Quantitative Proteomic Analysis Using Isobaric Protein Tags Enables Rapid Comparison of Changes in Transcript and Protein Levels in Transformed Cells

Richard D Unwin,Andrew Pierce,Rod B Watson,David W Sternberg,Anthony D Whetton

doi:10.1074/mcp.m400193-mcp200

Abstract

Isobaric tags for relative and absolute quantitation, an approach to concurrent, relative quantification of proteins present in four cell preparations, have recently been described. To validate this approach using complex mammalian cell samples that show subtle differences in protein levels, a model stem cell-like cell line (FDCP-mix) in the presence or absence of the leukemogenic oncogene TEL/PDGFRbeta has been studied. Cell lysates were proteolytically digested, and peptides within each sample were labeled with one of four isobaric, isotope-coded tags via their N-terminal and/or lysine side chains. The four labeled samples are mixed and peptides separated by two-dimensional liquid chromatography online to a mass spectrometer (LC-MS). Upon peptide fragmentation, each tag releases a distinct mass reporter ion; the ratio of the four reporters therefore gives relative abundances of the given peptide. Relative quantification of proteins is derived using summed data from a number of peptides. TEL/PDGFRbeta leukemic oncogene-mediated changes in protein levels were compared with those seen in microarray analysis of control and transfected FDCP-mix cells. Changes at the protein level in most cases reflected those seen at the transcriptome level. Nonetheless, novel differences in protein expression were found that indicate potential mechanisms for effects of this oncogene.

Highlights

Isobaric tags for relative and absolute quantitation, an approach to concurrent, relative quantification of proteins present in four cell preparations, have recently been described
Comparing the ICAT reagent approach with two-dimensional gel electrophoresis, demonstrates that neither offers comprehensive coverage of a proteome [4]. This is true in part because many proteins do not contain cysteine, the amino acid used for covalent attachment of the isotopomer in ICAT reagents
Cell Line Preparation and Culture—FDCP-Mix cells were transduced with TEL/PDGFR␤ using a murine stem cell retroviral vector as described previously [8]

Summary

EXPERIMENTAL PROCEDURES

Cell Line Preparation and Culture—FDCP-Mix cells were transduced with TEL/PDGFR␤ using a murine stem cell retroviral vector as described previously [8]. To label the peptides with iTRAQ reagent (Applied Biosystems, Warrington, UK), one unit of label (defined as the amount required to label 100 ␮g of protein) was thawed and reconstituted in 70 ␮l of ethanol, with vortexing for 1 min. 60 ␮l of the peptide sample was loaded onto a 15-cm reversed phase C18 column (75 ␮m i.d.) using an UltiMate pump (LC Packings, Amsterdam, The Netherlands) and separated over a 120-min solvent gradient from 5.9% (v/v) acetonitrile/0.1% (v/v) formic acid to 41% (v/v) acetonitrile/ 0.1% (v/v) formic acid on-line to a QSTAR XL mass spectrometer (Applied Biosystems). ProQUANT pooled data from all LC-MS runs Assessment of these parameters for peptide and protein identification is described in Supplemental Table I.

RESULTS

Chaperonin groEL

DISCUSSION