Selection of Syk targets in breast cancer cells

To bootstrap the reconstruction of a comprehensive network of Syk downstream signaling in breast cancer cells, we analyzed tyrosine phospho-proteomic data acquired in two independent mass spectrometric studies using breast cancer cell lines with modified Syk catalytic activity or protein expression. On the one hand, we selected from our own study the proteins lost or gained in tyrosine-phosphorylated protein complexes of the Syk-positive MCF7 cells treated with a pharmacological Syk inhibitor (further referenced as the MCF7 dataset) [19]. On the other hand, we identified the proteins with modified tyrosine phosphorylation after exogenous Syk expression in the Syk-negative MDA-MB-231 cells (further referenced as the MDA231 dataset) [17]. Post-treatment procedures of the original phospho-proteomic data are detailed in the Materials and Methods section. From these two studies; we respectively selected 265 and 487 proteins as Syk targets (S1 and S2 Tables). Only 64 proteins were found in common, reflecting the complementarity of the two original phospho-proteomic studies. Indeed, the phospho-tyrosine enrichment prior to mass spectrometry as well as the experimental cell models used in those studies are different (see the Materials and methods section). We analyzed the two datasets separately to evaluate whether they point to distinct or similar cell signaling pathways.

Identification of overrepresented pathways

We searched for enriched pathways in the lists of Syk targets, using pathways from the KEGG database [37]. We selected pathways which contain at least one of the proteins from the target lists and used a Fisher exact test to assess their enrichment. As we are only interested in overrepresented pathways, we removed the underrepresented ones: i.e; the ones for which the ratio “number of proteins from the target list per total number of proteins” is lower than the same ratio in the background list.

Within the two rather poorly overlapping datasets, we found among the most enriched KEGG pathways those related to cell-cell and cell-substrate adhesions, actin cytoskeleton regulation and apoptosis (S3 and S4 Tables). This observation is consistent with the reported role of Syk on cell adhesion, motility, proliferation and death in breast cancer cells [19,38–43]. Furthermore, the similarity in pathway enrichment, despite the limited overlap between the two datasets, indicates their relationship. We merged the original datasets and present here the results obtained for the network reconstruction.

Network reconstruction

We assembled and explored a prior-knowledge interaction network to extract candidate mechanisms underlying the datasets. While such networks are often assembled using complete pathway or interaction databases, here we focused on previously identified enriched pathways. Using pathways rather than individual interactions will enable the extension of sub-networks with relevant interactions in their neighborhood for further analysis. By restricting our full network to a subset of pathways, some coverage may be lost but it allows to reduce the amount of irrelevant interactions and to better assess the relevance of the identified pathways. Hereafter we show that the enriched pathway can be used to identify candidate mechanisms. We also extended our search by using the Pathway Commons database [44]. KEGG provides a set of well-established pathways, while Pathway Commons allows a higher coverage by integrating pathways from multiple sources (notably Reactome, Panther, and PID). To select the most relevant pathways guaranteeing to cover most identified targets, we filtered the pathways based on their enrichment p-value and selected those presenting a p-value lower than 0.1 (in this step we aim to be as complete as possible, selecting 83 pathways from KEGG and 419 from Pathway Commons). Furthermore, we included the pathways containing Syk targets not covered by significantly over-represented pathways from the same database. This allowed to integrate 41 additional pathways from KEGG and 9 from Pathway Commons (S5 and S6 Tables). In this merged network, each protein and interaction keeps track of the list of pathways in which it is involved. We also used the GO annotation to identify the proteins involved in processes in which Syk is implicated (cell adhesion and motility, cell growth and death, immunity and inflammation, cell differentiation). The resulting oriented and partly signed network comprises 6438 proteins and 62322 interactions, from 552 pathways (124 from KEGG, 428 from Pathway Commons), covering 350 of the 687 identified targets (75 are only found in KEGG, 127 in Pathway Commons and 150 in both). Among these 350 targets, 245 are reachable from Syk (steps 1–2 in Fig 1). This network contains 979 interactions between two targets identified in the datasets. A closer scrutiny of these interactions further highlights connections between the two datasets: 146 and 260 interactions are associating targets specific to the MCF7 and MDA231 datasets respectively, 253 involve at least one target shared by the two datasets and 320 connect targets specific to different datasets.

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Fig 1. Workflow of the network reconstruction and signal propagation analysis.

The combination of simple steps unravels candidate mechanisms based on a list of proteins identified by (phospho-) proteomic experiments. (1) Identification of enriched pathways in the target list. (2) Building of a large network integrating interactions from the selected pathways. Proteins are associated with manually selected keywords based on their GO annotation. These annotations reflect functional categories associated to the enriched pathways (cell adhesion & motility, cell growth & death, cell differentiation and immunity & inflammation) and highlight phospho-tyrosine modifiers (tyrosine kinases and phosphatases), which are important to decipher this specific dataset. (3) Extraction from this large network of sub-networks allowing to propose candidate mechanisms via the action of Syk on its effectors, by a combination of weighted shortest paths and random walk methods. (4) Biological validation of candidate mechanisms. The individual steps are detailed in the Materials and Methods section.

