The complete table (available upon request) lists the phosphoproteins identified in RAW 264.7 cells from multiple experiments.
The table contains 3 classes of proteins: 1) proteins identified following SDS electrophoresis of anti-phosphotyrosine immunoprecipitates (PY ID) where a phosphorylation site was not identified; 2) proteins identified following IMAC enrichment of phospho-peptides from whole cell lysates of calyculin A-treated cells (IMAC) where phosphorylation site(s) were identified; and 3) proteins that were identified following anti-phosphotyrosine immunoisolation and IMAC enrichment (PY IMAC) where a phosphorylation site was identified.
Figure 2. Generation of phosphorylated proteins by phosphatase inhibitor treatment. RAW 264.7 cells were either left untreated (Ctrl), treated with 25 nM CLA (CLA), or treated with 100 uM PVD (PVD) for 30 min and lysed in SDS sample buffer. The proteins were resolved on a 10% SDS gel, transferred to nitrocellulose membranes, and immunoblotted with either an anti-phospho-threonine-proline antibody (P-Thr-Pro-101) (Panel A) or an anti-phosphotyrosine antibody (P-Tyr-100) (Panel B) from Cell Signaling Technology. The mass of molecular weight markers (M) are shown at the left.
Figure 1. Flow chart of procedure for the enrichment of phosphorylated proteins from whole-cell lysate.
References• Ficarro SB, McCleland ML, Stukenberg PT, et al. (2002) Nat. Biotechnol. 20(3), 301-305.
• Nuhse TS, Stensballe A, Jensen ON, and Peck SC (2003) Mol. Cell Proteomics 2(11), 1234-1243.
• Shu H., Chen S, Lyons K, Hsueh R, Brekken D (2003) AfCS Research Reports. Vol. 1, no. 3 [cited March 21, 2003]. Available from: http://www.signaling-gateway.org/reports/v1/DA0003.pdf
• Shu H, Chen S, Bi Q, Mumby M, Brekken DL (2004) Mol. Cell Proteomics 3(3), 279-286.
Building a Database of Phosphoproteins Present in RAW 264.7 CellsBrekken D, Bi Q, Lyons K, Sethuraman D, Shu H
Alliance for Cellular Signaling Laboratories, University of Texas Southwestern Medical Center, Dallas, TX
Abstract
A goal of the AfCS Protein Chemistry Laboratory is the identification of phosphoproteins present in the AfCS model cell systems. This poster describes the identification of a large number of phosphoproteins and phosphorylation sites in the RAW 264.7 macrophage cell line. RAW cells were treated with either tyrosine or serine/threonine phosphatase inhibitors to generate high levels of protein phosphorylation. Phosphoproteins and phosphopeptides were enriched using immuno-affinity chromatography with anti-phosphotyrosine antibodies and immobilized metal affinity chromatography (IMAC), either alone or in combination. Phosphoproteins and phosphorylation sites were then identified by tandem mass spectrometry. A total of 248 proteins and 210 distinct serine, threonine, and tyrosine phosphorylation sites were identified. The proteins identified included integral membrane proteins and proteins likely to be present at low levels in these cells. Phosphoproteins identified included kinases, phosphatases, transmembrane receptors, signaling proteins, cytoskeletal proteins, translation factors, cell adhesion proteins, and proteins involved in RNA metabolism. Many of the known proteins identified are components of macrophage signaling pathways. The list of proteins also includes a large number of proteins not previously known to be phosphorylated as well as completely novel proteins.
Acknowledgements
We would like to acknowledge Robert Cox, Laura Draper, Farah El Mazouni, and Marc Mumby from the AfCS Protein Chemistry lab for their contributions to this work.
Introduction
An important goal of the Alliance for Cellular Signaling (AfCS) is the global analysis of ligand-induced changes in protein phosphorylation. Important steps in this process are the identification of the repertoire phosphoproteins present in the AfCS model cell systems and determining their sites of phosphorylation. Due to the low abundance of many phosphorylated proteins and the fact that they are often phosphorylated at low stoichiometries, an enrichment step is usually needed in order to identify a broad spectrum of phosphorylated proteins in a given cell type. One useful method for enrichment of phosphoproteins is immuno-affinity isolation with antibodies that recognize phosphorylated amino acids. Anti-phosphotyrosine antibodies are particularly useful in this regard (Shu et al., 2003). Enrichment of phosphopeptides with immobilized metal affinity chromatography (IMAC) has allowed the identification of hundreds of phosphoproteins and phosphorylation sites in yeast (Ficarro et al., 2002), Arabidopsis plasma membrane proteins (Nuhse et al., 2003), and in WEHI 231 B lymphoma cells (Shu et al., 2004) . We have used a combination of these approaches to identify phosphoproteins and their phosphorylation sites in the murine RAW 264.7 macrophage cell line following treatment with phosphatase inhibitors. The list of proteins and phosphorylation sites is presented as a supplement to this poster. Because this is an ongoing project, the table will be updated periodically and eventually incorporated into a database directly accessible through the AfCS website.
