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Department of Oral and Dental Science, Division of Oral Medicine, Pathology and Microbiology, Bristol Dental Hospital and School, University of Bristol, Lower Maudlin Street, Bristol BS1 2LY, United Kingdom;
* corresponding author, Stephen.prime{at}bristol.ac.uk
Abstract (I) Introduction (II) Defects in Signal Transduction (A) RECEPTOR ANOMALIES (B) SMAD PROTEIN DEFECTS (III) Abnormalities in Smad Co-activators and Co-repressors (IV) Ligand Expression and Activation (V) Epithelial-Mesenchymal Transition (A) MORPHOLOGICAL CHANGES (B) EVIDENCE FOR TUMOR PROMOTION (VI) Metastases (VII) Oral Cancer (A) RAT-4,NITROQUINOLINE N OXIDE (4NQO) MODEL OF ORAL CARCINOGENESIS (B) HUMAN ORAL CANCER (VIII) Concluding Remarks Acknowledgments REFERENCES
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Key words. TGF-ß, epithelial, oral, cancer
| (I) Introduction |
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; Derynck et al., 2001; Roberts and Wakefield, 2003).
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| (II) Defects in Signal Transduction |
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) and are described below.
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Analysis of recent data has shown that there is an alternative mechanism by which tumor cells escape the negative effects of TGF-ß, and this is by the transcriptional repression of TGF-ß receptors (Kim et al., 2000). TßR-II transcription, for example, has been shown to be down-regulated by mutations in the TßR-II promoter (Munoz-Antonia et al., 1996; Seijo et al., 2001), oncogenic Ras (Zhao and Buick, 1995), over-expression of cyclin D (Okamoto et al., 1994), and epigenetic alterations such as histone deacetylation of the TßR-II promoter (Osada et al., 2001; Zhao et al., 2003) and methylation-mediated repression of the transcription factor, Sp1 (Jennings et al., 2001; Venkatasubbarao et al., 2001). Similarly, transcriptional repression of TßR-I has been shown to be due to hyper-methylation of the TßR-I promoter (Kang et al., 1999).
The biological consequences of attenuation of TGF-ß receptor activity are starting to be elucidated. Analysis of early data demonstrated that decreased TßR-II signaling conferred resistance to the growth-inhibitory effects of TGF-ß, with retention of other transcriptional responses, suggesting that the signal transduction pathway(s) leading to cell-cycle arrest were distinct from those that mediated other effects of TGF-ß (Chen et al., 1993). More recently, it has been shown that different signaling pathways and biological responses require different thresholds of TGF-ß activation (Yingling et al., 1995; McEarchern et al., 2001). Specifically, higher levels of TßR-I signaling are required to phosphorylate Smad2 than to activate the PI3K and MAPK pathways (Dumont et al., 2003), and, presumably, the pro-oncogenic effects of TGF-ß predominate in circumstances of low thresholds of TGF-ß activity. In some studies, TGF-ß signaling has been shown to be required for invasion and metastasis of carcinoma cells (Oft et al., 1998; McEarchern et al., 2001; Tang et al., 2003), and analysis of recent data shows that this is dependent upon an intact Smad pathway (Oft et al., 2002; Tian et al., 2003). Analysis of these data suggests that, in circumstances in which the tumor-suppressor properties of TGF-ß have been compromised, the Smad pathway can function to promote a more aggressive phenotype. Interestingly, colon cancers that contain mutant TßR-II—and therefore the complete absence of both tumor-suppressor and pro-oncogenic TGF-ß pathways—have a better prognosis than their counterparts with wild-type TGF-ß receptors (Bubb et al., 1996). Further, decreased expression of TßR-II correlates with high tumor grade in a variety of human and experimental tumors (S Kim et al., 2000; J Kim et al., 2001).
A recent development is the observation that the accessory receptor NMA (BAMBI) is a downstream target of the Wnt signaling pathway, and that NMA is aberrantly over-expressed in a high proportion of colorectal and hepatocellular carcinomas (Sekiya et al., 2004). Over-expression of NMA in tumor cells inhibits their response to TGF-ß (Sekiya et al., 2004), suggesting that NMA may play a role in tumorigenesis, particularly in those tumors with constitutive ß-catenin signaling.
