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Protein turnover: Measurement of proteome dynamics by whole animal metabolic labelling with stable isotope labelled amino acids

机译:蛋白质更新:通过用稳定同位素标记的氨基酸进行全动物代谢标记来测量蛋白质组动力学

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摘要

The measurement of protein turnover in tissues of intact animals is obtained by whole animal dynamic labelling studies, requiring dietary administration of precursor label. It is difficult to obtain full labelling of precursor amino acids in the diet and if partial labelling is used, calculation of the rate of turnover of each protein requires knowledge of the precursor relative isotope abundance (RIA). We describe an approach to dynamic labelling of proteins in the mouse with a commercial diet supplemented with a pure, deuterated essential amino acid. The pattern of isotopomer labelling can be used to recover the precursor RIA, and sampling of urinary secreted proteins can monitor the development of liver precursor RIA non-invasively. Time-series analysis of the labelling trajectories for individual proteins allows accurate determination of the first order rate constant for degradation. The acquisition of this parameter over multiple proteins permits turnover profiling of cellular proteins and comparisons of different tissues. The median rate of degradation of muscle protein is considerably lower than liver or kidney, with heart occupying an intermediate position.
机译:完整动物组织中蛋白质更新的测量是通过整个动物动态标记研究获得的,需要饮食上给予前体标记。很难在饮食中获得前体氨基酸的完整标记,如果使用部分标记,则每种蛋白质的周转率的计算都需要了解前体相对同位素丰度(RIA)。我们描述了一种用商业饮食补充纯净,氘代必需氨基酸的小鼠中动态标记蛋白质的方法。同位素标记的模式可用于恢复前体RIA,尿液分泌蛋白的采样可无创监测肝脏前体RIA的发展。对单个蛋白质的标记轨迹进行时间序列分析,可以准确确定降解的​​一级速率常数。在多种蛋白质上获取此参数可对细胞蛋白质进行周转分析,并比较不同组织。肌肉蛋白的中位降解率明显低于肝脏或肾脏,心脏处于中间位置。

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