• We are sorry, but NCBI web applications do not support your browser and may not function properly. More information
Logo of brjcancerBJC HomepageBJC Advance online publicationBJC Current IssueSubmitting an article to BJCWeb feeds
Br J Cancer. Jan 5, 2010; 102(1): 196–205.
Published online Dec 1, 2009. doi:  10.1038/sj.bjc.6605451
PMCID: PMC2813755

Notch1 regulates the functional contribution of RhoC to cervical carcinoma progression

Abstract

Background:

The role of Notch signalling in human epithelial cancers is of immense interest. In this study, we examine the interplay between Notch signalling and RhoC, a well-established molecular factor in metastasis. By linking the function of Notch and RhoC, we further strengthen the notion that there is a pro-oncogenic role of Notch signalling in human cervical cancers.

Methods:

RhoC protein expression in cervical carcinoma cell lines was assessed by western blotting. Using CaSki and SiHa cells (cervical carcinoma cells lines), we show that RhoC contributes to wound healing, invasion and migration, anoikis resistance, colony formation, in vitro tube formation and tumour formation. Immunohistochemical studies were carried out to assess the co-expression of RhoC, pAkt and Notch1 in clinical sections.

Results:

An assessment of the changes associated with epithelial-to-mesenchymal transition (EMT) shows that both Notch1 and RhoC have similar phenotypic contribution to EMT. Rho activity assessment on Notch1 inhibition with DAPT shows decreased RhoC activity. We further show that constitutively active RhoC rescues the phenotypic effect of Notch1 inactivation, and a comparison of Notch1 with RhoC expression shows an overlap between the two proteins in the same areas of the tissue.

Conclusion:

This study has provided evidence to suggest that RhoC is an effector of Notch1 in cervical carcinoma.

Keywords: Notch1, RhoC, cervical carcinoma, angiogenesis, invasion, PI3K/Akt

Notch has an important role in cell fate determination, stem cell maintenance and development (Artavanis-Tsakonas et al, 1999). Notch1 signalling regulates the maintenance of haematopoietic stem cells and the development of T cells (Allman et al, 2002). The Notch receptor is activated on DSL ligand interaction-induced proteolytic cleavage, leading to the formation of intracellular Notch1 (ICN). Intracellular Notch1 translocates to the nucleus and acts as a transcriptional modulator (Honjo, 1996). Activating mutations have been reported in human T-ALL Notch1 (Weng et al, 2004); however, limited sequencing of a similar region in Notch1 alleles of cervical carcinoma suggests the absence of such a mutation (D Subramanyam and S Krishna, unpublished data). Dysregulated Notch signalling has been implicated in other tumours including mammary and cervical cancer (Zagouras et al, 1995; Daniel et al, 1997; Politi et al, 2004). Cervical carcinoma, the second most prevalent cancer in women, is initiated and sustained in part by the presence of high-risk human papillomavirus oncogene expression (zur Hausen, 2002), and has an aberrant expression of Notch1, its ligand Jagged1 and downstream target Hes1 (Ramdass et al, 2007).

There is a wealth of data suggesting the contribution of ICN to features of tumour progression, including invasion, epithelial-to-mesenchymal transition (EMT), metastasis and angiogenesis (Timmerman et al, 2004; Wang et al, 2006, 2007; Zhang et al, 2008). Notch1 induces anoikis resistance, inhibits p53 activity and upregulates myc in cervical carcinoma (Rangarajan et al, 2001; Nair et al, 2003; Klinakis et al, 2006; Subramanyam and Krishna, 2006; Weng et al, 2006) and also inhibits the growth inhibitory effects of TGF-β during cell growth (Masuda et al, 2005). Our earlier report suggests that PI3K-mediated EMT in cervical cancer correlates with Jagged1 expression (Veeraraghavalu et al, 2005). Although there is data supporting the role of Notch1 in tumour progression, there is paucity of evidence of factors downstream of it that regulate these processes. There is emerging evidence that RhoC regulates features of tumour progression. It regulates invasion, metastasis, EMT and angiogenesis in various carcinomas (Sequeira et al, 2008; Wang et al, 2008; Boone et al, 2009), regulating features similar to Notch1.

RhoC, a small GTPase, belongs to the Rho GTPase family. Activated Rho GTPases affect actin cytoskeleton dynamics, transcriptional regulation, cell cycle progression, membrane trafficking and tumour progression (Vega and Ridley, 2008). It has also been shown that functional Rho GTPases are required for Ras-dependent transformation (Qiu et al, 1995). Genomic comparison of melanoma variants suggested that proteins regulating actin organisation, such as RhoC, were overexpressed in highly metastatic melanoma cells (Clark et al, 2000). It has also been shown to regulate tumour progression in various carcinomas (Suwa et al, 1998; Clark et al, 2000; Kleer et al, 2002; Kondo et al, 2004). He et al (2008) showed that RhoC-siRNA (short-interfering RNA) reduced adhesion to Matrigel invasion and migration of SiHa cells. Studies indicate that a cross-talk exists between RhoC and other signalling molecules such as MAPK and vascular endothelial growth factor (Vegf). RhoC modulates the MAPK pathway and increases Vegf, basic fibroblastic growth factor and interleukins 6 and 8 expression (van Golen et al, 2000a, 2002). In another study, RhoC-siRNA inhibited the growth and invasion of gastric carcinoma cells through the PI3K/Akt pathway (Sun et al, 2007), and regulated Pyk2 during tumour metastasis (Iiizumi et al, 2008).

