Introduction
Breast cancer is one of the most significant malignancies of women [
1,
2]. Despite successful treatment of the primary malignancy, tumors relapse and subsequent metastasis often occur at distant sites, including bone, lung, liver, and brain [
3‐
5]. The presence of breast cancer metastasis significantly influences patients' prognosis. The five-year survival rate from breast cancer drops from 96% to 75% with regional spread, and drops to 20% with distant spread [
6,
7]. Understanding the molecular mechanism that regulates breast cancer metastasis is critical to developing therapies to treat breast cancer and increase the survival rate; and defining markers that predict metastatic potential will be a key for defining therapeutic approaches.
Phosphatidylinositol 4,5-bisphosphate (PI4,5P
2) plays central roles in regulating cell migration, a key step of cancer metastasis, by modulating adhesion turnover and dynamic cytoskeleton rearrangements [
8]. By interacting with cofilin, PI4,5P
2 regulates the elongation of newly polymerized actin filaments via controlling cofilin cellular distribution and activation [
9,
10]. Including cofilin, PI4,5P
2 also regulates the reorganization of actin cytoskeleton by associating with other proteins such as α-actinin, WASP/N-WASP, gelsolin, profilin, and villin [
8,
11]. Furthermore, PI4,5P
2 regulates adhesion turnover by binding to and modulating talin, vinculin, ezrin/radixin/moesin, calpain, and other proteins involved in adhesion dynamics [
8,
11].
Type I gamma phosphatidylinositol phosphate kinase (PIPKIγ) is one of the major enzymes in cells that generate PI4,5P
2 by phosphorylation of phosphatidylinositol(4)phosphate [
12]. Via the spatial and temporal control of PI4,5P
2 synthesis
, PIPKIγ plays a key role in multiple biological processes [
8,
13‐
18]. Loss of PIPKIγ leads to defects of cardiovascular and neuronal development, which is consistent with changes in cadherin function and cell migration [
19]. PIPKIγ is also required for the integrity of the membrane cytoskeleton [
20]. The PIPKIγ is alternatively spliced in cells, resulting in at least two major variants, PIPKIγ635 and PIPKIγ661 (now named PIPKIγi1 and PIPKIγi2), which differ by a 26 amino acid C-terminal extension [
21,
22]. The short splicing variant PIPKIγi1 is reported to be a major contributor of the PI4,5P
2 pool that supports G protein-coupled receptor-mediated inositol 1,4,5-trisphosphate generation and plays a critical role in Ca
2+ flux [
23]. Unlike PIPKIγi1, PIPKIγi2 binds to talin via the 26 amino acid C-terminal extension in a process regulated by tyrosine phosphorylation, targeting PIPKIγi2 to adhesions [
17,
24]. The phosphorylation is mediated by both growth factor receptors and by the non-receptor tyrosine kinase, Src [
8,
17,
18]. By generating PI4,5P
2 and regulating talin assembly, PIPKIγi2 modulates nascent adhesion formation at the leading edge to facilitate cell migration. Specifically, the PIPKIγi2 regulates epidermal and other growth factor stimulated chemotaxis [
25], a process key to intravasation of cancer cells where cells migrate into the vasculature and lymphatic system, a first step in the metastasis of breast cancers [
9].
The loss of E-cadherin cell-cell contacts is a hallmark for the progression of cancers of epithelial origin [
26]. Remarkably, the PIPKIγ also regulates the ability of epithelial cells to assemble E-cadherin-based cell-cell contacts [
16]. This occurs by an association of PIPKIγi2 with E-cadherin and the recruitment of specific clathrin adaptors required for basolateral and endocytic trafficking by an association with the PIPKIγi2 C-terminus. A loss of PIPKIγ expression leads to a loss of E-cadherin targeting to the plasma membrane and a loss of E-cadherin-based cell-cell contacts [
16]. Thus, PIPKIγ regulates the plasma membrane targeting of E-cadherin-based cell-cell contacts and the polarization of epithelial cells. The positioning of the PIPKIγ as a regulator of both E-cadherin cell-cell contact assembly and growth factor stimulated cell migration positions the PIPKIγ as a key-signaling molecule in physiological functions that are fundamental to the metastasis of cancers of epithelial origin.
In spite of the increasing evidence indicating that PIPKIγ plays a crucial role in cell migration so that it is likely implicated in cancer metastasis, the pathological correlation between the lipid kinase and cancer progression remains uninvestigated. Here, we analyzed breast carcinomas via tissue microarray analyses for the levels of PIPKIγ and demonstrated a significant inverse correlation between strong positive PIPKIγ expression and overall survival. In addition, the requirement of PIPKIγ for the migration, invasion, and growth of breast cancer cells has been confirmed using in vitro models.
