Modeling cell line-specific recruitment of signaling proteins to the insulin-like growth factor 1 receptor
Fig 1
IGF1R phosphotyrosine contact map in HeLa S3 cells.
(A) Ligand-free and inactive IGF1R. Prior to crosslinking of dissimilar sites S1 and S2 of each IGF1R protomer in a dimer, the two kinase domains are not in contact and are thus unable to autophosphorylate receptor tyrosines. (B) IGF1R phosphotyrosine interactions in HeLa S3 cells. Each IGF1R in an IGF1R dimer contains six autophosphorylation tyrosine sites, labeled “Y” followed by the site’s position within the polypeptide chain (according to UniProt numbering). The kinase domains of each IGF1R subunit are labeled accordingly and encompass the region spanning positions 999 to 1274. Autophosphorylation and dephosphorylation of activated (IGF1-crosslinked) receptors in a dimer occur at the tyrosine sites indicated. Signaling proteins containing SH2 and/or PTB domains are recruited to their cognate tyrosine sites in a phosphorylated IGF1R dimer as indicated by the colored lines that begin at a tyrosine site and end at the protein that is recruited to that site.