(B) SMAD PROTEIN DEFECTS
Smad4 was originally isolated as a tumor-suppressor gene on chromosome 18q21, a site that is frequently deleted or mutated in a large proportion of human pancreatic cancers (Hahn et al., 1996). Genetic inactivation of Smad4, however, is largely restricted to pancreatic and gastro-intestinal tumors and is uncommon in a broad spectrum of other solid tumors (Schutte et al., 1996). Transgenic mouse models of colorectal carcinogenesis have given some clues as to the biological significance of Smad4 inactivation and indicate that haploid insufficiency of Smad4 may be sufficient for tumor initiation, and that bi-allelic loss is important for tumor progression (de Caestecker et al., 2000). In support of this proposal, complete genetic inactivation of Smad4 appears to be a late event in human colorectal cancer (Miyaki et al., 1999). Immunocytochemical studies have shown that loss of Smad4 protein in human cancer may occur more frequently than would be predicted from genetic analyses, indicating that epigenetic mechanisms (Natsugoe et al., 2002; Salovaara et al., 2002) and/or other anomalies (Saha et al., 2001) may be involved in Smad4 silencing. Interestingly, loss of Smad4 protein expression is often associated with the development of the invasive/metastatic phenotype and, concomitantly, a worse clinical outcome (Maitra et al., 2000; Natsugoe et al., 2002; Xie et al., 2002).
The gene encoding Smad2 is also located at 18q21 and is the target of inactivating mutations in a small subset of colorectal and lung cancers only (Eppert et al., 1996; Riggins et al., 1996). The majority of mutations in Smad2 and Smad4 disrupt Smad-dependent TGF-ß signaling either by blocking receptor-dependent phosphorylation or by preventing heteromeric interactions between Smad proteins (Eppert et al., 1996; Shi et al., 1997). Certain mutations of Smad2 and Smad4, however, do not disrupt Smad activation or function, but rather target the mutant protein for ubiquitination and proteosome degradation (Xu and Attisano, 2000). Interestingly, loss of Smad4 has been shown to enhance the activity of the Ras/Erk pathway and to promote tumor progression in transformed keratinocytes containing mutant Ras (Iglesias et al., 2000).
Smad3 is located on chromosome 15q21-22 (Riggins et al., 1996), and this, again, is a frequent site of allelic loss in a broad spectrum of tumors (Hahn et al., 1995; Park et al., 2000). There is no evidence to suggest that Smad3 is mutationally inactivated in human cancer. However, certain strains of mice with a homozygous deletion of Smad3 develop aggressive metastatic colorectal cancer at an early age (Zhu et al., 1998). Further, loss of Smad3 protein has been reported recently in gastric tumors, possibly via the transcriptional repression of the Smad3 gene, and the re-introduction of Smad3 in gastric cell lines restored TGF-ß responsiveness and suppressed tumorigenicity in vivo (Han et al., 2004).
Smad7 is located on chromosome 18q21.1 (Roijer et al., 1998) and, as an inhibitor of TGF-ß signaling, is a putative oncogene. Reports implicating Smad7 in human cancer, however, are limited (Kleeff et al., 1999), but analysis of recent data indicates that Smad7 gene amplification is associated with a worse prognosis in patients with colorectal cancer (Boulay et al., 2003).
| (III) Abnormalities in Smad Co-activators and Co-repressors |
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| (IV) Ligand Expression and Activation |
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Classically, both alleles of a tumor-suppressor gene must be inactivated for a tumor to form. The TGF-ß pathway, however, does not appear to act in this on/off manner, and threshold effects are now known to be important in ligand-receptor interactions (Tang et al., 1998). This raises the possibility that TGF-ß1 levels might affect susceptibility to cancer in humans, and there is some evidence to support this proposal (Ziv et al., 2001). Further, it is now recognized that the effect of TGF-ß is context-dependent, and what is observed in one tumor type does not always apply to another. For example, studies to examine the function of TGF-ß in regulating tumor behavior in vivo have produced conflicting results. Using a variety of different strategies, including the transfection of tumor cells with sense or antisense TGF-ß expression constructs, investigators have demonstrated that TGF-ß1 has the capacity to promote (Steiner and Barrack, 1992; Huang et al., 1995; Park et al., 1997) or inhibit (Wu et al., 1993; Pierce et al., 1995) tumor development and/or progression. Furthermore, high levels of TGF-ß expression characterize carcinomas of the breast, colon, and pancreas (Dalal et al., 1993; Friess et al., 1993; Picon et al., 1998), whereas, in tumors of the integument, ligand expression is either decreased or remains unchanged (Schmid et al., 1996; Paterson et al., 2001).