In the absence of reported mutations of the Notch1 locus, as in leukaemias (Weng et al, 2004), the mechanism of Notch activation is likely to involve dysregulated ligand expression or altered patterns of modifiers of the pathway. As phenotypically both Notch and RhoC signalling molecules regulate similar features during tumour progression, we explore the possibility of RhoC being a downstream effector of Notch1. Our results show that RhoC contributes to invasion, EMT, anoikis resistance, tumour growth and angiogenesis in cervical carcinoma. We show that inhibition of Notch1 inactivated the RhoC protein. Using a combination of genetic and molecular tools, we show that Notch1 inactivation can be rescued by RhoC. Constitutively active RhoC (caRhoC) can rescue phenotypic changes associated with siRNA-mediated Notch1 inactivation. Immunohistochemical analysis of archival tissue suggests a correlation between RhoC and Notch1 expression in human cervical carcinoma tissues. The results imply that RhoC is an effector of Notch1.

Materials and methods

Cell culture and reagents

CaSki, SiHa and HaCaT cells were cultured in 1 × Dulbecco's modified Eagle's medium (DMEM) containing 10% FBS (foetal bovine serum) and penicillin/streptomycin (100 μg ml−1) at 37°C in 5% CO2 atmosphere. LY294002, GGTI and DAPT were purchased from Calbiochem (Darmstadt, Germany) and Sigma (Poole, UK). The following plasmid constructs were used: pcDNA3-Neo (Invitrogen, Carlsbad, USA), wild-type RhoC (wtRhoC) and dominant-negative RhoC (dnRhoC) (UMR cDNA Resource Center), mouse caRhoC (gift from Professor SA Baldwin), glutathione S-transferase-Rho binding domain (GST-RBD) (gift from Professor A Ridley) and dn-Akt (Rangarajan et al, 2001). To generate stable clones, transfected cells were treated with G418 and drug-resistant colonies were selected after RhoC expression analysis. All transfections were carried out with Lipofectamine 2000 (Invitrogen), as specified by the manufacturer.

RNA interference

Short-interfering RNAs for Notch1 (ID 16704), RhoC (ID 120897) and negative control (−ve siRNA) were purchased from Ambion (Austin, TX, USA). After transfection with 30 pmol of siRNA, using Lipofectamine 2000 (Invitrogen), cells were cultured for 48 h before harvesting for further experiments.

The Notch1 (N1)-shRNA and scrambled shRNA was cloned in GenScript vector (pRNATin-H1.2/Neo) as a BamHI/HindIII fragment.

N1-shRNA: (5′-GGATCCCACTCGCAGTGGAAGTCATTGATTGATATCCGTCAATGACTTCCACTGCGAGTTTTTTTCCAAAAGCTT) and scramble shRNA: (5′-GGATCCCAAGTCACGCTAGTGATAGAATTTGATATCCGATTCTATCACTAGCGTGACTTTTTTTTCCAAAAGCTT).

Immunoblotting

Cells washed with cold PBS were incubated with lysis buffer (20 mM Tris–HCl (pH 7.5), 150 mM NaCl, 1% NP-40, 1% (v/v) sodium deoxycholate, 0.1% (w/v) SDS, 50 mM NaF, 1 mM Na3VO4, 50 μg ml−1 PMSF, 1 μg ml−1 leupeptin, 1 μg ml−1 pepstatin) for 30 min on ice, homogenised with a 23-G needle and centrifuged at 14 000 r.p.m. for 10 min at 4°C. The lysate was resolved using SDS–PAGE, blotted and probed using the appropriate antibody. The primary antibodies used were β-actin (Sigma, clone AC-74), Notch1 (Sigma, cat. no. N6786), Vegf (Oncogene, Cambridge, MA, USA, PC-36) and RhoC (Santa Cruz Biotechnology, Inc., CA, USA, cat. no. sc-26481) at appropriate dilutions.

Immunohistochemistry

Immunohistochemistry was performed on formalin-fixed, paraffin-embedded tissue sections. Briefly, the sections were deparaffinised in xylene, followed by rehydration. After peroxide quenching and antigen retrieval with sodium citrate, the sections were incubated overnight at 4°C with the following antibodies: RhoC (Santa Cruz Biotechnology, Inc., cat. no. sc-26481), Notch1 (Santa Cruz Biotechnology, Inc.), Hifα (Santa Cruz Biotechnology, Inc, cat. no. sc-10790), Vegf (Oncogene, PC-36), Akt (Cell Signaling Technology, Beverly, MA, USA, clone 736E11) and anti-mouse CD31 (BD Pharmingen, CA, USA, cat. no. 550274). The sections were then successively incubated with biotinylated secondary antibody (Vector Laboratories, Burlingame, CA, USA) and streptavidin–HRP complex (Vector Laboratories) at room temperature for 40 min each. The colour was developed using DAB (3,3′-diaminobenzidine, Sigma, UK). After counterstaining with haematoxylin, sections were dehydrated, mounted and visualised under a microscope.

Immunoreactivity was considered significant when the characteristic immunostaining was observed in more than 10% of cells. The protein expression was classified as mild (+), moderate (++) and intense (+++) on the basis of the intensity of immunostaining.

Immunofluorescence

Cells grown on coverslips were fixed with 4% (w/v) paraformaldehyde (PFA) for 10 min at 37°C. The cells were quenched with 50 mM NH4Cl and permeabilised with 0.1% (v/v) Triton X-100 in PBS for 5 min. After blocking for 1 h with 0.2% (v/v) fish skin gelatin in PBS, the cells were incubated overnight with the following primary antibodies: anti-fibronectin (Sigma, cat. no. F6140), Notch1 (Santa Cruz Biotechnology), RhoC (Santa Cruz Biotechnology, Inc, cat. no. sc-26481) and Plakoglobin (Sigma, cat. no. P8087), followed by appropriate secondary antibody conjugates. Finally, the coverslips were mounted on microscope slides and imaged using Nikon Inverted Microscope ECLIPSE TE2000-S, Melville, NY, USA.

