(Received for publication, October 24, 1995; and in revised form, November 30, 1995)
From the
Shc is an Src homology 2 (SH2) domain protein thought to be an important component of the signaling pathway leading from cell surface receptors to Ras. A new phosphotyrosine interaction (PI) domain (also known as the phosphotyrosine binding (PTB) domain) has been described in the amino terminus of Shc. The Shc PI domain binding specificity is dependent on residues lying amino-terminal to the phosphotyrosine rather than carboxyl-terminal as is seen with SH2 domains. We randomly mutagenized the Shc PTB/PI domain in an effort to identify residues in the domain crucial for interaction with phosphotyrosine-containing peptides. We then screened the mutants for binding to the tyrosine-phosphorylated carboxyl-terminal tail of the epidermal growth factor (EGF) receptor. Most striking were mutations that altered a phenylalanine residue in block 4 of the domain severely impairing PI domain function. This phenylalanine residue is conserved in all but one subfamily of PI domains that have been identified to date. Reconstitution of this phenylalanine mutation into full-length Shc created a protein unable to interact with the EGF receptor in living cells.
Controlled protein interactions play an important role in signal
transduction. One example is the interaction of cytoplasmic signaling
proteins with tyrosine-phosphorylated growth factor
receptors(1, 2, 3) . One large class of
molecules that binds to tyrosine-phosphorylated receptors contains SH2 ()domains. Recently, a second domain has been described that
binds to tyrosine-phosphorylated peptides. This domain that we called
the PI domain, also known as the phosphotyrosine binding (PTB) domain,
was first described in the amino terminus of
Shc(4, 5, 6) . Shc also contains an SH2
domain and appears to be important in Ras activation. Shc becomes
tyrosine-phosphorylated after cell activation with a large number of
cytokines and growth factors (7, 8, 9) creating a high affinity binding
site for the SH2 domain of Grb2. Grb2 is in turn complexed to the Son
of Sevenless Ras guanine nucleotide exchange factor that converts Ras
from its inactive GDP-bound state to its active GTP-bound
state(1, 2, 3) .
The exact role of the SH2 domain versus the PI domain in Shc signaling has not been determined. The binding of the PI domain to phosphotyrosine-containing peptides differs from SH2 domain binding in that its specificity is determined by residues lying amino-terminal to the phosphotyrosine(6, 10, 11, 12, 13, 14, 15) . Due to this difference in specificity it is assumed that the structural basis of interactions between phosphopeptides and the PI domain will differ from those used by SH2 domains. We have identified domains in several different proteins that have primary sequence similarity with the PI domain of Shc(16) . In an effort to understand residues in the PI domain important in mediating binding to phosphorylated peptides, we performed random mutagenesis of the Shc PI domain and screened the mutants for binding to tyrosine-phosphorylated EGF receptor. We have identified several different mutations within the domain that impair its binding ability.
Figure 1:
A, Shc 1-209/Myc pTOPE vector.
Shc 1-209 was subcloned into the pTOPE vector with a Myc epitope
at its carboxyl terminus as described under ``Experimental
Procedures.'' The pTOPE vector allows protein expression in
bacteria expressing T7 polymerase. cDNA encoding Shc 76-209 that
had been subjected to random mutagenesis by PCR was cloned into the BstEII and PstI site. The mutagenesis did not include
the Myc tag or pTOPE vector. B, screening of bacterial
colonies expressing the mutagenized Shc PI domain. The mutagenized Shc
1-209/Myc pTOPE plasmids were used to transform bacteria and
plated to yield approximately 150 colonies/100-mm plates. After
overnight growth, the colonies were transferred to nitrocellulose and
lysed. After blocking the filters, they were probed with the P-labeled carboxyl terminus of the EGF receptor (EGFR), washed, and exposed to film. After autoradiography,
the filters were reprobed with an anti-Myc antibody using colorimetric
detection. The autoradiograms were then aligned with the Myc
antibody-stained filters. The panel on the right shows screening for Myc tag expression using monoclonal antibody
9E10 against the Myc epitope. The panel on the left shows binding of labeled EGF receptor to the same filter. The arrow depicts a colony selected for further analysis with
normal binding of the Myc antibody but defective EGF receptor
binding.
