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选择性富集新合成蛋白质进行定量分泌组分析。

Selective enrichment of newly synthesized proteins for quantitative secretome analysis.

机构信息

EMBL, Genome Biology Unit, Heidelberg, Germany.

出版信息

Nat Biotechnol. 2012 Oct;30(10):984-90. doi: 10.1038/nbt.2356. Epub 2012 Sep 23.

Abstract

Secreted proteins constitute a large and biologically important subset of proteins that are involved in cellular communication, adhesion and migration. Yet secretomes are understudied because of technical limitations in the detection of low-abundance proteins against a background of serum-containing media. Here we introduce a method that combines click chemistry and pulsed stable isotope labeling with amino acids in cell culture to selectively enrich and quantify secreted proteins. The combination of these two labeling approaches allows cells to be studied irrespective of the complexity of the background proteins. We provide an in-depth and differential secretome analysis of various cell lines and primary cells, quantifying secreted factors, including cytokines, chemokines and growth factors. In addition, we reveal that serum starvation has a marked effect on secretome composition. We also analyze the kinetics of protein secretion by macrophages in response to lipopolysaccharides.

摘要

分泌蛋白是一类在细胞通讯、黏附和迁移中发挥重要作用的蛋白质,它们构成了蛋白质的一个很大的且具有生物学意义的子集。然而,由于在含有血清的培养基背景下检测低丰度蛋白质的技术限制,分泌组学的研究还不够充分。在这里,我们介绍了一种结合点击化学和脉冲稳定同位素标记与细胞培养中氨基酸的方法,该方法可选择性地富集和定量分泌蛋白。这两种标记方法的结合使得无论背景蛋白质的复杂程度如何,都可以对细胞进行研究。我们对各种细胞系和原代细胞进行了深入和差异的分泌组学分析,定量了包括细胞因子、趋化因子和生长因子在内的分泌因子。此外,我们还揭示了血清饥饿对分泌组组成有显著影响。我们还分析了巨噬细胞对脂多糖反应时的蛋白质分泌动力学。

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