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通过整合同位素标记、化学富集和多重蛋白质组学技术,同时定量糖蛋白降解和合成速率。

Simultaneous Quantitation of Glycoprotein Degradation and Synthesis Rates by Integrating Isotope Labeling, Chemical Enrichment, and Multiplexed Proteomics.

机构信息

School of Chemistry and Biochemistry and the Petit Institute for Bioengineering and Bioscience, Georgia Institute of Technology , Atlanta, Georgia 30332, United States.

出版信息

Anal Chem. 2017 Oct 3;89(19):10361-10367. doi: 10.1021/acs.analchem.7b02241. Epub 2017 Sep 13.

Abstract

Protein glycosylation is essential for cell survival and regulates many cellular events. Reversible glycosylation is also dynamic in biological systems. The functions of glycoproteins are regulated by their dynamics to adapt the ever-changing inter- and intracellular environments. Glycans on proteins not only mediate a variety of protein activities, but also creates a steric hindrance for protecting the glycoproteins from degradation by proteases. In this work, a novel strategy integrating isotopic labeling, chemical enrichment and multiplexed proteomics was developed to simultaneously quantify the degradation and synthesis rates of many glycoproteins in human cells. We quantified the synthesis rates of 847 N-glycoproteins and the degradation rates of 704 glycoproteins in biological triplicate experiments, including many important glycoproteins such as CD molecules. Through comparing the synthesis and degradation rates, we found that most proteins have higher synthesis rates since cells are still growing throughout the time course, while a small group of proteins with lower synthesis rates mainly participate in adhesion, locomotion, localization, and signaling. This method can be widely applied in biochemical and biomedical research and provide insights into elucidating glycoprotein functions and the molecular mechanism of many biological events.

摘要

蛋白质糖基化对于细胞存活至关重要,并调节许多细胞事件。生物系统中的可逆糖基化也是动态的。糖蛋白的功能受其动力学调节,以适应不断变化的细胞内外环境。蛋白质上的聚糖不仅介导多种蛋白质活性,还为糖蛋白免受蛋白酶降解创造了空间位阻。在这项工作中,我们开发了一种新的策略,将同位素标记、化学富集和多重蛋白质组学相结合,以同时定量测定人细胞中许多糖蛋白的降解和合成速率。我们在生物学重复实验中定量测定了 847 种 N-糖蛋白的合成速率和 704 种糖蛋白的降解速率,其中包括许多重要的糖蛋白,如 CD 分子。通过比较合成和降解速率,我们发现由于细胞在整个时间过程中仍在生长,因此大多数蛋白质具有更高的合成速率,而一小部分合成速率较低的蛋白质主要参与黏附、运动、定位和信号转导。这种方法可以广泛应用于生化和生物医学研究,并为阐明糖蛋白功能和许多生物事件的分子机制提供新的见解。

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