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首页> 外文期刊>Analytical Biochemistry: An International Journal of Analytical and Preparative Methods >Stable isotope labeling method targeting terminal tyrosine for relative peptide quantitation using mass spectrometry
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Stable isotope labeling method targeting terminal tyrosine for relative peptide quantitation using mass spectrometry

机译:靶向末端酪氨酸的稳定同位素标记方法,用于使用质谱进行相对肽定量

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摘要

Many neuropeptides lack suitable amino acid residues for modification by existing selective isotope labeling methods and use in relative quantitation by mass spectrometry. To address this issue, a new stable isotope labeling method that targets tyrosine residues by coupling with light cysteine (d_0) or heavy cysteine (d_2) in the presence of tyrosinase was developed. Optimal derivatization conditions for 1μM leucine-enkephalin were achieved when 10mM cysteine and 200U/ml tyrosinase at pH 6.8 to 7.2 were used for a 60-min incubation period at room temperature. Under these conditions, leucine-enkephalin present at concentrations as low as 125nM was successfully labeled. When comparisons between the lightly labeled (d_0) and heavily labeled (d_2) forms were made, a discrepancy between the actual concentration ratio and the raw peak intensity ratio was observed; this is due to the overlap of an isotopic peak of the d_0 with the monoisotopic peak of d_2. Fortunately, this discrepancy can be corrected by one of two simple computational approaches described. The quantitative labeling of this method to neuropeptides with the terminal tyrosine was confirmed and provides an alternative when other selective isotope-coded affinity tagging methods are not suitable.
机译:许多神经肽缺乏合适的氨基酸残基,无法通过现有的选择性同位素标记方法进行修饰,并且无法通过质谱法进行相对定量。为了解决这个问题,开发了一种新的稳定同位素标记方法,该方法通过在酪氨酸酶存在下与轻度半胱氨酸(d_0)或重度半胱氨酸(d_2)偶联来靶向酪氨酸残基。当在室温下将60m的10mM半胱氨酸和200U / ml酪氨酸酶在pH值为6.8至7.2的条件下使用60分钟时,可达到1μM亮氨酸-脑啡肽的最佳衍生条件。在这些条件下,成功地标记了浓度低至125nM的亮氨酸-脑啡肽。当比较轻度标记(d_0)和重度标记(d_2)形式时,观察到实际浓度比与原始峰强度比之间存在差异。这是因为d_0的同位素峰与d_2的单同位素峰重叠。幸运的是,可以通过上述两种简单的计算方法之一来纠正这种差异。确认了使用末端酪氨酸对神经肽进行定量标记的方法,当其他选择性同位素编码的亲和标记方法不适用时,该方法可提供替代方法。

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