Wound-healing assay

Cells cultured to 95% confluence were scratched with a 10-μl pipette tip. Wounds were photographed at 0 h time point, followed by imaging at later time points, ensuing wound closure using a Nikon Inverted Microscope ECLIPSE TE2000-S. The nude area was measured using Image-Pro-Plus (Media Cybernetics, Bethesda, MD, USA) and percentage wound closure was calculated.

Anoikis assay

Cells were cultured in 1 × DMEM in PolyHEMA-coated dishes, harvested at different time points, fixed with 4% PFA, stained with Hoechst (1 μg ml−1; Sigma) and cell death was estimated by counting apoptotic nuclei using the Nikon Inverted Microscope ECLIPSE TE2000-S.

Soft agar colony formation

Cell lines were transfected with indicated plasmids and cultured for 48 h. They were trypsinised and 2 × 105 cells were mixed in 0.33% agar in DMEM containing 10% FBS and seeded into 35 mm dishes containing 0.5% agar in DMEM. Cells were grown for 21 days and 200 μl of medium was added every third day to the dishes. At the end of 21 days, 10 random fields were selected and colonies were counted using a Nikon Inverted Microscope ECLIPSE TE2000-S.

Invasion and motility assay

For motility and invasion assay, 0.5 × 106 cells in 1 × DMEM were seeded in the top chamber of uncoated or Matrigel-coated transwell filters with 8 μm pores (BD Biosciences, CA, USA). The bottom chamber contained 1 × DMEM with 10% FBS and served as a chemoattractant. After incubation for 20 h at 37°C, the cells at the bottom of the upper chamber were stained with Hoechst and counted under the Nikon Inverted Microscope ECLIPSE TE2000-S.

RhoC activity assays

Rho activity assays were performed using the GSTRBD fusion protein, Rhotekin (for Rho activity) (a gift from Professor Anne Ridley, UCL, London, UK). Briefly, glutathione sepharose was used to extract GST-RBD from BL21 cells expressing the GST-RBD fusion protein. Cultured mammalian cells (pharmacologically treated and untreated) were lysed using ice-cold lysis buffer (25 mM Hepes (pH 7.5), 150 mM NaCl, 10 mmol l−1 MgCl2, 1% NP-40, 1 mM EDTA, 25 mM NaF, 1 mM NaO4Va and 10% glycerol along with 2 mmol l−1 phenylmethylsulphonyl fluoride. Lysates were clarified, protein content was estimated using a BCA assay and an equal amount of protein was taken for the assay. GST-RBD-coupled sepharose beads were added to the lysates and incubated for 1 h at 4°C to pull down active RhoC. Beads were washed, denatured, separated by electrophoresis and transferred onto a nitrocellulose membrane for subsequent analysis by western blotting.

MTT assay

An equal number of cells were seeded in 96-well plates and cultured for varying hours. At given time points, the cells were washed with PBS, and 200 μl of MTT (Sigma) working solution (0.5 mg ml−1) was added to the wells and incubated at 37°C for 2 h. The media were removed and the converted dye was solubilised in 200 μl isopropanol. The absorbance of the converted dye was measured at a wavelength of 570 nm with background subtraction at 650 nm.

Tumour formation in nude mice

Cells were grown in 145-mm-diameter dishes to confluence, trypsinised, resuspended in 200 μl of 1 × DMEM and injected subcutaneously into the flanks of N:NIH-Swiss mice. Each mouse (aged between 6 and 8 weeks), were injected with 5 × 106 cells. After 21 days, the mice were killed and the tumour was weighed.

Measurement of tumour vascularity

To measure vascularity, the tumours were processed for immunohistochemical analysis by fixing the tumour overnight in 4% PFA and cryoprotecting in increasing concentrations of sucrose (10–30%). Tissues were embedded in O.C.T. embedding medium and 4 μm sections were collected. The cryosections were immunostained for RhoC and rat anti-mouse CD31 (BD Pharmingen). Sections were examined by light microscopy under magnifications × 400, and the number of blood vessels from 10 high-power fields was counted using the Nikon Inverted Microscope ECLIPSE TE2000-S.

In vitro tube formation assay

A 50-μl Matrigel bed (60%) was prepared in wells of 96-well plates and was allowed to set for 2 h at 37°C in 5% CO2 in a humidified incubator. A total of 7000 human umbilical vascular endothelial cells were seeded per well in EBM2 media (Cambrex, MD, USA). The media was supplemented with 50 μl of conditioned media for the assay and tube formation allowed for 16 h. The tubes were imaged using a Nikon Inverted Microscope ECLIPSE TE2000-S (at 200 × magnification) and the length of the tube was measured as the distance between two nodes using Image-Pro-Plus (Media Cybernetics).

Statistical analysis

Significance of data has been analysed by Student's t-test. The correlation of RhoC expression with cervical carcinoma and other parameters was analysed by the χ2-test.

Results

RhoC drives tumour progression in cervical carcinoma

The transition from in situ carcinoma to metastatic tumour in solid tumours involves motility, invasion, anoikis resistance and sustained growth. To assess the contribution of RhoC to invasion and metastasis, we used cervical carcinoma-derived CaSki and SiHa cells. Figure 1A-i and A-ii shows the expression levels of RhoC in CaSki and SiHa cells, with higher total RhoC and higher active RhoC levels in CaSki cells compared with SiHa cells. This phenotype was complemented in SiHa cells by stably expressing wtRhoC in stable clones (Supplementary Figure 1A). Dominant-negative RhoC was also stably expressed in CaSki and SiHa cells.

Figure 1
RhoC drives tumour progression in cervical carcinoma. (A-i) Cell extracts were analysed for RhoC expression in CaSki and SiHa cells. The SiHa cells show less RhoC expression and activity compared with CaSki cells (n=2). (A-ii) Graphical presentation of ...

