1. The principle of the immuno-SILAC method.
The principle of the immuno-SILAC method.A, absolute protein quantification using PrESTs as the internal standard. Peptides originating from the albumin binding protein (ABP) tag (yellow) are used to quantify each PrEST against an ultrapurified ABP protein standard. The PrEST can thereafter be used as an internal standard in unknown samples to quantify the corresponding endogenous protein (red) in LC-MS. B, schematic representation of the immuno-SILAC workflow. Highly purified and accurately quantified isotopic heavy-labeled PrESTs are spiked into cell lysates prior to trypsin digestion, thereby minimizing the risk of differences arising between samples and standards during sample preparation. Antibodies coupled to magnetic solid phase support enrich target peptides from the digested sample, and the endogenous protein concentration is calculated from the ratio of heavy to light peptides detected via MS. C, comparison between the SISCAPA technology (7) using heavy-labeled peptides (blue) and immuno-SILAC using heavy-labeled protein fragments (green) for absolute protein quantification.
Fredrik Edfors et al. Mol Cell Proteomics 2014;13:
© 2014 by The American Society for Biochemistry and Molecular Biology, Inc.