Abstract
Quantitation of protein abundance is a vital component in the proteomic analysis of biological systems, which can be achieved by differential stable isotopic labeling. To analyze tissue-derived samples, the isotopic labeling can be performed using chemical labeling of the peptides post-digestion. Standard chemical labeling procedures often require many manual sample handling steps, reducing the accuracy of measurements. Here, we describe a fully automated, online (in nanoLC columns), labeling procedure, which allows protein quantitation using differential isotopic dimethyl labeling of peptide N termini and lysine residues. We show that the method allows reliable quantitation over a wide dynamic range and can be used to quantify differential protein abundances in lysates and, more targeted, differences in composition between purified protein complexes. We apply the method to determine the differences in composition between bovine liver and spleen 20 S core proteasome complexes. We find that although all catalytically active immunoproteasome subunits were up-regulated in spleen (compared with liver), only one of the normal catalytic subunits was down-regulated, suggesting that the tissue-specific immunoproteasome assembly is more diverse than previously assumed.
Highlights
Quantitation of protein abundance is a vital component in the proteomic analysis of biological systems, which can be achieved by differential stable isotopic labeling
The most common way to analyze and compare whole proteomes was by two-dimensional polyacrylamide gel electrophoresis (PAGE), with quantitative information being gleaned from the intensity of the spots observed after staining the separated proteins in the gel
One of the most efficient reactions for chemical labeling of peptides is the specific dimethylation of free amines by reductive amination using formaldehyde and cyanoborohydride [7]
Summary
Quantitation of protein abundance is a vital component in the proteomic analysis of biological systems, which can be achieved by differential stable isotopic labeling. We describe a fully automated, online (in nanoLC columns), labeling procedure, which allows protein quantitation using differential isotopic dimethyl labeling of peptide N termini and lysine residues. One of the most efficient reactions for chemical labeling of peptides is the specific dimethylation of free amines (peptide N termini and Lysine residues) by reductive amination using formaldehyde and cyanoborohydride [7]. In this reaction, which is performed in near neutral conditions (between pH 6 and pH 8.5), the primary amines react with formaldehyde to create a Schiff base, which is reduced by the cyanoborohydride. We apply the method to determine quantitatively differences in composition between proteasomes purified from different tissues
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