To assess the contribution of RhoC to motility, we used stable clones of SiHa cells expressing wtRhoC and dnRhoC in a wound-healing assay. SiHa-wtRhoC cells closed 80% (P<0.05) of the wound area as compared with 35% by SiHa Neo cells (expressing empty vector) in 24 h (Figure 1A-iii and iv). The effect of RhoC depletion on motility and invasion of CaSki cells in a transwell chamber assay is shown in Figure 1A-v. Compared with control siRNA (−ve siRNA), RhoC-siRNA treatment resulted in a 75% (P<0.01) and 45% (P<0.02) decrease in motility and invasion, respectively, of CaSki cells. The specificity of siRNA activity has been shown in Supplementary Figure 1B. Immunofluorescent analysis of RhoC expression in squamous cervical carcinoma (SCC) tissues from patients shows the presence of RhoC-expressing cells in adjoining blood vessels (Supplementary Figure 1C), suggesting that RhoC is involved in metastasis.

Metastatic cells need to resist anoikis in blood vessels to re-grow as metastases at a distant site. Figure 1B-i shows that a reduction in RhoC protects cells from anoikis. When cultured for 7 h under anoikis, there were 30% (P<0.001) non-apoptotic CaSki-dnRhoC cells as compared with 57% non-apoptotic CaSki cells. Similarly, wtRhoC protected SiHa cells maximally from anoikis for 48 h (Supplementary Figure 1D).

CaSki and SiHa cells transiently expressing wtRhoC formed bigger colonies (Figure 1B-ii), whereas dnRhoC resulted in a lesser number of colonies (Figure 1B-iii) in a clonogenic assay. The number of colonies formed by the CaSki-dnRhoC clone (16 colonies/10 fields) was significantly less compared with CaSki cells forming 39 colonies/10 fields (P<0.003).

To determine the contribution of RhoC to tumour growth, we used (5 × 106 cells) stable clones of CaSki and SiHa cells expressing dnRhoC and wtRhoC, respectively, and generated xenografts in nude mice over a period of 21 days. As illustrated in Figure 1C-i and ii, the ectopic expression of RhoC and its mutant altered the tumour growth properties of CaSki and SiHa cells. SiHa-wtRhoC cells formed larger tumours (mean weight 353 mg; P<0.02) compared with SiHa cells (16 mg). Similarly, CaSki-dnRhoC cells formed tumours that were significantly smaller (0.016 g; P<0.047) than those formed by CaSki cells (0.054 g). Interestingly, the tumours formed by SiHa-wtRhoC cells were more angiogenic, with a high microvessel density of 12.5 (P<0.009) microvessels, as opposed to 1.75 in SiHa tumours (Figure 1D-i and ii; Supplementary Figure 2A). An immunohistochemical analysis for CD31 and RhoC on xenograft sections suggests CD31 localisation at the microvessels. We measured the effect of RhoC on in vitro tube formation using human umbilical vascular endothelial cells. As illustrated in Figure 1D-iii and iv, conditioned media derived from cultures of CaSki, CaSki-dnRhoC, SiHa and SiHa-wtRhoC cells were used to test the effect. There was significant loss in tube formation and a resultant reduction in tube length with CaSki-dnRhoC-derived media (33.66 μm; P<0.0001) as compared with CaSki (41.33 μm) media, whereas wtRhoC in SiHa cells enhanced the tube length (63.45 μm; P<0.001) as compared with SiHa cells. We extended these observations to clinical sections and assessed the expression of RhoC, Hifα and Vegf in matched cervical samples. Representative images suggest an expression of RhoC, Hifα and Vegf in the same area of the tumour (Figure 1E) with negligible immunodetection in normal cervix tissues suggesting a co-expression of these molecules. Moreover, a change was observed in Vegf expression because of RhoC expression. Supplementary Figure 2B shows that ectopic expressions of wtRhoC and dnRhoC resulted in elevated and reduced Vegf levels, respectively, in SiHa and CaSki cells.

Do Notch1 and RhoC regulate similar function during tumour progression?

Notch1 cooperates with various signalling pathways to promote tumour progression, including NF-κB, VEGF, TGF-β and p53 (Nair et al, 2003; Masuda et al, 2005; Wang et al, 2006). As both Notch1 and RhoC are involved in tumour progression and metastasis, we investigated whether the two signalling molecules regulate similar functions during cervical tumour progression. Treatment of SiHa and CaSki cells with DAPT (presenilin-dependent gamma-secretase inhibitor that blocks proteolytic processing of Notch1) blocked wound healing in CaSki cells but had no effect in SiHa cells (Supplementary Figure 2C). Furthermore, CaSki cells are phenotypically similar to most cervical cancers with regard to its expression of Jagged1, features of activated Notch1 and PI3K signalling and dependence on Notch1 signalling for growth and survival (Veeraraghavalu et al, 2005). We thus used CaSki cells to assess the relationship between RhoC and Notch1.

Depletion of Notch1 and RhoC with siRNA against Notch1 (N1-siRNA) and RhoC (RhoC-siRNA) inhibited motility and invasion in CaSki cells (Figure 2A). The motility of CaSki cells reduced to 25% (P<0.01) and 30% (P<0.01) for N1-siRNA- and RhoC-siRNA-transfected cells. There were 78% (P<0.01) and 66% (P<0.01) invading RhoC and Notch1 knockout cells compared with CaSki cells. The effect of N1-siRNA on Notch1 levels has been shown (Supplementary Figure 2D). Concurrently, in a wound-healing assay, inhibition of Notch1 with DAPT (40 μM), and that of PI3K with chemical inhibitor LY294002 (LY; 20 μM) and RhoGTPase inhibitor (geranylgeranyl transferase inhibitor (GGTI); 10 μM) for 14 h caused reduced wound healing with 24, 52 and 35% (P<0.03) wound closure, respectively, compared with DMSO-treated cells. Treatment of CaSki cells with the above inhibitors also resulted in RhoC localisation changes (Supplementary Figure 2E).