Materials and methods
Antibody
Polyclonal PIPKIγ anti-serum was generated from rabbit (Covance, Princeton, NJ, USA) using purified His-tagged PIPKIγ. Anti-serum was purified on an affinity column generated by coupling recombinant C-terminus of PIPKIγ to cyanogen bromide-activated Sepharose 4B (Sigma-Aldrich, Saint Louis, MO, USA) as described [
17,
25,
27]. The affinity-purified antibody recognizes both PIPKIγi1 and PIPKIγi2.
Constructs
The siRNA sequence targeting PIPKIγ is 5'-GGACCUGGACUUCAUGCAG-3'. The sequence of control scrambled siRNA is 5'-GUACCUGUACUUCAUGCAG-3'. Oligonucleotide sequences used for generation of short hairpin RNA (shRNA) specific for PIPKIγ were: GCCACCTTCTTTCGAAGAA (PIPKIγ shRNA) and GCCTTCTTCGCTAAACGAA (Control shRNA). Generation of replication-defective infectious viral particles and the transduction of the cells were carried out following the protocol provided by Addgene (Addgene Inc., Cambridge, MA, USA). In brief, synthesized oligonucleotides were annealed and cloned into HpaI and XhoI sites of pLL3.7 vector (Addgene Inc., Cambridge, MA, USA). Stabl3 competent cells (Invitrogen, Carlsbad, CA, USA) were used for transformation and DNA purification to minimize the mutagenesis. The integrity of lentiviral vector-containing cloned shRNA sequences were validated by DNA sequencing.
Cell cultures and transfection
MDA-MB-231 and MDA-MB-435S cells were cultured using DMEM supplemented with 10% FBS. SKBR3 cells were cultured in DMEM/F12 with 10% FBS. For siRNA transfection, cells were transfected with Oligofectamine (Invitrogen, Carlsbad, CA, USA) following the manufacturer's instructions.
A tissue microarray was constructed out of 438 archival invasive breast carcinoma samples at Vancouver General Hospital. These cases were collected between 1974 and 1995. Ethics board approval was obtained for all cases. Patients' demographics, pathological features of the tumors and expression of various biomarkers have been reported previously [
28]. In brief, median age of the patients at the moment of diagnosis was 61.5 years; median survival time was 11.9 years. Histological distribution included 379 infiltrating ductal carcinoma, 41 infiltrating lobular carcinoma and 8 special types.
Three tissue microarray blocks were assembled using a manual tissue microarrayer (Beecher Instruments, Inc., Silver Springs, MD, USA) from formalin fixed paraffin-embedded tissue as described previously [
29]. Tissue sections (4 μm thick) were cut from the donor blocks and stained with hematoxylin and eosin for tissue review. Representative areas of tumor were circled on the slides and corresponding donor blocks; duplicate 0.6 mm cores were taken from these blocks and inserted into three recipient blocks. Sections (4 μm thick) were cut from the recipient blocks and deparaffinized with CitriSolve and dehydrated through three alcohol changes. Antigen retrieval was performed using a steamer for 30 minutes in 0.1 M citrate buffer (pH 6.0). After that, sections were rinsed with PBS three times for five minutes each time. Hydrogen peroxide and serum free protein block (Dako, Carpenteria, CA, USA) were used to block endogenous peroxidases and prevent non-specific protein binding. Sections were then incubated with anti-PIPKIγ antibody (0.5 μg/ml) in a sealed immunochamber overnight at 4°C and Dako Envision anti-rabbit secondary antibody was applied at room temperature for 30 minutes. The NovaRed Substrate Kit (Vector Labs, Burlingame, CA, USA) was used to visualize the protein. Slides were then counterstained with hematoxylin and mounted.
Digital image database
The hematoxylin and eosin and immunohistochemistry images of all cores used in this study are publicly available at the companion site [
30]. The site was constructed using a GPEC database and a Java applet provided by Bacus Laboratories, Inc (Bacus Laboratories, Inc., Lombard, IL, USA). All the slides were scanned with a BLISS scanner (Bacus Laboratories, Inc., Lombard, IL, USA), and posted on the site. WebSlide Browser for Windows (Bacus Laboratories, Inc., Lombard, IL, USA) can be used for viewing preview images of the arrays and images of individual cores.
Cell migration assay
The assays were performed in modified Boyden chamber transwell (Neuroprobe, Gaithersburg, MD, USA) as described [
31,
32]. The membrane was pre-coated with type I collagen (10 μg/ml). Per well, 50,000 cells were applied. Chemotaxis assays were performed at 37°C in humidified air with 5% CO
2 for four hours. Cells migrated through to the underside of the membrane were counted in five high power fields, in a blinded fashion. The migration index for each experiment was calculated as the mean number of cells that migrated toward medium-containing 1% FBS divided by the mean number of cells that migrated toward medium-containing BSA only.
Invasion assay
Matrigel-coated Transwells (BD Bioscience, San Jose, CA, USA) were incubated with DMEM for four hours and 5 × 104 cells were plated in the upper chambers. The lower chambers contained 1% FBS conditioned DMEM. The inserts were incubated at 37°C in humidified air with 5% CO2 for 24 hours. The cells that had invaded the lower surface of the membrane were fixed with 4% polyformaldehyde and stained with 0.2% crystal violet. The number of cells that had invaded was quantified by counting random fields using a light microscope.