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Sub-networks extraction by shortest paths analysis

The paths connecting Syk to the identified targets in the reconstructed network describe possible mechanisms for its signal propagation. As a massive amount of alternative paths exist, it is crucial to identify the appropriate candidates amongst the mass by extracting the sub-networks that exhibit selected connections between Syk and a specific target (step 3 in Fig 1; S1 Fig).

We focused on the signal propagation from Syk to its targets involved in cell adhesion and motility, and in particular on cortactin and ezrin, two proteins that are differentially phosphorylated in a Syk-dependent manner and that functionally link the plasma membrane to the actin cytoskeleton [45,46]. We first considered a parsimonious approach to find the paths implicating the fewest nodes, and searched for these shortest paths using the classical Dijkstra algorithm [47].

We observed that the shortest paths between Syk and cortactin contain two intermediates, with three alternative proteins directly upstream of cortactin (Fig 2A). Src is the only phospho-tyrosine modifier (tyrosine kinases and phosphatases) amongst them, suggesting that the paths involving Src are more credible to explain the change in cortactin phosphorylation.

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Fig 2. Proposed sub-networks for the effect of Syk on cortactin (A) and ezrin (B) identified by shortest paths analysis.

The grey nodes are only involved in the unweighted shortest paths, while the white ones are also involved in the weighted ones. The red borders denote phospho-tyrosine modifiers (tyrosine kinases and phosphatases). Note that some related proteins have been grouped in single nodes for clarity (denoted by curly brackets at the end of the name, and “PI3K class I”). Interactions annotated as “phosphorylation” (not particularly on tyrosine) appear in red, while “protein modifications” in general appear in blue. Line ends indicate the sign of the interaction: arrow for positive, T for negative, and circle for unknown. Finally, node shapes denote identified proteins: squares have identified differentially phosphorylated peptides (MDA231 dataset), circles correspond to differentially enriched proteins (MCF7 dataset), and diamonds are not part of the datasets.

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The shortest paths network linking Syk to ezrin included more proteins and contained also two intermediate nodes (Fig 2B). These paths were related with the classical regulation of ezrin by the membrane lipid PIP2 or its phosphorylation on serine/threonine residue(s) [48,49]. None of the nodes directly upstream of ezrin were phospho-tyrosine modifiers that could explain the effect of Syk on ezrin tyrosine phosphorylation. The sub-networks obtained for cortactin and ezrin illustrate the need for careful analysis of phospho-tyrosine modifiers to explain the phosphorylation-based modifications noticed in the MDA231 dataset.

Weighted shortest-path analysis

To take into account the importance of phospho-tyrosine modifiers, we extended the GO annotation of network nodes with the corresponding terms (S7 Table) and modulated the length of the path using distances attached to the interactions: a path involving more steps associated to small distances can be selected over a short path with longer steps. We assigned distances giving the priority to paths linking a phospho-tyrosine modifier upstream of proteins experimentally identified as differentially phosphorylated. We also favored the inclusion of other experimentally identified proteins by reducing the distances of their outgoing interactions.

The introduction of these distances led to more realistic suggestions for the cortactin sub-network, in which Src is the only protein directly upstream of cortactin (paths via white nodes in Fig 2A). As shown in the dedicated Results subsection, biological validation confirmed the role of Src in mediating Syk signal propagation to cortactin. However, it did not enable the identification of significantly better suggestions for ezrin, suggesting a “missing link” (paths via white nodes in Fig 2B). To resolve this inconsistency, we decided to evaluate the possibility of a direct interaction between Syk and ezrin. These results are described below and prompted us to propose that Syk directly phosphorylates ezrin.

Taking into account our biological validation, we added the new protein interaction from Syk to ezrin to the Syk network. We also extended the list of Syk direct substrates by integrating the results of a third dataset that identified the peptides phosphorylated on tyrosine by Syk after an in vitro kinase reaction [18] (S2 Table; for details, see Materials and methods). Finally, we added the direct interactions between Syk, E-cadherin and alpha-catenin, both members of the same cell-cell adhesion complex that we previously identified as direct Syk substrates [19] (step 4 in Fig 1).

Path ranking by random walk refinement and overflow

The sub-networks obtained with the weighted shortest-paths analysis still contain several equivalent paths which we would like to classify further by integrating a parameter based on the network topology. A random walk process provides a “reachability” score for each protein. By taking into account both a mix of network topology and the weighted interactions, this score highlights key proteins that are involved in multiple interesting and plausible candidate paths. To integrate this parameter into our analysis method, we used these scores to refine the distances associated to their outgoing edges, allowing the shortest-path approach to also include such key proteins. The weight refinement algorithm is fully described in the Methods section.