Figure 2
Does Notch1 and RhoC regulate similar function during tumour progression. (A) RhoC-siRNA and N1-siRNA reduced motility (P<0.05) and invasion (P<0.05) of CaSki cells. −ve siRNA did not alter motility and invasion of CaSki cells. ...

As reported earlier, the Notch1 ligand, Jagged1, generates EMT response in CaSki cells in a Notch1-PI3K-dependent but CBF-independent manner (Veeraraghavalu et al, 2005). In this study, CaSki cells transfected with N1-siRNA, RhoC-siRNA and dominant-negative Akt (dn-Akt) were subjected to wound healing for 14 h and assessed for fibronectin, plakoglobin and actin stress fibre organisation. With the progression of wound healing, there was elevated fibronectin expression and actin stress fibre formation in untreated CaSki cells at 14 h (Figure 2C); however, N1-siRNA, RhoC-siRNA and dnAkt prevented fibronectin expression and actin stress fibre formation in cells adjoining the wound site. Control cells at the 0 h time point neither showed fibronectin expression nor had actin stress fibre formation. Plakoglobin expression was lost in untreated cells during wound healing at 14 h but contrary to reversal of fibronectin expression, plakoglobin expression showed no reversal with inhibitors. The data collectively suggest that RhoC phenocopies the effect of Notch1 in EMT and invasion.

Is RhoC function regulated by Notch1?

The phenotypic similarity between Notch1 and RhoC suggests that RhoC may be regulated by Notch1. To assess this relationship, we used GST-RBD (Taylor et al, 2001) to pull down active RhoC-GTP after treating the cells with the Notch and PI3K inhibitors. Figure 3A illustrates that the RhoC activation level is decreased after Notch1 inhibition. The same results were obtained after PI3K inhibition, indicating that RhoC, which phenocopies the Notch1 effect on EMT, is regulated by the latter. SiHa cells that lack Jagged1 were used to assess the regulation of RhoC by Notch1. As shown in Figure 3B-i and -ii, overexpression of wtRhoC and Jagged1 in SiHa cells formed big (diameter >30 mm) colonies (6 and 13/10 fields, respectively) in a clonogenic assay. Co-expression of dnRhoC in Jagged1-expressing SiHa cells led to the abolition of big colonies (P<0.005). We also show that inhibition of PI3K resulted in the abolition of colonies formed by Jagged1 (Figure 3B-i). This is in agreement with an earlier report that PI3K mediates Jagged1-mediated EMT changes (Veeraraghavalu et al, 2005). The Notch1 expression in HaCaT cells (HaCaT-ACN1) enhances anoikis resistance through the PKB/Akt pathway (Rangarajan et al, 2001). In this study, we show that GGTI treatment resulted in reduced anoikis resistance of HaCaT-ACN1 cells. HaCaT-ACN1 cells showed 33% non-apoptotic cells at 14 h, which reduced to 10% (P<0.002) on treatment with GGTI (Figure 3B-iii).

Figure 3
Is RhoC function regulated by Notch1. (A-i) RBD-GST pull down protein extracts of CaSki cells treated with DAPT, LY and GGTI were assessed for levels of active RhoC. The crude protein extracts were immunoblotted for total RhoC and β-actin (indicating ...

Rescue of RNAi-mediated loss-of-function phenotype by expressing caRhoC, which is refractory to upstream signalling events, was used to further corroborate RhoC as a downstream target of Notch1. Ectopic expression of caRhoC in CaSki cells with depleted Notch1, by N1-siRNA or Notch1 shRNA (N1-shRNA), rescued the loss-of-function phenotype of Notch1. As shown in Figure 3C-i, the N1-siRNA expression in CaSki cells reduced colonies to 15/10 fields compared with 32 control colonies. Expectedly, co-expression of caRhoC resulted in significantly increased colonies (49/10 fields; P<0.0001). Similarly, caRhoC also rescued the inhibition of the motility and invasion of CaSki cells because of N1-siRNA expression. Co-expression of caRhoC resulted in a significant increase in motility (151%; P<0.005) and invasion (173%; P<0.04) compared with N1-siRNA (51% motility and 82% invasion)-transfected cells (Figure 3C-ii). Co-expression of caRhoC in CaSki cells carrying N1-shRNA also enhanced anoikis resistance (68% non-apoptotic cells; P<0.005) compared with N1-shRNA cells (40% non-apoptotic cells). The specificity of N1-shRNA and N1-siRNA has been shown in Supplementary Figure 2D.

As RhoC inhibition phenocopied the Notch1 and PI3K inhibitory phenotype, we used CaSki-dnAkt cells (Rangarajan et al, 2001) to confirm the effect of PI3K inhibition of RhoC activity in Figure 3A. Expression of dnAkt in CaSki cells caused decreased motility and enhanced anoikis. As shown in Figure 3D-i, there was significant reduction in the motility of CaSki-dnAkt cells (16%; P<0.003) compared with CaSki cells. RhoC activity as assessed by RBD-GST binding suggested a decreased activity of RhoC in CaSki-dnAkt cells (Figure 3D-ii). Subsequently, as expected, overexpression of caRhoC in CaSki-dnAkt cells generated enhanced anoikis resistance (25% non-apoptotic cells; P<0.01) compared with 12% non-apoptotic CaSki-dnAkt cells in 14 h. These results convincingly position RhoC as a downstream effector of Notch1 and PI3K signalling in cervical carcinoma cells.

