Lentivirus transduction

Stable SALL4 knockdown cells were established by lentiviral shRNA infection. The lentiviral particles carrying shRNA against SALL4 (shSALL4, sh#1 and sh#2) or negative control (shNC) were generated and provided by Obio Technology (Shanghai, China). The cells (ACHN, 786-O) were transduced with lentivirus following the manufacturer’s instructions. To establish stable cell lines, the infected cells were treated with puromycin (2μg/mL) for 7days. The shRNA sequences for SALL4: GCCTTGAAACAAGCCAAGCTA (sh#1) and GAGGATGAAGCCACAGTAA (sh#2); the shRNA sequence for negative control: TTCTCCGAACGTGTCACGT (shNC).

Cell counting Kit-8 (CCK-8) assay

Cells (1×10³ cells/well) were seeded in 96-well plates and maintained for indicated time. Cell growth was monitored by incubation with CCK-8 solution (Sangon Biotech) following the manufacturer’s protocols. Then a microplate reader (Bio-Rad) was used to detect absorbance at 450nm. Three repetitions were conducted in triplicate.

Clonogenic assay

Stable transfected cells (200 cells/well) were seeded into six-well plates and grown for 10days. After fixed by 4% paraformaldehyde, the colonies were incubation with 0.1% crystal violet for 20min. Then images were acquired and the number of colonies was counted.

Flow cytometry analysis

For cell cycle analysis, cells were harvested and fixed with 70% ethanol, followed by sequential treatment with RNase A (100μg/mL) and propidium iodide (PI) staining buffer. To analyze cell apoptosis, HUVECs treated as indicated were harvested and labeled with Annexin V-FITC and PI. Cell cycle distribution and apoptosis index were assessed by flow cytometry.

Senescence-associatedβ-galactosidase (SA-β-gal) staining

A SA-β-gal staining kit (Beyotime) was used to evaluate cellular senescence via detection of β-galactosidase activity following the manufacturer’s protocols. Cells were plated in six-well plates and cultivated for 48h. Then cells were washed with PBS and treated with fixative buffer for 15min. After washed with PBS for three times, cells were incubated with premixed staining solution in a CO₂-free atmosphere overnight. The images were acquired and SA-β-gal positive cells were counted under a microscope.

Wound healing assay

Cells seeded on six-well plates were cultivated to nearly full confluence. A yellow pipette tip was used to scratch a wound on the monolayer cells. Then photographs of scratched cells were taken under a microscope to monitor wound closure at indicated time.

Transwell assay

Transwell assays were conducted to evaluate the capacities of migration and invasion. Cells were resuspended in medium without FBS and counted. The 8-μm-pore chambers (Corning) were coated with (for invasion assay) or without (for migration assay) Matrigel (BD Biosciences) and inserted into 24-well plates. Resuspended cells were placed into upper chamber for transwell migration (2×10⁴ cells/well) and invasion (1×10⁵ cells/well) assay. Chambers were then incubated with medium containing 10% FBS in 24-well plates for 24h. Penetrated cells were stained with crystal violet and images were acquired for cell count under a microscope.

Conditioned medium (CM) collection

Stable transfected cells (ACHN-shNC, ACHN-sh#1) were re-suspended with DMEM/F-12 containing 10% FBS and plated in 60mm dishes (5×10⁵ cells/dish). After incubation for 12h, cells were washed and normal growth medium was replaced with serum-free medium (SFM) (5ml/dish). After incubation for 24h, cell culture supernatants from ACHN-shNC and ACHN-sh#1 cells were harvested. Cell debris in the supernatants was removed with a centrifuge.

Enzyme-linked immunosorbent assay (ELISA)

The levels of VEGFA in conditioned medium from ACHN-shNC and ACHN-sh#1 cells were detected by using an ELISA kit (Sino Biological) according to the manufacturer’s protocols. Then a microplate reader (Bio-Rad) was used to measure absorbance at 450nm.