We subcloned the cDNA encoding the amino terminus of murine p52 Shc (Fig. 1A) into the pTOPE vector allowing expression in bacteria expressing T7 polymerase. We added a Myc epitope in-frame at amino acid 209 that contained a unique XhoI site at its carboxyl terminus and introduced a PstI site between the Myc epitope and the PI domain. We then created a library of PI domains with mutations running from amino acid 76 to 209 of p52 Shc but excluding the Myc epitope as described under ``Experimental Procedures.'' Bacterial colonies expressing the library of PI domain mutants were lifted onto nitrocellulose and screened for EGF receptor binding and Myc epitope expression. Colonies selected for further study stained positive for Myc (indicating full-length protein expression) but had reduced EGF receptor binding. Such an example is shown in Fig. 1B. Plasmids were isolated from these bacterial colonies and subcloned into the pGEX4T-1 vector. This allowed the production of soluble GST fusion proteins that were spotted on nitrocellulose at a known concentration and probed with the radiolabeled EGF receptor. These plasmids were also subjected to DNA sequencing. Several of the mutants that had more than one mutation were not further analyzed. The binding of some of the PI domains with single point mutations and binding less than 50% of control are displayed in Fig. 2A while the sites of the mutations are shown in Fig. 2B. The binding percentage compared with wild type, displayed in Fig. 2B, represents an average of the binding to 100 and 200 ng of GST fusion protein.
Figure 2:
Identification and characterization of PI
domain mutants. A, binding of P-labeled EGF
receptor to PI domain mutants. PI domain mutants identified using the
method in Fig. 1were subcloned into pGEX4T-1 vector. GST fusion
proteins were prepared as described under ``Experimental
Procedures'' with 200, 100, and 50 ng spotted on nitrocellulose.
The wild type (WT) and mutant PI domains were then probed with
P-labeled EGF receptor. For quantitation, squares were cut
from the filters and Cerenkov counts determined. Duplicate filters
spotted with GST fusion protein and probed with anti-Myc were utilized
to ensure comparable amounts of protein were spotted for each protein
(results not shown). B, sites of PI domain mutations. The PI
domain point mutations isolated by random mutagenesis are listed above
the wild type Shc sequence. The numbers in parentheses represent the binding of GST fusion proteins containing these
mutations to the EGF receptor as a percent of wild type control. The numbers represent an average of the binding to 100 and 200 ng
of GST fusion protein. C, effects of PI and SH2 domain
mutagenesis on binding to EGF receptor (EGFR). GST fusion
proteins (3 µg of Shc PI domain; 10 µg of Shc SH2 domain) were
immobilized on glutathione beads, and EGF-stimulated HER14 cell lysate
was added (1.5 mg of protein). After incubation for 90 min at 4 °C,
the beads were washed with radioimmune precipitation buffer and the
bound proteins separated by SDS gel. After transferring to
nitrocellulose, the bound EGF receptor was detected by immunoblotting
with anti-phosphotyrosine antibodies. As a control, lysate (100 µg)
was run directly on the gel (far right lanes). It should be
noted that although the binding of the wild type SH2 and PI domain (PID) appear equivalent, three times as much SH2 domain was
used.
Also displayed in Fig. 2A is the binding of two mutations that were created based on the previously published PI domain alignment (16) . In this alignment two absolutely conserved residues were identified, a glycine at residue 58 and a serine at residue 151 of p52 Shc. The S151A mutation had impaired binding and mapped to a region of Shc where several of the random mutants were located. This mutation resulted in a binding approximately 1.0% of wild type. No binding was detected in the G58A mutation. However, a large fraction of this protein became insoluble when expressed in bacteria, suggesting that this mutation adversely affected the conformation of the protein.
The effects of two of the phenylalanine mutations on PI domain binding are shown using a different assay in Fig. 2C (left panel). In this assay, the GST fusion proteins were immobilized on glutathione-agarose, and cell lysates containing tyrosine-phosphorylated EGF receptor were added. Both of the phenylalanine mutations, F198V and F152L, markedly reduced the PI domain binding in agreement with the results shown in Fig. 2A. Shown for comparison in the right panel of Fig. 2C is the effect of mutating arginine 397 of the Shc SH2 domain to lysine. This is an arginine within the SH2 domain that is crucial for phosphotyrosine interaction. As expected this mutation completely abolished the ability of the Shc SH2 domain to bind to the EGF receptor.
The alignment presented in Fig. 3maps the mutations we have generated to the conserved blocks found in PI domains(16) . The blocks were confirmed by another round of sequence data base searches in which we were able to retrieve 10 more members of the PI domain family. Among them are the partial sequences of two new proteins, Est2 and FE6L, that have been identified in this work. FE6L (for FE65-like protein) belongs to the FE65 subfamily while Est2 appears to be yet another divergent member of the PI domain family. The other 8 sequences are probably orthologues of existing PI domain containing proteins which, nevertheless, indicate conserved regions in the alignment. The relationship of the PTB domains of IRS-1 and IRS-2 to our PI domain alignment is not clear(6, 22) . We have not been able to include them without severely impairing the quality of the PI domain alignment.