RhoC expression correlates with Notch1 expression in cervical tumour progression

To further corroborate our findings in a clinical setting, we examined the expression of RhoC and its relationship with Notch1 in archival cervical carcinoma specimens using immunohistochemical technique. The specimens were randomly selected and the expression of Notch1, RhoC and pAkt was assessed in them. Our results suggest RhoC is strongly expressed in SCC tissues (Figure 4A). There was significant difference in the extent of cellular positivity and intensity of RhoC expression across the grades (P<0.007). Although cytoplasmic expression of RhoC was observed in all the cases across all grades of tissues, the percentage of positive cases increased across the tumour grades. Only 5 out of 12 (41%) normal cervical tissues showed RhoC expression compared with 21 out of 24 (87%) SCC tissues. Of the 87% cases, 65% had mild, 14% had moderate and 8% had intense RhoC expression.

Figure 4
RhoC expression correlates with Notch1 expression in cervical tumour progression. Immunodetection of Notch1, RhoC and pAkt in cervical carcinoma. Immunohistochemical analysis was carried out on paraffin-embedded cervical carcinoma tissue sections using ...

Correlation of RhoC with Notch1 and pAkt was assessed on serial sections of SCC tissues and all the molecules were found to be expressed in the same areas of the various tumour sections (Figure 4B). Importantly, RhoC expression in the SCC specimens showed significant correlation with Notch1 expression (P<0.006) and pAkt expression (P<0.006). Out of 17 SCC specimens, RhoC was expressed in 14 specimens, whereas Notch1 and pAkt expression was observed in all 17 specimens. These data collectively suggest a correlation between RhoC, Notch1 and pAkt. We thus propose RhoC to be a downstream effector of Notch1 in cervical tumour progression.

Discussion

Carcinoma progression is a multi-step process engaging various signalling pathways. There are surmounting evidences elucidating the contribution of two such pathways including Notch1 and RhoC to carcinoma progression. Notch1 has been shown to exert regulations on tumour growth, invasion, metastasis and angiogenesis in various carcinomas. Increased expression of RhoC in metastatic melanoma cells in comparison with the poorly metastatic counterparts (Clark et al, 2000) was the advent of studies implicating RhoC in carcinoma progression especially metastasis.

In accordance with its contribution to motility and invasion of several cancers (van Golen et al, 2000b; He et al, 2008), our data show that RhoC contributes to tumour progression by affecting invasion, anoikis resistance, tumour growth and angiogenesis in cervical carcinoma cell lines. We show that RhoC drives tumour progression by regulating invasion, metastasis, tumour growth and angiogenesis (Figure 1). We find increased vasculature associated with increased RhoC expression in xenografts grown from SiHa cells. Immunohistochemical assessment of archival tissue sections showed expression of RhoC, Vegf and Hifα in the same areas of tumour sections. Immunofluorescent analysis of paraffin-embedded SCC tissue sections for RhoC expression showed the presence of invading cells in the adjoining blood vessels and at the periphery of the tumour, underlining the importance of RhoC to invasion.

We previously proposed that Notch1 regulates EMT response in the cervical epithelial cell line, CaSki (Veeraraghavalu et al, 2005). In this study, we show that RhoC regulates EMT during tumour progression in a manner similar to Notch1. Inactivation of RhoC resulted in similar phenotypic changes, as associated with the effect of Notch and PI3K inhibition of EMT (Figure 2). This finding parallels that of Hutchison et al (2009), in which RhoC has been shown to regulate stress fibre formation during EMT. However, we also show that RhoC regulates fibronectin expression during EMT changes. Considering that both Notch1 and RhoC regulate similar features during tumour progression, we explored the possibility of cross-talk between Notch1 and RhoC. Biochemical assays suggest that Notch1 regulates RhoC activity in CaSki cells. In this study, we show that inhibition of Notch and PI3K with pharmacological agents resulted in reduced RhoC activity in CaSki cells (Figure 3), with no effect on total RhoC levels. When SiHa cell-overexpressing Jagged1 was complemented with dnRhoC, there was reduced colony formation. Concomitantly, HaCaT-ACN1 cells (Rangarajan et al, 2001) when treated with GGTI resulted in reduced anoikis-resistant cells. Consistent with the observation that Notch1 signalling generates anoikis to resistance in keratinocytes and CaSki cells (Rangarajan et al, 2001; Veeraraghavalu et al, 2005), we find that complementation of Notch1-depleted CaSki cells with caRhoC resulted in increased resistance to anoikis. In parallel, CaSki cells, expressing Notch1 siRNA or shRNA, when complemented with caRhoC formed more colonies in a colony formation assay (Figure 3). Dominant-negative Akt also reduced RhoC activity in CaSki cells. When CaSki-dnAkt cells were complemented with caRhoC, there was resultant increase in non-apoptotic cells. However, it should be noted that RhoC promotes invasion of human melanoma cells in a PI3K/Akt-dependent manner and promotes metastasis of prostrate cancer cells by activation of Pyk2, which regulates Akt phosphorylation (Ruth et al, 2006; Iiizumi et al, 2008).

Using immunohistochemical techniques, we show that there is expression of both Notch1 and RhoC in the same areas of cervical carcinoma tissue sections with significant correlation while there was negligible expression of the proteins in the normal cervical tissue sections (Figure 4). We observed that Notch1 activation and activated PI3K/Akt regulate RhoC activity in CaSki cells; but we cannot rule out the role of other signalling pathways regulating RhoC activity. SiHa cells, for example, lack Jagged1-activated Notch1 signalling (Veeraraghavalu et al, 2005), yet they exhibit RhoC activity, which may be regulated by another signalling pathway. Notch1, which has no reported mutation in solid tumours, may likely use downstream effectors to execute its functions in tumour progression. We thus propose RhoC as downstream effector of Notch1 during tumour progression. Interestingly, RhoC is not imperative for embryogenesis but is important for metastasis alone (Hakem et al, 2005), and thus it can serve as a good therapeutic target. Our data re-iterates the role of Notch1 in carcinoma progression and places RhoC as its downstream target.