This methodology was applied to refine analysis of the Syk signal propagation to its targets involved in cell adhesion and motility. The size of this sub-network (e.g. number of nodes and edges) decreased after modulation of the length of the paths and even more after random walk refinement (Fig 3). This ranking property was appropriate to highlight the most likely paths regarding our biological and topological criteria. These observations were confirmed by the sub-networks linking Syk to its targets involved in Syk-related cell processes (S2–S4 Figs)

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Fig 3. Successive refinements of the shortest-paths sub-networks associated to cell adhesion and motility.

Evolution of the sub-network for the effect of Syk on proteins associated to cell adhesion and motility, starting with unweighted shortest paths, after the integration of weights (A), and by refining them using random walks (B). White nodes correspond to target proteins, grey nodes are intermediate proteins preserved by the refinement. The other colors denote nodes and edges that are affected by the refinement: blue elements are lost, while orange ones are introduced. The shape of nodes symbolizes the identification of the corresponding proteins in the original dataset, as in Fig 2. The ezrin and the cortactin sub-networks illustrated in Fig 2 are included in the adhesion and motility network.

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Nevertheless, we considered this method as too stringent and searched for near-shortest paths instead of strict shortest paths in order to generate a set of alternatives, selecting all paths for which the total distance is up to 20% higher than that of the shortest path. Using this setting for the analysis of the signal propagation from Syk to its targets involved in cell adhesion and motility, we retrieved a sub-network as large as the one obtained without random walk refinement. Moreover, the sets of interactions linking Syk to its targets involved in Syk-related cell processes were slightly distinct as compared to the sub-networks obtained after weighted shortest paths analysis, and after refinement with random walks, both allowing a 20% overflow (Fig 4 and S5–S7 Figs). This suggests that introducing the “reachability” parameter not only ranks the alternatives, but also selects novel elements that allow to generate hypotheses on Syk signal propagation.

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Fig 4. Extension of the shortest-paths sub-networks.

Evolution of the sub-network for the effect of Syk on proteins associated to cell adhesion and motility using weighted shortest paths, and after refinement with random walks, both allowing a 20% overflow. White nodes correspond to target proteins (which are all involved in cell adhesion or motility), grey nodes are intermediate proteins selected with the two approaches. The other colors denote nodes and edges that are specifically selected in one of the two methods: blue for weighted shortest paths, orange with random walk. The shape of nodes symbolizes the identification of the corresponding proteins in the original dataset, as in Fig 2. Although the new paths introduced by the overflow lie outside the cortactin and ezrin sub-networks, this methodological figure is useful for illustrating the flexibility of our approach.

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Taken together, the purpose of Figs 3 and 4 is to illustrate the flexibility of our method. These two figures tell us that (i) taking into account the molecular biology parameters by attaching distances to interactions for shortest-paths analysis and (ii) taking into account the network topology by the random walk refinement, leads not only to shortest paths to be biologically validated in the first instance (Fig 3, network size decrease), but also to novel alternative paths that were absent in the unweighted shortest paths analysis, and to rank more realistically the set of paths.

Syk controls cortactin tyrosine phosphorylation via the Src tyrosine kinase

Weighted shortest-path analysis from Syk to cortactin pointed to the Src tyrosine kinase as the phospho-tyrosine modifier that could account for the Syk impact on cortactin tyrosine phosphorylation (paths via white nodes in Fig 2A). This hierarchy was contradictory with previous studies describing the direct interaction of Syk and cortactin in breast cancer cells [18,42,50], and the impact of Src on Syk phosphorylation in colon cancer cells, opposite to our observations [51]. To test the ability of Src to drive the Syk signal propagation, we analyzed cortactin tyrosine phosphorylation, together with Syk and Src activity in cells treated with tyrosine kinase inhibitors. Cortactin phosphorylation and Src activity, evaluated by the phosphorylation of its tyrosine 418 residue, were decreased after cell pretreatment with Syk or Src pharmacological inhibitors (Fig 5A and 5B). Syk activity, evaluated by its auto-phosphorylation on the tyrosine 525/526 residues, was not affected by Src inhibitors, demonstrating the Syk-Src-cortactin hierarchy. In the MCF7 dataset, cortactin is poorly affected by Syk inhibition. As the quantitative measurement was obtained by calculating the median SILAC ratio of several peptides from cortactin, we decided to analyze the phosphorylation of its individual peptides. The quantity of the phosphotyrosine pTyr334 cortactin peptide was ~2 fold decreased by Syk inhibition (S8 Fig). Conversely, Tyr446 phosphorylation was not affected (S9 Fig). Those observations were consistent with the data from MDA231 dataset (Fig 5C). Taken together, our results indicate that the signal transmission from Syk to cortactin is mediated by the Src kinase.