HUVECs recruitment assay

The Boyden chamber (Millipore) assay was performed to determine the effect of ccRCC cells on HUVECs recruitment. Briefly, HUVECs were resuspended with SFM and placed into upper chamber (2×10⁴ cells/well). Chambers were then incubated with indicated CMs (SFM, shNC-CM, sh#1-CM) or co-cultured with ccRCC cells (ACHN-shNC, ACHN-sh#1) in lower chamber for 24h. Penetrated cells were stained with crystal violet and images were acquired for cell count under a microscope.

Tube formation assay

Matrigel (BD Biosciences) (50μl/well) was used to coat the wells of 96-well plates. After solidification for 1h at 37°C, HUVECs (4×10⁴ cells/well) were re-suspended with indicated CMs (SFM, shNC-CM, sh#1-CM) and plated onto the matrigel. After 6-h incubation at 37°C for tube formation, tubules were observed and pictures were acquired by microscopy. ImageJ software was used to analyze the formed tubes.

Western blotting

Immunoblotting assay was carried out as we previously described [16]. Cells were lysed using RIPA buffer containing protease and phosphatase inhibitors. The protein sample was resolved by SDS-PAGE, followed by transference of proteins onto PVDF membranes. The membrane was then treated with 5% bovine serum albumin, followed by overnight incubation with specific antibodies against Akt (1:1000, Cell Signaling Technology, CST), p-Akt (1:1000, CST), GSK-3β (1:1000, CST), p-GSK-3β (1:1000, CST), VEGFA (1:500, Sangon Biotech), SALL4 (1:1000, CST) and GAPDH (1:2000, Sangon Biotech). The corresponding HRP-conjugated secondary antibody and ECL substrate were used to visualize the protein bands.

Immunofluorescence staining

Cells were plated and grown on coverslips overnight. After fixed in 4% paraformaldehyde, cells were treated with 0.5% triton X-100 for cell permeabilization. The coverslips were then immersed in blocking solution (Beyotime) for 1h, followed by incubation with anti-p-GSK-3β (1:300, CST) and anti-p-Akt (1:200, CST) overnight. The Alexa Fluor 594-conjugated secondary antibody (1:200, Zsbio) was used for fluorescence labeling. Coverslips were incubated with DAPI for nuclei staining. Cells were observed and pictures were acquired by fluorescence microscope.

In vivo tumorigenicity assay

Immunodeficient BALB/c mice (six-week-old) were provided by Experimental Animal Center of Fourth Military Medical University (FMMU) and kept under SPF conditions. The procedures involving animals received approval of the Animal Research Ethics Committee of FMMU and the research was conducted in accordance with institutional guidelines. For tumor growth assay, 786-O sublines (1×10⁷ cells) were implanted subcutaneously into the flanks of mice (six per group). A vernier caliper was used to measure tumor size every 5days. The formula (volume=length × width²/2) was used to calculate tumor volume. Mice were sacrificed 5 weeks after inoculation. Tumor nodules were collected for further examination.

Human tissue samples

Patient specimens (tumor and matched normal tissues) were acquired from ccRCC patients (n=10) undergoing nephrectomy at Tangdu Hospital of FMMU. The patients received clinical and pathological diagnosis. Written informed consent was provided by the patients. This research gained the approval of Medical Ethics Committee of Tangdu Hospital.

Immunohistochemistry (IHC) staining

Immunohistochemistry staining was carried out as we previously described [16]. Morphology analysis of formalin-fixed and paraffin-embedded (FFPE) sections were performed with hematoxylin and eosin staining. For IHC staining, heat-based antigen unmasking was conducted using microwave in citrate buffer after dewax and rehydration of sections. Tissue sections were exposed to 3% H₂O₂ to block endogenous peroxidase, followed by treatment with blocking solution for nonspecific binding. Subsequently the sections were stained with specific antibodies against SALL4 (1:100, Abcam) overnight. After incubation with corresponding secondary antibodies, a DAB substrate kit was used to visualize positive antigen binding. Haematoxylin counterstaining was performed and pictures were captured by microscopy.