Supplementary Material

Supplementary Figures 1 and 2:

Acknowledgments

We thank Professor Anne Ridley, KCL, UK, for providing RBD-GST construct. We thank Professor SA Baldwin, University of Leeds, UK, for providing RhoC plasmids. This study was supported by core funding from NCBS, TIFR and a grant support by DBT (Department of Biotechnology, Government of India).

Notes

Supplementary Information accompanies the paper on British Journal of Cancer website (http://www.nature.com/bjc)

References

  • Allman D, Aster JC, Pear WS. Notch signaling in hematopoiesis and early lymphocyte development. Immunol Rev. 2002;187:75–86. [PubMed]
  • Artavanis-Tsakonas S, Rand MD, Lake RJ. Notch signaling: cell fate control and signal integration in development. Science. 1999;284:770–776. [PubMed]
  • Boone B, Van Gele M, Lambert J, Haspeslagh M, Brochez L. The role of RhoC in growth and metastatic capacity of melanoma. J Cutan Pathol. 2009;36:629–636. [PubMed]
  • Clark EA, Golub TR, Lander ES, Hynes RO. Genomic analysis of metastasis reveals an essential role for RhoC. Nature. 2000;406:532–535. [PubMed]
  • Daniel B, Rangarajan A, Mukherjee G, Vallikad E, Krishna S. The link between integration and expression of human papillomavirus type 16 genomes and cellular changes in the evolution of cervical intraepithelial neoplastic lesions. J Gen Virol. 1997;78 Part 5:1095–1101. [PubMed]
  • Hakem A, Sanchez-Sweatman O, You-Ten A, Duncan G, Wakeham A, Khokha R, Mak TW. RhoC is dispensable for embryogenesis and tumor initiation but essential for metastasis. Genes Dev. 2005;19:1974–1979. [PMC free article] [PubMed]
  • He X, Qian Y, Cai H, Wang Z. The effect of RhoC siRNA on the invasiveness and proliferation of human cervical cancer cell line SiHa cells. J Huazhong Univ Sci Technolog Med Sci. 2008;28:665–669. [PubMed]
  • Honjo T. The shortest path from the surface to the nucleus: RBP-J kappa/Su(H) transcription factor. Genes Cells. 1996;1:1–9. [PubMed]
  • Hutchison N, Hendry BM, Sharpe CC. Rho isoforms have distinct and specific functions in the process of epithelial to mesenchymal transition in renal proximal tubular cells. Cell Signal. 2009;21:1522–1531. [PubMed]
  • Iiizumi M, Bandyopadhyay S, Pai SK, Watabe M, Hirota S, Hosobe S, Tsukada T, Miura K, Saito K, Furuta E, Liu W, Xing F, Okuda H, Kobayashi A, Watabe K. RhoC promotes metastasis via activation of the Pyk2 pathway in prostate cancer. Cancer Res. 2008;68:7613–7620. [PMC free article] [PubMed]
  • Kleer CG, van Golen KL, Zhang Y, Wu ZF, Rubin MA, Merajver SD. Characterization of RhoC expression in benign and malignant breast disease: a potential new marker for small breast carcinomas with metastatic ability. Am J Pathol. 2002;160:579–584. [PMC free article] [PubMed]
  • Klinakis A, Szabolcs M, Politi K, Kiaris H, Artavanis-Tsakonas S, Efstratiadis A. Myc is a Notch1 transcriptional target and a requisite for Notch1-induced mammary tumorigenesis in mice. Proc Natl Acad Sci USA. 2006;103:9262–9267. [PMC free article] [PubMed]
  • Kondo T, Sentani K, Oue N, Yoshida K, Nakayama H, Yasui W. Expression of RHOC is associated with metastasis of gastric carcinomas. Pathobiology. 2004;71:19–25. [PubMed]
  • Masuda S, Kumano K, Shimizu K, Imai Y, Kurokawa M, Ogawa S, Miyagishi M, Taira K, Hirai H, Chiba S. Notch1 oncoprotein antagonizes TGF-beta/Smad-mediated cell growth suppression via sequestration of coactivator p300. Cancer Sci. 2005;96:274–282. [PubMed]
  • Nair P, Somasundaram K, Krishna S. Activated Notch1 inhibits p53-induced apoptosis and sustains transformation by human papillomavirus type 16 E6 and E7 oncogenes through a PI3K-PKB/Akt-dependent pathway. J Virol. 2003;77:7106–7112. [PMC free article] [PubMed]
  • Politi K, Feirt N, Kitajewski J. Notch in mammary gland development and breast cancer. Semin Cancer Biol. 2004;14:341–347. [PubMed]
  • Qiu RG, Chen J, McCormick F, Symons M. A role for Rho in Ras transformation. Proc Natl Acad Sci USA. 1995;92:11781–11785. [PMC free article] [PubMed]
  • Ramdass B, Maliekal TT, Lakshmi S, Rehman M, Rema P, Nair P, Mukherjee G, Reddy BK, Krishna S, Radhakrishna Pillai M. Coexpression of Notch1 and NF-kappaB signaling pathway components in human cervical cancer progression. Gynecol Oncol. 2007;104:352–361. [PubMed]
  • Rangarajan A, Syal R, Selvarajah S, Chakrabarti O, Sarin A, Krishna S. Activated Notch1 signaling cooperates with papillomavirus oncogenes in transformation and generates resistance to apoptosis on matrix withdrawal through PKB/Akt. Virology. 2001;286:23–30. [PubMed]
  • Ruth MC, Xu Y, Maxwell IH, Ahn NG, Norris DA, Shellman YG. RhoC promotes human melanoma invasion in a PI3K/Akt-dependent pathway. J Invest Dermatol. 2006;126:862–868. [PubMed]