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Fig 5. Syk controls cortactin tyrosine phosphorylation via the Src tyrosine kinase.

(A) Phosphorylation of indicated signaling proteins (left) in MCF7 cells that were treated with kinase inhibitors (Syk1, R406; Syk2, PRT062607; Src1, PP2; Src2, AZD0530) and either left unstimulated or stimulated with pervanadate (PV). CTTN, cortactin; IP, immunoprecipitation; WCL, whole cell lysate. Molecular weight standards (MW) are indicated (right). (B) Protein tyrosine phosphorylation of Syk, Src and cortactin quantified after pTyr stimulation and inhibition of Syk or Src catalytic activity. In the stimulated conditions, all the values obtained with the different inhibitors are statistically significant compared to the value obtained without inhibitor (P < 0.05; n = 3), except for the Syk phosphorylation with both Src inhibitors. (C) Cartoon illustrating the Syk-dependent cortactin tyrosine-phosphorylation. The structure of cortactin comprises an NTA region (NH₂-terminal acidic), 6.5 tandem repeats (37 amino acids each), a helical region (helical), a proline-rich (P-rich) region, and a C-terminal SH3 domain. The localization of the identified phosphorylated tyrosines and their dependency on Syk are indicated (+, dependent; 0, independent;?, undetermined).

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Syk phosphorylates ezrin on the Tyr424 residue

None of the nodes directly upstream of ezrin were phospho-tyrosine modifiers that could explain the Syk impact on ezrin tyrosine phosphorylation (Fig 2B). To explore this more profoundly, we evaluated the possibility of a direct interaction between Syk and ezrin. Both proteins are localized in phospho-tyrosine enriched plasma membrane extensions (ruffles) of MDA-MB-231 breast cancer cells in which actin is dynamically reorganized (Fig 6A). Colocalization of Syk and ezrin was evaluated quantitatively (Fig 6B). Purified recombinant Syk was able to induce direct ezrin phosphorylation on tyrosine residue(s) in in vitro kinase assays (Fig 6C). Moreover, in an immune-complex in vitro kinase assay using endogenous or exogenously expressed FLAG tagged or GFP fusion-proteins, ezrin was phosphorylated dependent on the Syk catalytic activity (S10A and S10B Fig). It is worth noting that tyrosine phosphorylation of Syk is also enhanced in the presence of ezrin (compare lane 3 with lane 1) in both autoradiography and Western blot analyses which may have a biological explanation. Ezrin contains a canonical ITAM motif that has been shown to interact with Syk [52] and even play a role in Syk recruitment and activation by binding to its tandem SH2 domains [53]. A positive feedback loop may thus exist as binding of Syk is activated by its SH2 domain binding to bi-phosphorylated ITAM motifs but should be explored more deeply. Detailed analysis of the ezrin post-translational modifications by isoelectric focusing revealed that its in vitro phosphorylation by Syk induced a unique phosphorylation of one third of the total ezrin protein (S10C and S10D Fig). Mass spectrometric analysis demonstrated that ezrin is phosphorylated by Syk on a peptide containing the phosphorylated Tyr424 residue (S11 Fig). The same ezrin phospho-peptide was the only one identified in the Syk-positive breast cancer cells in the MDA231 dataset. Taken together, these results prompted us to propose the new protein interaction between Syk and ezrin, leading to ezrin phosphorylation on the Tyr424 residue(Fig 6D).

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Fig 6. Syk phosphorylates ezrin on the Tyr424 residue.

(A) Syk and ezrin are both localized in pTyr-enriched plasma membrane ruffles of MDA-MB-231 cells (arrowheads). Scale bar 5 μm. (B) Quantitative analysis of Syk and ezrin colocalization with the merged picture of Syk and ezrin channels in which colocalized pixels are displayed in white (upper panel, scale bar 5 μm) and the scatter plot of pixel intensities in Syk and ezrin channels (lower panel). (C) Direct in vitro tyrosine phosphorylation of ezrin by Syk. The phosphorylation of purified Syk and ezrin (left) are analyzed by autoradiography or Western blot (pTyr). Molecular weight standards (MW) are indicated (right). *, non-specific band. (D) Cartoon illustrating the ezrin phosphorylation on Tyr424 residue by Syk. The structure of ezrin comprises a NH₂-terminal FERM domain followed by a helical domain and the C-terminal actin-binding domain (C-ERMAD).

