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Acid-Catalyzed Oxygen-18 Labeling of Peptides

机译:肽的酸催化氧18标记

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In enzymatic ~(18)O-labeling strategies for quantitative proteomics, the exchange of carboxyl oxygens at low pH is a common, undesired side reaction. We asked if acid-catalyzed back exchange could interfere with quantitation and whether the reaction itself could be used as method for introducing ~(18)O label into peptides. Several synthetic peptides were dissolved in dilute acid containing 50percent (v/v) H_(2)~(18)O and incubated at room temperature. Aliquots were removed over a period of 3 weeks and analyzed by tandem mass spectrometry (MS/MS). ~(18)O-incorporation ratios were determined by linear regression analysis that allowed for multiple stable-isotope incorporations. At low pH, peptides exchanged their carboxyl oxygen atoms with the aqueous solvent. The isotope patterns gradually shifted to higher masses until they reached the expected binomial distribution at equilibrium after approx11 days. Reaction rates were residue- and sequence-specific. Due to its slow nature, the acid-catalyzed back exchange is expected to minimally interfere with enzymatic ~(18)O-labeling studies provided that storage and analysis conditions minimize low-pH exposure times. On its own, acid-catalyzed ~(18)O labeling is a general tagging strategy that is an alternative to the chemical, metabolic, and enzymatic isotope-labeling schemes currently used in quantitative proteomics.
机译:在定量蛋白质组学的酶促〜(18)O标记策略中,低pH值下羧基氧的交换是常见的不良反应。我们询问了酸催化的反向交换是否会干扰定量分析,以及反应本身是否可用作将〜(18)O标记引入肽的方法。将几种合成肽溶于含有50%(v / v)H_(2)〜(18)O的稀酸中,并在室温下孵育。在3周内取出等分试样,并通过串联质谱(MS / MS)进行分析。通过线性回归分析确定〜(18)O的掺入比例,该分析允许多次稳定的同位素掺入。在低pH下,肽与水性溶剂交换其羧基氧原子。同位素模式逐渐转移到更高质量,直到大约11天后达到平衡的预期二项式分布。反应速率是残基和序列特异性的。由于其缓慢的性质,只要存储和分析条件使低pH值的暴露时间最小化,酸催化的反向交换有望最小程度地干扰酶促〜(18)O标记研究。单独使用酸催化〜(18)O标记是一种通用的标记策略,可以替代目前在定量蛋白质组学中使用的化学,代谢和酶促同位素标记方案。

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