  • Sequeira L, Dubyk CW, Riesenberger TA, Cooper CR, van Golen KL. Rho GTPases in PC-3 prostate cancer cell morphology, invasion and tumor cell diapedesis. Clin Exp Metastasis. 2008;25:569–579. [PubMed]
  • Subramanyam D, Krishna S. c-Myc substitutes for Notch1-CBF1 functions in cooperative transformation with papillomavirus oncogenes. Virology. 2006;347:191–198. [PubMed]
  • Sun HW, Tong SL, He J, Wang Q, Zou L, Ma SJ, Tan HY, Luo JF, Wu HX. RhoA and RhoC-siRNA inhibit the proliferation and invasiveness activity of human gastric carcinoma by Rho/PI3K/Akt pathway. World J Gastroenterol. 2007;13:3517–3522. [PMC free article] [PubMed]
  • Suwa H, Ohshio G, Imamura T, Watanabe G, Arii S, Imamura M, Narumiya S, Hiai H, Fukumoto M. Overexpression of the rhoC gene correlates with progression of ductal adenocarcinoma of the pancreas. Br J Cancer. 1998;77:147–152. [PMC free article] [PubMed]
  • Taylor SJ, Resnick RJ, Shalloway D. Nonradioactive determination of Ras-GTP levels using activated ras interaction assay. Methods Enzymol. 2001;333:333–342. [PubMed]
  • Timmerman LA, Grego-Bessa J, Raya A, Bertran E, Perez-Pomares JM, Diez J, Aranda S, Palomo S, McCormick F, Izpisua-Belmonte JC, de la Pompa JL. Notch promotes epithelial–mesenchymal transition during cardiac development and oncogenic transformation. Genes Dev. 2004;18:99–115. [PMC free article] [PubMed]
  • van Golen KL, Bao LW, Pan Q, Miller FR, Wu ZF, Merajver SD. Mitogen activated protein kinase pathway is involved in RhoC GTPase induced motility, invasion and angiogenesis in inflammatory breast cancer. Clin Exp Metastasis. 2002;19:301–311. [PubMed]
  • van Golen KL, Wu ZF, Qiao XT, Bao L, Merajver SD. RhoC GTPase overexpression modulates induction of angiogenic factors in breast cells. Neoplasia. 2000a;2:418–425. [PMC free article] [PubMed]
  • van Golen KL, Wu ZF, Qiao XT, Bao LW, Merajver SD. RhoC GTPase, a novel transforming oncogene for human mammary epithelial cells that partially recapitulates the inflammatory breast cancer phenotype. Cancer Res. 2000b;60:5832–5838. [PubMed]
  • Veeraraghavalu K, Subbaiah VK, Srivastava S, Chakrabarti O, Syal R, Krishna S. Complementation of human papillomavirus type 16 E6 and E7 by Jagged1-specific Notch1-phosphatidylinositol 3-kinase signaling involves pleiotropic oncogenic functions independent of CBF1;Su(H);Lag-1 activation. J Virol. 2005;79:7889–7898. [PMC free article] [PubMed]
  • Vega FM, Ridley AJ. Rho GTPases in cancer cell biology. FEBS Lett. 2008;582:2093–2101. [PubMed]
  • Wang W, Wu F, Fang F, Tao Y, Yang L. RhoC is essential for angiogenesis induced by hepatocellular carcinoma cells via regulation of endothelial cell organization. Cancer Sci. 2008;99:2012–2018. [PubMed]
  • Wang Z, Banerjee S, Li Y, Rahman KM, Zhang Y, Sarkar FH. Down-regulation of notch-1 inhibits invasion by inactivation of nuclear factor-kappaB, vascular endothelial growth factor, and matrix metalloproteinase-9 in pancreatic cancer cells. Cancer Res. 2006;66:2778–2784. [PubMed]
  • Wang Z, Kong D, Banerjee S, Li Y, Adsay NV, Abbruzzese J, Sarkar FH. Down-regulation of platelet-derived growth factor-D inhibits cell growth and angiogenesis through inactivation of Notch-1 and nuclear factor-kappaB signaling. Cancer Res. 2007;67:11377–11385. [PubMed]
  • Weng AP, Ferrando AA, Lee W, Morris JPt, Silverman LB, Sanchez-Irizarry C, Blacklow SC, Look AT, Aster JC. Activating mutations of NOTCH1 in human T cell acute lymphoblastic leukemia. Science. 2004;306:269–271. [PubMed]
  • Weng AP, Millholland JM, Yashiro-Ohtani Y, Arcangeli ML, Lau A, Wai C, Del Bianco C, Rodriguez CG, Sai H, Tobias J, Li Y, Wolfe MS, Shachaf C, Felsher D, Blacklow SC, Pear WS, Aster JC. c-Myc is an important direct target of Notch1 in T-cell acute lymphoblastic leukemia/lymphoma. Genes Dev. 2006;20:2096–2109. [PMC free article] [PubMed]
  • Zagouras P, Stifani S, Blaumueller CM, Carcangiu ML, Artavanis-Tsakonas S. Alterations in Notch signaling in neoplastic lesions of the human cervix. Proc Natl Acad Sci USA. 1995;92:6414–6418. [PMC free article] [PubMed]
  • Zhang P, Yang Y, Zweidler-McKay PA, Hughes DP. Critical role of notch signaling in osteosarcoma invasion and metastasis. Clin Cancer Res. 2008;14:2962–2969. [PMC free article] [PubMed]
  • zur Hausen H. Papillomaviruses and cancer: from basic studies to clinical application. Nat Rev Cancer. 2002;2:342–350. [PubMed]

Articles from British Journal of Cancer are provided here courtesy of Cancer Research UK
PubReader format: click here to try

Formats:

Related citations in PubMed

See reviews...See all...

Cited by other articles in PMC

See all...

Links

Recent Activity

Your browsing activity is empty.

Activity recording is turned off.

Turn recording back on

See more...