The cells were lysed using 1% Triton lysis buffer supplemented with 1mM Na₃VO₄, 50 mM NaF, 1 mM PMSF and protease inhibitors cocktail. All the lysis buffer reagents were obtained from Sigma Aldrich (Merck KGaA). The extracted proteins were quantified by Pierce BCA protein assay from Invitrogen (23225; Thermo Fisher Scientific, Inc.). The proteins were then resolved in a 10% SDS-PAGE gel. Immunoblotting was performed by probing proteins transferred onto PVDF membranes with the following antibodies: Anti-Smad2 (ab40855; Abcam), anti-phosphorylated-Smad2 (ab184557; Abcam), anti-histone H3 (ab1791; Abcam), anti-extracellular signal-regulated kinase (ERK; cat. no. 9102; Cell Signaling Technology, Inc. (CST)], anti-phosphorylated-ERK (pERK; cat. no. 9101; CST), Anti-TGFβ receptor I antibody (ab31013; Abcam), anti-β actin (A5441; Sigma Aldrich; Merck KGaA) and anti-green fluorescent protein (GFP; sc-9996; Santa Cruz Biotechnology, Inc.). To enable detection of the primary antibody, a rabbit or a mouse secondary antibody coupled to HRP was used according to the primary antibody species (ab7628 and ab191866, respectively; Abcam). All the primary antibodies were incubated over night at 4°C, while the secondary antibodies were incubated for 1 h at RT. The membranes were developed employing ECL Western Blotting substrate kit from Promega, USA (W1015). The images were acquired by Bio-Rad ChemiDoc touch imaging system. Human TGFβ (T2815; Sigma-Aldrich; Merck KGaA) was used for cell treatment at 5 ng/ml at 37°C.

293 and G5 cells were a kind gift from Dr Prigent (University of Leicester, Leicester, UK). The G5 cell line was generated by Samrein Ahmed, 2013, (University of Leicester). The GF cell line was generated by Samrein Ahmed at the University of Sharjah (UAE). The method of how stable cell lines were generated is described by Ahmed et al (19). FM-55p (13012417) and MM138 (10092321) melanoma cell lines were supplied from Sigma Aldrich (Merck KGaA) from the ECACC collection. The two cell lines were maintained as indicated by ECACC instructions.

The 293, G5, and GF cell lines were cultured in Dulbecco's Modified Eagle's medium (D6429; Sigma Aldrich; Merck KGaA) supplemented with 10% FBS (F9665; Sigma Aldrich; Merck KGaA) and 1% penicillin/streptomycin. G5 and GF cells were cultured with 200 µg/ml neomycin or hygromycin, respectively for selection. The cells were incubated at 37°C and 5% CO₂. Before and during the experiments, the cells were maintained without selection pressure to eliminate any effect of the selection treatment.

Total RNA was extracted from cells using a total RNA Purification Kit 1700 (Norgen Biotek Corp.). mRNA was then converted into cDNA using a TruScript Reverse Transcriptase kit following the manufacturer's protocol (cat. no. 54440; Norgen Biotek Corp.). qPCR was performed using a SYBR Green PCR kit (204145; Qiagen GmbH) and the following primers:

Homo sapiens VEGF forward, 5′-CTACCTCCACCATGCCAAGT-3′, and reverse, 5′-GCAGTAGCTGCGCTGATAGA-3′; homo sapiens MMP-2 forward, 5′-TCTCCTGACATTGACCTTGGC-3′, and reverse, 5′-CAAGGTGCTGGCTGAGTAGATC-3′; Homo sapiens SNAIL forward, 5′-ACCACTATGCCGCGCTCTT-3′, and reverse, 5′-GGTCGTAGGGCTGCTGGAA-3′; homo sapiens SLUG forward, 5′-TGTTGCAGTGAGGGCAAGAA-3′, and reverse, 5′-GACCCTGGTTGCTTCAAGGA-3′; and homo GAPDH forward, 5′-AGGGCTGCTTTTAACTCTGGT-3′, and reverse, 5′-CCCCACTTGATTTTGGAGGGA-3′. The RT-qPCR parameters for each of the genes are demonstrated in Table I. Fluorescence signals were detected using a Qiagen Rotor Gene Q PCR fluorescence analyser (Qiagne GmbH). The obtained quantification cycle (Cq) values were analysed using the 2^−ΔΔCq method (20).

Briefly, 1.25×10⁵ cells were resuspended in DMEM containing 0.1% serum and then added to upper Boyden chambers. Conditioned medium was made by adding fresh DMEM with 10% FBS to TGFβ-treated or untreated GF, or G5 cell-derived medium at a ratio of 1:1. The lower chambers contained the conditioned medium, and the cells were allowed to migrate for 16 h at 37°C. After the incubation time, the Boyden chamber membranes were stained with 0.2% crystal violet in 10% ethanol for 30 min at room temperature, and absorbance readings were obtained at 570 nm using Thermo Scientific Varioskan Flash-Elisa microplate reader (Thermo Fisher Scientific, Inc.).