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Reasonability of network reconstruction and shortest path analysis

Using datasets extracted from two published complementary phospho-proteomic studies that identified Syk targets in breast cancer cells, we reconstructed a Syk-controled molecular network by integrating the components of signaling pathways enriched for Syk targets (S1 File). Two different breast cancer cell models were used: Syk-positive MCF7 cells treated or not with a pharmacological Syk inhibitor versus exogenous Syk expression in the Syk-negative MDA-MB-231 cells. This was expected to bring some heterogeneity in the molecular paths linking Syk to its targets. Nevertheless, lists of Syk targets emerging from the different datasets showed similarities in pathway enrichment. Moreover, in the Syk network subpart containing the reachable targets, we found that one third of the interactions involving two targets connect targets identified in different datasets, which justified combining them into a unique set despite the partial overlapping. This proportion is conserved after shortest paths analysis, suggesting that a number of mechanisms by which Syk activates its targets are common to the cell models used. Although the biochemical methods to enrich protein extracts before mass spectrometry analysis were distinct (enrichment of tyrosine phosphorylation dependent-protein complexes versus tyrosine-phosphorylated peptides), they produced complementary information. On the one hand, phospho-proteomic studies at the protein level identified not only proteins that are differentially phosphorylated but also their partners present in the protein complexes. Several conserved protein domains are involved in phospho-tyrosine-dependent protein-protein interaction. On the other hand, phospho-proteomic studies at the peptide level identified the differentially phosphorylated tyrosine residues, allowing to increase the precision of our experimental validations. Knowing the phosphosites provides insight in the functional consequences of the phosphorylation and the integration of this functional information allows to construct more coherent networks.

The introduction of distances was a crucial step in our approach that allowed the selection of realistic paths. The extra random walk step enabled the refinement of these distances, so the selection of too many paths having the same length was avoided. In contrast to methods proposing a unique solution (or too many alternatives), our method allows to downscale to a few biologically significant alternative paths. The simplified network obtained by sub-network extraction allowed us to generate computational hypothesis about Syk signal propagation that were subsequently validated.

Validation of the cortactin signaling axis: Cortactin phosphorylation by Syk is dependent on Src

As a result of our biological validations, we proposed a new molecular explanation of the impact of Syk on cortactin, a protein involved in cell adhesion and motility by its ability to regulate the cortical actin cytoskeleton. Previous studies described cortactin as a direct Syk substrate [42,50]. However, in the phospho-proteomic data exploited in our study, the cortactin Tyr421 residue directly phosphorylated by Syk in vitro [18] does not match the Tyr residues phosphorylated in a Syk-dependent manner in cellulo [17]. In our model, we proposed a new Syk-Src-cortactin signaling axis (paths via white nodes in Fig 2A). We demonstrated that cortactin tyrosine phosphorylation induced by Syk is dependent on Src catalytic activity. Conversely, inhibition of Src did not affect the Syk catalytic activity, but both are required to induce cortactin phosphorylation in breast cancer cells (Fig 5A and 5B). This tyrosine kinase hierarchy does not match previous observations showing that Src inhibition induces a decreased tyrosine phosphorylation of Syk [51]. This discrepancy could be explained by the distinct cell models (breast cancer versus colorectal cancer cells) and by the fact that Leroy and colleagues [52] analyzed global Syk phosphorylation rather than specific phosphorylation on the Tyr525/526 residues, which are located in the activation loop of the Syk kinase domain and are more relevant to detect changes in Syk catalytic activity [54]. Multiple tyrosine phosphorylation sites have been described within cortactin (for review, [46]http://www.phosphosite.org/). We confirmed that the phosphorylation of cortactin Tyr446 residue is not directy affected by Syk (Fig 5C). Conversely, the phosphorylation of the Tyr334 residue is Syk-dependent, but can, according to our model, be phosphorylated also by Src [55]. There is currently no information about the functional consequences of this residue’s phosphorylation. Finally, the Syk-Src-cortactin signaling axis we proposed is consistent with the positive impact of Syk on E-cadherin dependent cell-cell adhesion [19,42]. Src-dependent phosphorylation of cortactin is necessary to link the E-cadherin adherens junction complex to the actin cytoskeleton, that subsequently supports cell-cell contact formation [56,57].

Validation of the ezrin signaling axis: Syk directly phosphorylates ezrin

Our initial computational hypotheses of molecular circuits linking Syk to ezrin did not explain its tyrosine phosphorylation, by the lack of a phospho-tyrosine modifier directly upstream of ezrin (Fig 2B). We demonstrated that Syk phosphorylates ezrin in a direct manner on its Tyr424 residue and that both proteins colocalize in the plasma membrane ruffles in breast cancer cells (Fig 6A and 6B). Previous studies described a Syk-dependent tyrosine phosphorylation of ezrin in B lymphocytes on its Tyr353 residue [58,59], a site that can be also phosphorylated by the epidermal growth factor receptor (EGFR) [60]. Phosphorylation of this residue leads to activation of the ezrin downstream signaling pathways as JNK or PI3K/Akt [59,61]. Two other ezrin tyrosine residues, Tyr146 and Tyr478, can be phosphorylated by Src (Tyr146, also being phosphorylated by EGFR), mediating cell scattering and stimulating motility [62,63]. We showed here that in breast cancer cells, Syk phosphorylates ezrin on the Tyr424 residue, rather than Tyr353 as it occurs in B lymphocytes, and could induce a signaling cascade different than the ones previously described for tyrosine phosphorylated ezrin. This novel molecular regulation of ezrin could help to explain the negative impact of Syk on epithelial cell motility.