Results
Conclusions
• The phosphoprotein table contains 481 separate protein identifications that identify a total of 248 proteins from three different experimental approaches.
• 210 unique phosphorylation sites were identified (59 P-Tyr, 116 P-Ser, and 35 P-Thr).
• A total of 24 novel proteins were also identified. These are listed as “hypothetical proteins”, “Riken cDNAs”, or “Unknown protein products”. The identification of peptides corresponding to these proteins not only established that they are expressed in RAW 264.7 cells, but also shows they are phosphorylated.
• A large number of proteins known to be involved in signaling in macrophages and other immune cells were also identified (Table 2).
• This information will be used to expand the signaling “parts list” identified in these cells and allow the development of probes that will be used to monitor ligand-dependent changes in protein phosphorylation.
Methods
PVD
CLAP-Tyr IP
Trypsin1D gel
Trypsin
Trypsin
IMAC
LC-MS/MS(IMAC)
Esterification
LC-MS/MS(PY ID)
IMAC
P-Tyr P-Ser/P-Thr
LC-MS/MS(PY IMAC)
25
37
50
75100
250150
25
37
50
75100
250150
Ctrl PVDCtrl CLAA.
P-Thr-Pro
B.
P-Tyr
M M
Protein Name Protein GI Phosphopeptide
Phosphor-ylated amino acid #
highest Mascot score
# of pept
Locus Link AfCS ID Expt # Type
Btk 7709994 YVLDDEYT*SSVGSK T552 12229 A000038 235PY
IMAC
Cortactin 15030315 GFGGKY*GIDK Y199 13043 235PY
IMAC
DEAD/H (Asp-Glu-Ala-Asp/His) box polypeptide 3, X-linked 6753620 163 4 13205 294 PY ID
Fc receptor, IgE, high affinity I, gamma polypeptide 6753830 SQETY*ETLKHEKPPQ Y76 14127 A000543 326 IMAC
Hematopoietic cell specific Lyn substrate 1; HS1 13938627 DY*SHGFGGR Y153 15163 A001149 241
PY IMAC
Myosin X 9506909 105 3 17909 A001583 232b PY ID
Paxillin beta 22902122YAHQQPPS*PLPVY*SSSAK S83, Y88 19303 A001736 236
PY IMAC
Phospholipase C, gamma 2 26986603 DINSLY*DVSR Y753 234779 A001810 236
PY IMAC
PTK2; FAK 6679741 272 10 14083 A000900 232b PY ID
Shp1; PTPN6 7305133 166 2 15170 A002156 294 PY ID
Table 1. Sample of RAW Phosphoprotein table. The table lists the name and protein GI number that was identified. Where possible, the protein name is derived from the NCBI LocusLink entry. If a phosphorylation site was identified, the phosphopeptide detected is listed with an asterisk (*) following the phosphorylated amino acid. There is a column that lists the residue number of the identified phosphorylation site(s) within the amino acid sequence of the protein. Note that these numbers are based on the sequence listed in the corresponding GI entry and do not always represent the full-length sequence. For proteins that were identified directly by LC-MS/MS (i.e., without an IMAC step), the highest Mascot score and # of peptides detected are listed. The Mascot score is the absolute probability that the observed match is a random event (-10*Log(P), where P is the probability that the observed match is a random event). Mascot scores greater than 62 were considered significant (p<0.05). If available, the LocusLink and AfCS ID numbers are also listed in the table. The table also includes columns listing the number and type of experiment where the protein was identified.
Btk Lck
Dok1 Lyn
Dok2 PLC2
FcεRI SHIP
Fgr Shp1
Fyb/SLAP130 Shp2
Fyn SHPS-1
Hematopoietic cell specific Lyn substrate/HS1 SLP-76
Immunoglobulin superfamily member 4
Protein Site(s) identified Activation Loop residue
Fgr Y400 Y400
Btk T552 Y551
Lck T394 Y393
Lyn T397 Y396
Table 2. A table listing a sample of identified proteins that are known to be involved in immune signaling.
Table 3. Phosphorylation sites identified and activation loop residues in several proteins identified. The tyrosine phosphorylation sites identified in Fgr is a known sites within the activation loop that is associated with activation of kinase activity. In contrast, the phosphorylation sites identified in Btk, Lck, and Lyn were all threonine residues immediately adjacent to the activating tyrosine phosphorylation site of these kinases. These threonine phosphorylation sites were all identified in pervanadate treated cells.
Phosphoprotein Table
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