Figure 3: Alignment of the conserved blocks of PI domains with mutations generated in this study. This figure represents an extension of our previously published alignment (16) with data base search and alignments performed as described previously. Above the alignment are the locations of the mutations within the conserved blocks of the PI domain. Except for the mutations of G58A and S151A, the Shc mutations were isolated by screening a library of PI domain mutations (see ``Results and Discussion''). !, indicates new identified proteins; *, indicates probable orthologues from other species; +, this entry has been amended with fragments from other expressed sequence tags (Est); . . . , only a fragment of this protein is available in the data base.
Some of the mutations we identified mapped to relatively conserved residues while others did not. The mutations affecting phenylalanine at residue 198 were the most striking because they had the greatest effect on the binding of the Shc PI domain. This phenylalanine is conserved in all PI domains except those of the FE65 subfamily where it is replaced by a cysteine. The fact that mutagenesis of the conserved residues, Phe-198 and Ser-151, severely impairs phosphopeptide binding lends strong support to the validity of PI domain sequence alignment. The mutation of residues analogous to the Phe-198 or Ser-151 in other PI domains could lead to proteins with impaired PI domain function. The finding that one subfamily of PI domains, the FE65-like proteins, has cysteine instead of phenylalanine at the position equivalent to Phe-198 of Shc points to a possible diversification of PI domain binding specificity. Thus it is conceivable that the PI domain represents more of a general protein interaction domain, one subtype of which is involved in phosphotyrosine binding.
The PI domain, not the SH2 domain, is known to be crucial for the interaction of Shc with the nerve growth factor receptor, TrkA(11, 12) . However the relative roles of these domains in Shc interactions with EGF receptor are less clear because both the Shc SH2 and PI domains can bind the EGF receptor in vitro. We proceeded to reconstitute the PI domain and SH2 domain point mutations we had created into full-length Shc to analyze the role of these domains in the interaction of Shc with tyrosine-phosphorylated EGF receptor in living cells. We performed these studies by transiently transfecting four forms of Myc-tagged Shc into HeLa cells. These forms were wild type Shc, R397K Shc, F198V Shc, and a double mutant, F198V/R397K. The expressions of all these forms of Shc were equivalent as assessed by blotting cell lysates with anti-Myc antibody (Fig. 4, upper left panel). By immunoprecipitating with anti-Myc antibody we could analyze the associations of the wild type and mutant forms of Shc with endogenous EGF receptor present in HeLa cells. We found that while mutations in the SH2 domain had only minor effects on binding, mutations in the PI domain severely impaired binding (lower panel). Despite the ability of PI domain mutations to interfere with Shc binding, we saw no significant effect of these mutations on EGF-induced Shc tyrosine phosphorylation (upper right panel). This is not surprising as there have been several previous studies demonstrating that Shc does not need to bind to EGF receptor to become tyrosine-phosphorylated(23, 24, 25, 26) . It may be that a low affinity interaction between Shc and the EGF receptor is all that is required for Shc tyrosine phosphorylation or that a separate EGF-responsive kinase can also phosphorylate Shc. Regardless, these results confirmed that the F198V mutation abrogates PI domain function in living cells and points to the important role PI domains play in Shc interactions with growth factor receptors. The isolation of these PI domain mutation will be an important tool to understand the role of this domain in Shc signaling as well as the role of the PI domain in other proteins.
Figure 4: Mutagenesis of the PI domain blocks the interaction of Shc with EGF receptor in living cells. The mutations F198V and R397K either separately or together were reconstituted into full-length murine Shc containing a Myc tag epitope at its carboxyl terminus. Wild type and mutant Shc constructs were then transiently transfected into HeLa cells. Forty-eight hours after transfection the HeLa cells were stimulated with EGF (250 ng/ml) for 5 min. Cells were then lysed in 500 µl of a 1% Triton-based lysis buffer containing protease and phosphatase inhibitors. The majority of the lysate (400 µl) was subjected to immunoprecipitation with anti-Myc antibody. After washing with HNTG, the immunoprecipitates (IP) were run out on an SDS gel and transferred to nitrocellulose. The high molecular weight portion of the nitrocellulose was then blotted with anti-phosphotyrosine to detect EGF receptor while the lower molecular weights were probed with anti-Myc (lower panel). Lysate (20 µl) was also run directly on an SDS gel, transferred to nitrocellulose, and blotted with anti-Myc or anti-phosphotyrosine (Anti-PTyr, upper panels).
Note Added in Proof-While this manuscript was in press, the structure of the PI/PTB domain bound to a phosphopeptide was published (Zhou, M-M., Ravichandran, K. S., Olejniczak, E. T., Petros, A. M., Meadows, R. P., Sattler, M., Harlan, J. E., Wade, W. S., Burakoff, S. J., and Fesik, S. W.(1995) Nature378, 584-592). This structure [Medline] indicates that Phe-198 is a crucial residue making direct contact with the phosphopeptide at residues -3 and -5 to the phosphotyrosine.