Bioinformatics analysis

To identify the expression pattern and clinical characteristics of SALL4, public datasets (TCGA Renal 2 and TCGA-KIRC cohorts) were analyzed in Oncomine (http://www.oncomine.org/) and UALCAN [17] (http://ualcan.path.uab.edu/) databases. The correlation between SALL4 expression and survival in ccRCC patients was assessed by GEPIA (http://gepia.cancer-pku.cn/) and Kaplan-Meier Plotter (http://kmplot.com/analysis/) databases. Genome-wide association analysis of SALL4 was performed with Cancer Regulome Tools (http://explorer.cancerregulome.org/). Gene correlation analysis, mutation analysis and methylation analysis were carried out using LinkedOmics [18] (http://www.linkedomics.org/) and TCGAportal (http://tumorsurvival.org/) databases.

SALL4 promotes ccRCC cells growth in vitro and in vivo

To further validate its oncogenic activities in ccRCC, we set out to check the putative function of SALL4 on ccRCC cell growth. Lentiviral shRNA-mediated knockdown of SALL4 was conducted and downregulated SALL4 protein levels in ccRCC cells (ACHN, 786-O) were detected (Fig. 2a). The cells were then subjected to CCK-8 and colony formation assays to determine the influence of SALL4 downregulation on ccRCC cell proliferation. We found that knockdown of SALL4 in ACHN and 786-O cells resulted in slower growth rate compared with control cells (Fig. ​(Fig.2b).2b). Similarly, the number of colonies formed by cells with downregulated SALL4 was significantly reduced (Fig. ​(Fig.2c).2c). To test whether SALL4 also drives cell cycle progression, flow cytometry analysis was performed. The results showed that remarkable changes of cell cycle distribution were induced by SALL4 silencing in ccRCC cells. As indicated by increased G1-phase cells and decreased S/G2-phase cells, downregulation of SALL4 in ccRCC cells arrested cell cycle by restraining G1-S transition (Fig. ​(Fig.2d).2d). Resistance to senescence or apoptosis has been identified as a hallmark of cancer cells and plays a crucial role in cell survival and tumorigenesis [19]. In particular, it has been demonstrated that some cells are more prone to senescence rather than apoptosis even following intensive exogenous stress [20]. SA-β-gal is the most frequently used marker for senescence and senescent cell exhibits high SA-β-gal activity. To further elucidate the functional role of SALL4 in cell senescence, ccRCC cells with stable SALL4-targeted or control shRNA were assayed using SA-β-gal staining kit. We observed that depletion of SALL4 in ACHN and 786-O cells upregulated SA-β-gal synthesis (Fig. ​(Fig.2e)2e) indicating that SALL4 depletion triggered cells senescence. By analyzing a public dataset of 533 ccRCC patients from TCGA, we found that SALL4 mRNA level was significantly correlated with the transcripts of genes related to proliferation, senescence and cell cycle, including CCNE1 (r=0.4145, P<0.0001), CDK3 (r=0.3811, P<0.0001), E2F1 (r=0.3302, P<0.0001) and RB1 (r=−0.3032, P<0.0001) (Fig. ​(Fig.2f-i2f-i and Additional file 3: Figure S3, Additional file 4: Table S1). Next, to investigate the oncogenic activity of SALL4 in ccRCC tumorigenesis in vivo, tumor formation was evaluated by subcutaneous inoculation of 786-O sublines in nude mice. we found that downregulation of SALL4 in ccRCC cells resulted in a dramatic decrease in tumorigenic potential, as evidenced by decreased tumor size, repressed tumor growth and reduced tumor weight (Fig. ​(Fig.2j-l).2j-l). Together, these findings validate that SALL4 drives ccRCC cell growth by promoting cell cycle progression and restraining cell senescence.