The steps conducted to separate the nuclear fraction from the cytoplasmic fraction are described by Ahmed and Prigent (21). Briefly, cells were pelleted at 4°C at 122 × g for 5 min and the pellets were treated with hypotonic buffer (10 mM HEPES pH 7.8, 25 mM β-glycerophosphate, 25 mM MgCl₂, 0.1 mM Na₃VO₄, 0.5 mM EDTA and 0.1% protease inhibitors). Next, 10% NP-40 was added and accompanied with vigorous vortexing for 15 sec at room temperature. This was followed by 30 sec centrifugation at 13,000 × g at 4°C. Nuclear protein extraction was performed by adding a high salt buffer (50 mM HEPES pH 7.8, 50 mM KCl, 300 mM NaCl, 0.1 mM EDTA, 1 mM DTT, 10% glycerol, 0.2 mM NaF, 0.2 mM Na₃VO₄, and 0.1% protease inhibitor cocktail). Nuclear fractions were then analyzed by western blotting.

Each experiment was performed at least twice. Western blotting band analysis was performed using ImageJ-Version 1.50b (National Institutes of Health) (22) and Excel version 365. In the present study, the error bars represent the standard error of the mean. One-tailed student tests were used to calculate statistical differences. For the analysis of SLUG expression, one-way ANOVA was used as well as Dunnett's multiple comparison test for differences between multiple groups, using GraphPad Prism 7.04 (GraphPad Software, Inc.). P<0.05 was considered to indicate a statistically significant difference.

To determine the effects of ShcD on downstream TGFβ signalling, stable cell lines expressing GFP-ShcD or GFP were generated (G5 and GF, respectively), and the expression of GFP-ShcD or GFP was confirmed by immunoblotting with an anti-GFP antibody (Fig. 1). Next-generation sequencing showed that the ShcD expression level was 296 times higher in G5 cells than in GF cells (data not shown).

The 293, GF, G5, and two melanoma cell lines (FM-55p and MM138) were analysed to determine their TGFβ receptor type I expression profile to ensure cell responsiveness to TGFβ treatment (Fig. 1).

To examine whether ShcD contributes to TGFβ signalling transduction, 293, GF and G5 cells were treated with or without TGFβ. pERK was shown to be notably upregulated in GFP-ShcD-expressing cells than in GFP-expressing cells. Similar to pERK, but to a lesser extent (23), the levels of pSmad2 were increased in GFP-ShcD-expressing cells (Fig. 2). TGFβ treatment caused elevation of pERK by 1.8 fold in GFP-ShcD-expressing cells, while it resulted in increased pERK by 1-fold in GFP-expressing cells. The TGFβ-mediated Smad2 phosphorylation was less evident in GFP-ShcD-expressing cells than that of ERK phosphorylation. It was accordingly hypothesized that TGFβ treatment causes an increase in pERK and, to a lesser extent, in Smad2 phosphorylation in GFP-ShcD-expressing cells.

The role of TGFβ in establishing and maintaining EMT was reported to be partially achieved by inducing the transcription of various genes, such as the stemness genes SLUG and SNAIL (17). Therefore, SNAIL and SLUG expression was assessed via RT-qPCR. Upon TGFβ treatment, GFP-ShcD-expressing cells exhibited significantly upregulated expression of the stemness genes with or without the addition of 10% serum (Fig. 3A and B).

After cancer cells detach from neighbouring cells, resistance from the extracellular cellular matrix hinders cell motility; the secretion of extracellular proteinases, such as MMPs (23), is thus crucial for overcoming this resistance. MMP2 was found to be secreted and upregulated by various types of cancer cells to facilitate invasion (24). Furthermore, MMP2 expression was shown to be significantly increased in GFP-ShcD-expressing cells compared with corresponding GF cells when incubated with TGFβ and 10% serum but not with TGFβ alone (Fig. 3C).

Cancer metastasis is facilitated by new blood vessel formation (25). A previous report revealed that TGFβ induces angiogenesis via VEGF upregulation (26). Our findings failed to demonstrate any significant increase in VEGF gene expression in TGFβ-treated G5 cells, with or without complete medium addition, but interestingly, VEGF expression was upregulated in serum-deprived GFP-ShcD-expressing cells than in corresponding GFP-expressing cells (Fig. 3D).

In summary, SNAIL and SLUG expression was upregulated in GFP-ShcD-expressing cells in response to TGFβ treatment, unlike VEGF expression, which demonstrated higher levels when the cells were deprived of serum. MMP2 upregulation in GFP-ShcD-expressing cells was induced by the combination of 10% serum and TGFβ, but not by TGFβ alone (Table II).

A parallel set of cells was obtained for western blotting to assess ERK phosphorylation. pERK levels were notably upregulated in GFP-ShcD-expressing cells than in control cells upon TGFβ treatment regardless to complete addition (Fig. 3E).

GFP-ShcD-expressing cells were found to have higher expression levels of SNAIL, SLUG and MMP2 than control cells; thus, we investigated the nuclear levels of pERK upon TGFβ treatment. GF and G5 cells were either starved or treated with TGFβ with or without 10% serum. The nuclear fraction of GFP-ShcD-expressing cells exhibited higher nuclear pERK levels than that of GFP-expressing cells in starvation, TGFβ, or TGFβ treatment with complete medium conditions (P>0.05; 0.2, 0.18 and 0.09, respectively; Fig. 4A and B).

To determine the migration ability of ShcD-overexpressing cells, Transwell assays were employed. The cells were allowed to migrate against a gradient created by adding conditioned medium derived from TGFβ-treated or untreated cells expressing GFP-ShcD or GFP. GFP-ShcD-expressing cells exhibited increased migration than their control counterparts, while a slight increase in cell migration towards conditioned medium derived from TGFβ-treated G5 cells was observed (Fig. 5). Despite GFP-ShcD-expressing cells showed higher migratory abilities, the data was not statistically significant.