Interest for cancer research and extent of application of the methods

By this study, we do provide to the cancer cell signaling community access to the Syk network and sub-networks of the paths from Syk to its targets involved in (i) cell adhesion and motility, (ii) cell growth and death, (iii) cell differentiation and (iv) immunity and inflammation (see Supporting Information). As Syk is involved in breast cancer suppression, it is not surprising that these cellular processes involved in cancer progression can be affected by Syk in breast cancer cells. Nonetheless, many of the Syk interactions described in pathway databases are extracted from molecular studies in cells of hematopoietic origin. More precisely, Syk signaling has been extensively studied in B lymphocytes where it is indispensable for immune cell differentiation. Which part of Syk signaling is shared between epithelial and hematopoietic cell types could be determined by Syk related phospho-proteomic experiments with a more comprehensive collection of cell models.

At this stage, our model suggests a number of plausible mechanisms linking Syk with cancer-related cellular processes. These can be used to generate more hypotheses, validation and provide valuable inputs for further developments. A crucial issue in Syk-related research is how to activate compensatory mechanisms maintaining tumor suppression signaling even when Syk is downregulated. The network we propose here is the first step towards addressing this question. To advance towards more refined mechanistic models the annotation of the interactions, for instance the sign, should be completed by integration of more data and by formal inference methods [64,65]. The careful consideration of possible feed-backs should also be considered in these developments. For instance, in tyrosine kinase signaling, many feed-back interactions involve phosphatase players whose role and significance are largely ignored even for very well studied pathways such as MAPK. New biological experiments are needed to unravel new players and interactions. Basic networks like the one resulting from our approach can be used for planning such experiments. As a simple example, if phosphatases are present upstream in the network one would want to test the effect of their inhibition on downstream proteins.

The bioinformatics method we used to reconstruct and prune the Syk signaling network can be used in other studies, whenever the focus is on finding candidate mechanisms explaining how signals propagate in large networks and how the network state-changes under perturbations. We consider that the combination of ad-hoc distances, random walk, and near-shortest paths provides good candidate mechanisms, by implementing the following requirements: (i) minimize the number of steps (shortest paths); (ii) fit with the data (ad-hoc distances); (iii) further favor intermediates which belong to multiple appropriate candidate paths (random walk); (iv) propose and rank multiple alternatives (near-shortest paths). This strategy can be generally applied to other studies of signaling networks using datasets based on distinct post-translational modifications, separately or combined. The open source code for the network reconstruction and extraction of relevant sub-networks will be made available for the computational biology community.

Online databases

Uniprot ID mapping from uniprot.org/downloads (2015/07)

HGNC dataset from genenames.org/cgi-bin/statistics (2015/07)

GO ontology from geneontology.org/page/download-ontology (go-basic.obo, 2015/10)

GO annotation from geneontology.org/page/download-annotations (goa_human.gaf, 2015/10)

KEGG: www.kegg.jp, release 75 (2015/07)

Pathway commons:pathwaycommons.org release 7 (2015/03)

Mapping protein identifiers

Proteins are identified by their Uniprot IDs, without the isoform postfix. We used Uniprot ID mapping files to associate KEGG and HGNC identifiers (transferred to the corresponding gene symbols) with these Uniprot IDs. When multiple Uniprot IDs are associated to the same KEGG or HGNC ID, they were grouped and a single ID is selected for the group, preferably a reviewed entry (allowing to map unreviewed Uniprot entries to the associated reviewed entry when possible).

Annotation of Syk network

The network is annotated based on the dataset, the pathways, and the GO annotation. Nodes and interactions keep track of the list of pathways in which they appear. Interactions types (phosphorylation, modification, regulation) and signs (+ or -) are transferred from the pathways when available. When the same interaction is described in several pathways, all types and a combination of the signs are conserved (an interaction described as positive in a pathway and negative in another is considered as unclear). We selected some groups of GO terms representing relevant processes and functions in this dataset, in particular cell adhesion and motility (GO:0048870, GO:0007155, GO:0034330, GO:0022610, GO:0060352, GO:0030030), cell growth and death (GO:0008283, GO:0007049, GO:0008219, GO:0019835, GO:0000920, GO:0007569, GO:0051301, GO:0060242), immunity and inflammation (GO:0002376, GO:0001906), and cell differentiation (GO:0030154, GO:0036166). We also annotated as phospho-tyrosine modifiers the components of the network with tyrosine kinases (GO:0004713) and tyrosine phosphatases (GO:0004725) GO terms and manually verified this list (S7 Table).