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Fig. 2

SALL4 promotes ccRCC cells growth in vitro and in vivo. a Western blot analyses of SALL4 expression in ccRCC cells stably expressing indicated shRNA (shNC, negative control shRNA; sh#1 and sh#2, shRNAs targeting SALL4). b The CCK-8 assays were performed in ACHN and 786-O cells treated with indicated shRNA. c Colony formation assays in ACHN and 786-O cells with indicated shRNA treatment. d Cell cycle distribution was examined by flow cytometry in ACHN and 786-O cells treated as indicated. e Cellular senescence was detected by SA-β-gal staining in ACHN and 786-O cells treated with shNC and shSALL4 (scale bar, 50μm). f-i Scatter plot analyses were performed to determine the correlation between SALL4 and CCNE1 (f), CDK3 (g), E2F1 (h) and RB1 (i) mRNA expression levels in 533 ccRCC patients from TCGA database. Data were analyzed via LinkedOmics bioinformatics. j The image of dissected tumors from nude mice. k, l The growth curve (k) and their weights (l) of subcutaneous tumors formed by 786-O cells with indicated treatment. * P<0.05, ** P<0.001 and *** P<0.001

SALL4 promotes ccRCC cells migration and invasion in vitro

Next, to explore whether SALL4 also function as a prometastatic factor in ccRCC, we performed a series of loss-of-function studies in ACHN and 786-O cells stably transfected with SALL4-targeted or control shRNA. The wound healing assays demonstrated that SALL4 downregulation markedly suppressed cell migration to delay healing of the scratched cell monolayer in ccRCC cells (Fig. 3a, c). Similar results were observed in transwell migration assays. We found that SALL4 silencing in ccRCC cells significantly impaired the migratory ability as measured by cells attached to the lower membrane surfaces. Consistently, in matrigel invasion assays of ACHN and 786-O cells, less cells were observed to penetrate through the matrigel barrier upon SALL4 knockdown, indicating a decrease in invasion potential (Fig. ​(Fig.3b,3b, d). These results were consistent with our finding that SALL4 was upregulated in metastatic ccRCC tumors (Fig. ​(Fig.1f).1f). The epithelial-mesenchymal transition has been reported to be involved in SALL4-mediated tumor metastasis [21]. In agreement with previous findings, we found that compared with the control cells, SALL4-deficient ACHN cells seemed to exhibit a tighter organization of cells in colonies (Additional file 5: Figure S4a). In addition, we analyzed the RNA-seq data of 533 ccRCC patients from TCGA and found that SALL4 mRNA level was significantly correlated with the transcripts of matrix metalloproteinases (MMPs) and tissue inhibitors of metalloproteinases (TIMPs) related to tissue remodeling and tumor invasiveness [22, 23], including MMP9 (r=0.1227, P=0.0005), MMP25 (r=0.2601, P<0.0001), TIMP3 (r=−0.2221, P<0.0001) and TIMP4 (r=−0.2761, P<0.0001) (Fig. ​(Fig.3e-h3e-h and Additional file 6: Figure S5, Additional file 7: Table S2). Collectively, these results support that SALL4 functions as a prometastasis oncogene in ccRCC progression.

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Fig. 3

SALL4 promotes ccRCC cells migration and invasion in vitro. a, c Cell migration ability was evaluated by wound healing assays in ACHN (a) and 786-O (c) cells with indicated shRNA treatment (scale bar, 200μm). b, d Transwell migration and matrigel invasion assays were conducted to determine the cell migration and invasion capabilities in ACHN (b) and 786-O (d) cells treated as indicated (scale bar, 100μm). e-h Scatter plot analyses were performed to determine the correlation between SALL4 and MMP9 (e), MMP25 (f), TIMP3 (g) and TIMP4 (h) mRNA expression levels in 533 ccRCC patients from TCGA database. Data were analyzed via LinkedOmics bioinformatics. ** P<0.001 and *** P<0.001