Cell proliferation assay
MDA-MB-231, MDA-MB-435S, or SKBR3 cells infected with lentivirus containing either control shRNA or PIPKIγ shRNA were seeded into 12-well culture plates at a density of 1000 cells/well. Then, manual cell counting was performed every two days for eight days.
Statistical analysis
We performed Kaplan-Meier survival analysis using log-rank test to determine differences in survival of the patients with different levels of PIPKIγ protein expression. Breslow test was also used to emphasize survival differences in the first 5 to 10 years of the follow up. The alpha level was determined as 5%. All the tests were two-sided. Spearman's correlation was utilized to estimate correlations between PIPKIγ protein content with that of other biomarkers and clinical prognostic factors.
Discussion
Here, we have shown that the expression of PIPKIγ is inversely correlated to the survival of breast cancer patients, indicating a potential prognostic value of PIPKIγ. Consistently, PIPKIγ is required for breast cancer cell migration, invasion, and proliferation. All these results support the fact that PIPKIγ plays an important role in breast cancer progression.
Overexpression of the EGFR has been shown to correlate with metastasis and poor prognosis of breast cancer [
39]. Our results show that EGFR expression is correlated to PIPKIγ expression in breast cancer cells, which hints that EGFR and PIPKIγ may cooperate to facilitate breast cancer metastasis. Upon EGF stimulation, EGF-induced phosphorylation of PIPKIγ causes a disassembly of the phospholipase C-γ1-PIPKIγ complex and this could enhance PI4,5P
2 accumulation and thus enhances talin assembly into adhesions and this in turn would facilitate the protrusion formation and stabilization of adhesions, which is required for cell migration [
25].
Our results demonstrate that PIPKIγ is not only required for breast cancer cell migration but also for breast cancer cell invasion. During invasion, cancer cells form actin-containing protrusions, called invadopodia, that extend into the extracellular matrix and participate in extracellular matrix degradation [
40]. ADP-ribosylation factor 6 (ARF6) is a regulator of invadopodia formation and cell invasion [
41] and ARF6 directly activates PIPKIγ [
42]. It is plausible that PIPKIγ plays a role in invadopodia formation by production of PI4,5P
2 that regulates actin filament dynamics via cofilin, α-actinin, and vinculin.
The PIPKIγ expression is correlated with E-cadherin in our tissue microarray results. It is consistent with the role of PIPKIγ in regulating E-cadherin trafficking. PIPKIγ binds directly to E-cadherin and recruits clathrin adaptor complexes AP1B to the E-cadherin-PIPKIγ complex and this controls the targeting of E-cadherin to the basolateral membrane [
14,
16]. The loss of PIPKIγ results in the loss of E-cadherin targeting to the plasma membrane and a loss of epithelial cell polarization. The PIPKIγ-interacting region in E-cadherin has some overlapping with β-catenin-binding domain [
16]. PIPKIγ may regulate E-cadherin-β-catenin interaction and then modulate β-catenin nuclear translocation. Transactivation of β-catenin correlated significantly with cyclin D1 expression, and that high β-catenin activity significantly correlated with poor prognosis of the patients and was a strong and independent prognostic factor in breast cancer [
43]. PIPKIγ may regulate breast cancer progression via E-cadherin-β-catenin signal pathway.
Breast cancers are heterogeneous in their ER and PR status and display different response to tamoxifen treatment [
44]. A study on the cellular phenotypes of breast cancer tumors in 19,541 white women with node-negative disease showed that ER+/PR+ is the most common phenotype of breast cancer constituting 66% of the tumors, followed by ER-/PR- (19%), ER+/PR- (12.5%), and ER-/PR+ (3.4%). Among these different tumors, ER-/PR- tumors are associated with the worst cancer-specific survival and are resistant to tamoxifen treatment [
45]. Our results show that higher expression of PIPKIγ correlates to lower expression of ER and/or PR and correlates to lower patient survival rates. It is consistent with the fact that ER-/PR- tumors are associated with poor breast cancer prognosis. Although it is not clear if PIPKIγ could directly modulate ER or PR expression and if PIPKIγ could regulate ER or PR signaling, our results provide evidence that PIPKIγ correlates with ovarian hormone receptors status. It is worthy to demonstrate the possible role of PIPKIγ in regulating ovarian hormone pathways in breast cancer progression.
Competing interests
The authors declare that they have no competing interests.
Authors' contributions
YS wrote the manuscript, performed the breast cancer migration and invasion assay. DT performed TMA and analyzed the statistical data and helped to draft the manuscript. KL provided the anti-PIPKIγ antibodies and helped to draft the manuscript. NT performed breast cancer proliferation assay. SL helped to perform TMA and analyze the statistical data. DH and RAA are the research group leaders, evaluated the data, edited and approved the final manuscript to be published. All authors read and approved the final manuscript.