Many nodes in KEGG pathways represent groups of proteins, where the same protein can be part of several groups (with variable overlap). These groups are conserved in the merged network by introducing “group nodes” with bidirectional links to their members. Proteins can thus have interactions associated directly to them or through one or several groups. Such groups are “exploded” before the path search step described below.

Network visualization

Cytoscape 3.4 (http://www.cytoscape.org/) was used to generate figures and Cytoscape web was used to provide interactive access to the Syk network.

Near-shortest paths

We searched for “near-shortest paths” between Syk and a list of targets, using an approach similar to the classical Dijkstra algorithm for shortest paths. We started by identifying the length of the shortest path for every node as in Dijkstra’s method (starting from the source node, we iteratively picked the closest new neighbor of all reachable nodes: at each step we obtained the best result for a new node, ending with the node with the longest of the shortest paths). In the Dijkstra algorithm, the shortest paths were then obtained by starting from the target nodes and going backward to the source by selecting the incoming edge(s) which can satisfy this best distance: i.e. the best distance of the current node is equal to the sum of that of the source and the distance of the edge. Here we define an acceptable extra distance to include additional nodes and edges during this backtracking step. Note that the resulting sub-network can contain paths that are longer than acceptable, but all selected nodes and edges are involved in at least one acceptable path. For example if (A,B,C) is the shortest path from A to C, and (A,I,B,C) and (A,B,J,C) are also acceptable, then the path (A,I,B,J,C) exists in the resulting sub-network despite being too long. In the resulting sub-network, the selected nodes and edges are annotated with the “overflow” needed to include them: i.e. the extra distance of the best path using them compared to the actual shortest path. Members of the shortest paths have no overflow.

Edge distances for the shortest paths

To improve the identified paths, we selected edge weights based on the available annotations: “normal” edges have a distance of 5 (d = 5), we promoted edges coming out of identified proteins (d = 3), edges reaching an identified protein while coming out of a tyrosine kinase or phosphatase (d = 2) or combining these two conditions (d = 1). On the other end, we demoted edges reaching a target identified as differentially phosphorylated, but which did not come from a tyrosine kinase or phosphatase (d = 8), even if they come out of another identified protein (d = 6). Finally, edge distances are refined to integrate the results of the random walk estimation: they are multiplied by the inverse of the normalized score of their source node.

Random walk

We adapted the netwalk implementation in R from the GUILD software [66]: http://sbi.imim.es/web/index.php/research/software/guildsoftware

Edge weights are based on the distances originally defined for the shortest paths search (reversed as a higher distance corresponds to a lower weight).

More precisely, let d_ij be the distance from a node i to its direct target j, previously defined for the shortest path search. Given a node i the set of all its direct targets (successors in the directed network) is denoted Succ(i). The random walk is defined by transition probabilities p_ij defined as: Where p₀ is the return probability to the origin node Syk.

The probabilities p_ij together with p₀ added as last entry of each row are the entries of the stochastic matrix P (each row of this matrix sums to one). The equilibrium or limiting distribution of the random walk is a normalized row vector π satisfying the equation:

This distribution can be estimated by starting the random walk from any node and running it a sufficiently long time for equilibration. A finite, connected network with possibility of return to the Syk node from terminal nodes is ergodic guaranteeing the existence and uniqueness of the equilibrium distribution.

Nodes are scored by the values of the equilibrium probabilities π_i. In order to eliminate biases created by topology a second simulation is performed where all edges have the same weight. The resulting scores in this second simulation are the equilibrium probabilities . The two scores are then used to refine the distances as follows

Cell culture

MCF7, MDA-MB-231 and COS7 cell lines were obtained from the ATCC and maintained in Dulbecco’s modified Eagle’s medium (DMEM, Gibco) supplemented with 10% fetal calf serum (FCS, Eurobio). All cell cultures were carried out at 37°C using a 5% CO2 atmosphere. For cell stimulation studies, cell lines were stimulated with Sodium pervanadate (PV, premix of 1 mM H₂O₂ and 1 mM Na₃VO₄) and incubated for 15 min at 37°C. For the evaluation of the effect of the kinase inhibitors (all from Selleckchem), cells were incubated in medium for 2 hours with 2.5 mM R406, 5 mM PRT062607, 1 mM PP2, 0.5 mM AZD0530. Stock solutions for all those kinase inhibitors were prepared in dimethyl sulfoxide (Sigma, Hybri-Max grade), which is used as vehicle negative control