SALL4 expression is associated with endothelium development and vasculogenesis

To further characterize SALL4’s biologic functions and discern its oncogenic mechanisms, we first characterized the differential association signature between SALL4 mRNA level and individual gene expression by analyzing the RNA-seq data of 533 ccRCC patients from TCGA. As shown in Additional file 8: Figure S6a, we identified 6315 (dark red dots) and 2862 (dark green dots) genes that were positively and negatively correlated with SALL4 (FDR<0.01), indicating that SALL4 may exert a widespread influence on the transcription profiles. We then performed cluster analysis of the correlation profiles and constructed a heatmap to visualize the top 50 most significant genes that were positively and negatively correlated with SALL4 transcripts (Additional file 8: Figure S6b, c). Statistical scatter plots for top-ranked genes were created and revealed a strong positive correlation between SALL4 mRNA level and NOD-like receptor family CARD domain containing 5 (NLRC5) gene expression (positive rank #2, r=0.62, P=6.66e-57) (Additional file 8: Figure S6d). NLRC5 was previously reported to be upregulated in ccRCC and positively associated with tumor progression [24]. Recent evidence indicates that NLRC5 is implicated in vascular remodeling and required for vascular intimal hyperplasia [25]. we next conducted gene ontology term enrichment and KEGG pathway analyses of SALL4-associated genes and found that SALL4 expression significantly correlated with genes controlling vasculogenesis, endothelium development and cellular response to vascular endothelial growth factor stimulus (Fig. 4a), confirming the potential role of SALL4 in modulating vascular remodeling. Vasculogenesis refers to the formation of new blood vessels. Endothelium development is a complex process in which endothelial cells are oriented towards their specific fate and specialized endothelial cells form the endothelium of an organ such as vasculature, lymph vessel and heart. Furthermore, gene set enrichment analysis (GSEA) were performed in human ccRCC samples and revealed a large number of significantly enriched gene sets, including vasculogenesis (Fig. ​(Fig.4b)4b) and endothelium development (Fig. ​(Fig.4c).4c). Genome-wide association of SALL4 mRNA expression with multifarious molecular signatures, including gene expression, protein level (reverse phase protein arrays, RPPA), microRNA expression, DNA methylation, copy number variation and somatic mutation, was analyzed and visualized using a circos plot (Additional file 8: Figure S6e) and a network (Additional file 8: Figure S6f). In agreement with our observations in Additional file 8: Figure S6a-d, we found that the transcription levels of NLRC5 and SALL4 mRNA expression were strongly associated in ccRCC patients (Additional file 8: Figure S6f). In summary, these data suggest that SALL4 may be involved in vasculogenesis and vascular remodeling.

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Fig. 4

SALL4 induces ccRCC angiogenesis in vitro. a Enriched gene ontology (GO) term and KEGG pathway analysis of genes significantly correlated with SALL4 in ccRCC. b, c Gene set enrichment analysis (GSEA) profiles for the genes significantly correlated with SALL4 in ccRCC. Data (a-c) from TCGA database were analyzed via LinkedOmics bioinformatics. d HUVECs were treated with serum-free medium (SFM) or conditioned medium (CMs) from ACHN-shNC/shSALL4 cells. After treatment for 72h, CCK-8 assays were performed to evaluate cell proliferation. e Flow cytometry analyses of cell cycle distribution in HUVECs treated with SFM or CMs from ACHN-shNC/shSALL4 cells. f Wound-healing assay was performed to determine the migration of HUVECs with CMs treatment (scale bar, 200μm). g Representative images and quantification analyses of the recruitment of HUVECs co-cultured with indicated CMs (upper) or ACHN-shNC/shSALL4 cells (lower) in lower chambers (scale bar, 100μm). h, i Representative images (h) and quantification analyses (i) of tube formation in HUVECs treated with SFM or indicated CMs (scale bar, 100μm). j The expression level of VEGFA in CMs from ACHN-shNC/shSALL4 cells was detected by ELISA assay. * P<0.05, ** P<0.001 and *** P<0.001

