarbonyl ethyl ester derivatives of the parent amino acids and their analogues by gas chromatography combustion isotope ratio mass spectrometry, and the average precision for replicate injections was found to be SD(delta(15)N) = 0.3parts per thousand. Position-specific delta(15)N values of the parent amino acid were directly observed or indirectly calculated using mass balance. The average precision obtained for directly measured positions was SD(delta(15)N) = 0.2-0.4parts per thousand. The average precision for indirectly obtained positions was SD(delta(15)N) = 0.6-1.3parts per thousand as a result of propagation of errors. Enrichment in the side chain-N with respect to the peptide-N was observed in nearly all of the amino acid sources, most notably in asparagine (average Deltadelta(side-peptide) = + 11parts per thousand), which may be indicative of its method of production. In some cases, it was possible to distinguish commercial sources by N-PSIA that could not be distinguished at the compound-specific level.
机译:N-15 / N-14同位素比率广泛用于研究涉及氨基酸的过程和系统。生物过程中的氮同位素分级分离主要发生在键断裂和形成的位置;这样就可以在特定位置上获得“同位素指纹图谱”的最佳判别和同位素通量的研究。尽管有许多关于自然分子内碳同位素变化的报道,但没有关于生物学相关分子的15N / 14N位置特异性同位素分析(N-PSIA)的文献报道。我们报告了四个多氮α-氨基酸(天冬酰胺,谷氨酰胺,赖氨酸,组氨酸)的高精度N-PSIA方法,并首次对这些生物分子中的天然分子内15N / 14N进行了调查。通过适当的酶促反应或酸水解,可以从多种母体氨基酸的多种商业标准物中选择性释放N原子。通过气相色谱燃烧同位素比质谱法对母体氨基酸的N-乙氧基羰基乙酯衍生物及其类似物进行15N / 14N测量,发现重复进样的平均精度为SD(delta(15)N)=千分之0.3直接观察或使用质量平衡间接计算母体氨基酸的位置特异性delta(15)N值。直接测量位置获得的平均精度为SD(delta(15)N)= 0.2-0.4份/千。由于误差的传播,间接获得的位置的平均精度为SD(delta(15)N)= 0.6-1.3份/千。在几乎所有氨基酸来源中均观察到相对于肽N富集侧链N,最显着的是天冬酰胺(平均Deltadelta(side-peptide)= + 11千分之一),这可能表明其生产方法。在某些情况下,可以通过N-PSIA区分商业来源,而在化合物特定水平上则无法区分。

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