Western blot analyses

Cells were washed with ice-cold phosphate buffered saline solution and scrapped in 10 mM Tris-HCl (pH 7.4), 150 mM NaCl, 0.5 mM EDTA (Sigma), 1% Nonidet-P40 (Sigma), 0.5% sodium deoxycholate (Sigma), 1 mM Na₃VO₄ (Sigma), 50 mM NaF (Sigma) and a protease inhibitor cocktail (Sigma) at 4°C. After transfer to an Eppendorf tube and extensive vortexing, lysates were cleared by centrifugation at 10,000 rpm for 10 min at 4°C and supernatants diluted in 4x SDS-PAGE sample buffer. Immunoprecipitations were performed as described previously [44]. Protein samples were diluted in 4x SDS-PAGE Laemmli sample buffer, denatured by boiling for 5 min at 95°c in SDS-PAGE sample buffer, separated electrophoretically and transferred to polyvinylidene difluoride membranes. Membranes were blocked using 5% BSA in tris-buffered saline solution with Tween-20 detergent (TBS-T; 25 mM Tris-HCl pH 8.0, 150 mM NaCl, 0.1% Tween-20) for 1 h and then incubated at 4°C with the appropriate primary antibodies diluted in blocking buffer. Those included a mix of two monoclonal antibodies to phospho-tyrosine (1:1 mix vol/vol mix of the 4G10 and PY20 hybridoma supernatants), monoclonal antibodies to the FLAG epitope (clone M2, Sigma), cortactin (clone 4F11; Millipore), Syk (clone 4D10, Santa Cruz) and alpha-tubulin (clone DM1A, Sigma), rabbit polyclonal antibodies to pTyr⁴¹⁸ Src (Invitrogen), GFP (Chemokine), a home-made rabbit polyclonal antibody to the COOH-terminal domain of human ezrin [67], and a rabbit monoclonal antibody to pTyr525/526 Syk (Cell Signaling Technology). After three washes with TBS-T, the membrane was incubated with horseradish peroxidase-conjugated appropriate secondary antibody (1:5000, Jackson ImmunoResearch) for 1 h at room temperature. Immunoblots were revealed using a standard chemoluminescent method (ECL, Ozyme) and a Multi-application gel imaging system (PXi, Syngene). Membranes were optionally stripped with the Restore PLUS Western blot stripping buffer (Thermo Scientific) before a second immunoblotting. Immunoblot-derived signals were quantified using the ImageJ software (NIH) with three independent biological and technical replicates for each quantification. The signals were normalized on the lane corresponding to the total protein quantity loaded (immunoglobulin heavy chain in case of immunoprecipitation; Tubulin-α in case of whole cell lysate) and the unstimulated condition was arbitrarily set at 1.

In vitro phosphorylation assay

Assays with proteins extracted from cell lysates, immunoprecipitations and Western blot analyses were performed as described previously [43]. Otherwise, recombinant GST-Syk (BPS Bioscience, San Diego, CA) and GST-ezrin (previously described in [68]) were used. In vitro kinase assays were performed as described [43]. For the two-dimensional electrophoresis analysis, proteins were precipitated for 2 h in two volumes of acetone at −20°C, and resuspended in 8 M urea, CHAPS 4%, and thiourea 2 M. We used 18 cm IPG-strips (Amersham Biosciences) with linear pH range of 3–10 for the first dimension. Proteins were loaded on the IPG-strips and run in a Multiphor II apparatus (Amersham Biosciences). After focusing, a second migration was performed in 10% SDS-PAGE gel and proteins were stained with silver nitrate (Amersham Biosciences).

Microscopy

MDA-MB-231 cells were transiently transfected with pDsRed-Syk [43] using Fugene 6 (Roche Applied Bioscience). Immunostaining procedures have been described before [43]. The following primary antibodies were used: monoclonal antibody 4G10 hybridoma supernatant (diluted 1:50 in TBS) and a home-made rabbit polyclonal antibody to the C-terminal domain of human ezrin [67]. The secondary antibodies used were goat-anti-mouse-Cy5 and donkey-anti-rabbit-FITC (Jackson ImmunoResearch Laboratories). Confocal images of immunostained cells were obtained as described [69]. For quantitative analysis of colocalization, we used the ImageJ software plug-ins (https://imagej.nih.gov/ij/) with the “Colocalization Finder” module (https://imagej.nih.gov/ij/plugins/colocalization-finder.html) to generate the merged picture of Syk and ezrin channels in which colocalized pixels are displayed in white, and with the “Coloc 2” module (http://imagej.net/Coloc_2) to generate the scatter plot of pixel intensities in Syk and ezrin channels and to compute the Pearson correlation of pixel intensities over space.

Proteomic analyses

Statistical analysis

Statistical analyses were performed using the two-tailed Student’s t test for paired and unpaired data versus control values. Experimental values in this work are all given as mean and standard error of the mean (SEM). Results with a P value ≤ 0.05 were considered as statistically significant.