SALL4 induces ccRCC angiogenesis in vitro

Given the potential role of SALL4 in vasculogenesis and vascular remodeling, we sought to investigate whether SALL4 modulates angiogenesis in ccRCC. In response to treatment with CM collected from ACHN sublines, we observed that HUVECs cultured in CM from ACHN-sh#1 cells showed significant reduction in viable cell number as measured by CCK-8 assay (Fig. ​(Fig.4d).4d). Flow cytometry analysis of HUVECs treated with CM from ACHN-sh#1 cells revealed an arrested cell cycle compared with that of cells treated with CM from ACHN-shNC cells (Fig. ​(Fig.4e),4e), but no significant alteration in cell apoptosis was observed (Additional file 5: Figure S4b, c). Scratch assay was performed on HUVECs treated with CMs. We found that migration of HUVECs was markedly alleviated after treatment with CM from ACHN-sh#1 cells (Fig. ​(Fig.4f).4f). In HUVECs recruitment assay, we observed that the chemotactic response of HUVECs migrating toward CM from ACHN-sh#1 cells was drastically suppressed in comparison with that of cells stimulated with CM from ACHN-shNC cells (Fig. ​(Fig.4g).4g). To explore the direct effect of SALL4 deficiency on the function of endothelial cells, we established a coculture system of HUVECs with ACHN sublines. Consistent with the above findings, we noticed that much fewer HUVECs were recruited toward ACHN cells lacking SALL4 (Fig. ​(Fig.4g).4g). To substantiate the relevance of SALL4 to angiogenesis in ccRCC, HUVECs were treated with CMs from ACHN sublines and assayed for tube formation. We observed that as expected, HUVECs exhibited diminished tube formation activity following stimulation with CM from SALL4-deficient ACHN cells (Fig. ​(Fig.4h,4h, i). Furthermore, we analyzed the levels of VEGFA in CMs from ACHN sublines and found that the concentration of VEGFA in CM from ACHN-sh#1 cells decreased (Fig. ​(Fig.4j).4j). Taken together, these in vitro observations validate the potent role of SALL4 in ccRCC angiogenesis.

SALL4 downregulation attenuates the activation of Akt/GSK-3β signaling and VEGFA expression in ccRCC

SALL4 was previously implicated in chromatin remodeling via modulation recruitment of nucleosome remodeling deacetylase (NuRD) complex [26]. The tumor suppressor PTEN has been reported to be a target gene repressed by SALL4 and counteract the PI3K pathway [13]. To validate the involvement of PI3K/Akt signaling in SALL4-mediated oncogenic activities in ccRCC, we evaluated the effects of SALL4 downregulation on PI3K pathway markers. Immunoblotting analysis of lysates from ccRCC cells revealed that SALL4 knockdown decreased the levels of phosphoprotein markers of PI3K pathway activation (p-Akt, p-GSK3β) without altering the total protein levels in ACHN and 786-O cells (Fig. 5a, b). Consistently, immunofluorescent staining (Fig. ​(Fig.5c)5c) further confirmed the observations in western blot assay. The extensive crosstalk and a positive feedback loop have been reported to exist between the PI3K/Akt and VHL/HIF pathways [7], contributing to ccRCC tumorigenesis and progression. Given the functional impact of SALL4 on angiogenesis and decreased VEGFA level in CM from SALL4-downregulated ACHN cells, we further investigated whether SALL4 modulates the synthesis of VEGFA, a downstream target of VHL/HIF pathway. We observed that depletion of SALL4 led to a dramatic reduction in VEGFA protein levels in ACHN and 786-O cells (Fig. ​(Fig.5a,5a, b), thus suggesting a link between SALL4 expression and VHL/HIF pathway. Collectively, these results indicate that SALL4 expression positively correlates with the activation of Akt/GSK-3β signaling and VEGFA expression.

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Fig. 5

SALL4 downregulation attenuates the activation of Akt/GSK-3β signaling and VEGFA expression in ccRCC. a, b Western blot analyses for protein levels of total Akt (t-Akt), phosphorylated Akt (p-Akt), total GSK-3β (t-GSK-3β), phosphorylated GSK-3β (p-GSK-3β) and VEGFA in ACHN (a) and 786-O (b) cells with indicated treatment. c Immunofluorescence staining of p-Akt and p-GSK-3β in ACHN (left) and 786-O (right) cells with indicated treatment (scale bar, 50μm)

We would like to thank Chong Liu from Medical Laboratory and Research Center, Tangdu Hospital, Fourth Military Medical University for the technical support.