An interesting hypothesis has recently been proposed which suggests that the mechanism by which TGF-ß is activated may influence whether the ligand acts to suppress or promote tumor progression (Dumont and Arteaga, 2002). Through activation of the latent TGF-ß complex, molecules such as thrombospondin and the integrins 
vß8 and vß5 have been linked with tumor suppression, while MMP 2 and MMP 9, the integrin vß6, and uPA/plasmin have been associated with tumor promotion. Clearly, these molecules are likely to be critical spatial and temporal determinants of the effects of TGF-ß on tumorigenesis. In future work, however, it will be essential to examine the expression of these molecules in the context of both the autocrine and paracrine effects of TGF-ß.
| (V) Epithelial-Mesenchymal Transition |
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TGF-ß-mediated EMT was first reported by Miettinen et al.(1994) in cultured murine epithelial cells, but the phenomenon has now been described in a broad spectrum of cell lines (Caulin et al., 1995; Oft et al., 1996; Piek et al., 1999; Gotzmann et al., 2002), including those of human origin (Geng et al., 1999; Janji et al., 1999; Zavadil et al., 2001; Yi et al., 2002). TGF-ß1 appears to induce EMT through autocrine mechanisms. TGF-ß1-mediated EMT, for example, is reversed in vitro and in vivo by the addition of dominant-negative TßRII cDNA in murine keratinocytes (Oft et al., 1998; Portella et al., 1998), and elevated levels of endogenous TGF-ß1 are thought to maintain the mesenchymal phenotype after the initial induction of EMT in MDCK and EpRas cells (Lehmann et al., 2000; Janda et al., 2002).
Significantly, TGF-ß1 requires a co-factor to induce EMT, and in the majority of cells studied, this is the presence of activated Ras or Raf (Oft et al., 1996; Lehmann et al., 2000; Janda et al., 2002). Current thinking suggests that Ras enhances the tumor-promoting effects of TGF-ß1 while at the same time attenuating its tumor-suppressor activities (Park et al., 2000; Yan et al., 2001). With the recognition that activated Ras is important in EMT, there has followed a plethora of studies that have examined the downstream targets of TGF-ß1 and Ras signaling and their involvement in EMT; a review of this work is outside the scope of this report but has been described in detail by Grunert et al.(2003). It is cautionary to note, however, that EMT appears to involve different signaling pathways in different cell types, that a variety of experimental conditions has been used in different studies, that experiments involving the use of dominant-negative constructs do not always completely abrogate protein expression, and that different workers have used various definitions of EMT (morphological change as opposed to scattering). Perhaps more importantly, however, is that while there is a large body of work regarding the pathways and mediators of EMT, the majority of evidence is derived from murine carcinoma cell lines, and very little has been published on studies wherein cells of human origin were used. The scientific community is necessarily aware of the differences between cells of rodent and human origin (Rangarajan and Weinberg, 2003).
(B) EVIDENCE FOR TUMOR PROMOTION
It has been argued that EMT is phenomenological only and unlikely to be an end-point of epithelial tumor progression in humans, not least because spindle cell tumors of the integument are extremely rare. Spindle cells, however, are found commonly at the invasive front of carcinomas, and it is widely held that this phenotype facilitates both tumor invasion and metastases (Gabbert et al., 1985). Support for the proposal that TGF-ß-induced EMT is important biologically has come from several sources. First, several studies have shown that transdifferentiated cells following TGF-ß-induced EMT are more motile and more invasive in vitro (Lehmann et al., 2000; Ellenrieder et al., 2001; Bakin et al., 2002; Yi et al., 2002). Second, cells that have undergone EMT are more tumorigenic and form less-differentiated tumors, with an elevated metastatic capacity following transplantation to athymic mice (Oft et al., 1998; Portella et al., 1998; Janda et al., 2002). And third, studies with cyclosporin have shown that the drug induces EMT and promotes tumor progression in a TGF-ß-dependent manner (Hojo et al., 1999). Interestingly, patients who have been treated with cyclosporin following organ transplantion appear to be susceptible to highly invasive squamous cell carcinomas of the skin (Marcil and Stern, 2001); in a clinical context, however, the potent immunosuppressive characteristics of cyclosporin cannot be excluded.
Indirect evidence to indicate that EMT has biological relevance is derived from studies of E-cadherin expression in malignancy. Cell lines with low levels of E-cadherin have increased invasive and metastatic capabilities (Frixen et al., 1991; Hoteiya et al., 1999), and in breast, gastric, bladder, and head and neck cancer, there is a clear correlation between decreased expression of E-cadherin and the more invasive/metastatic phenotype (Schipper et al., 1991; Oka et al., 1993; Wakatsuki et al., 1996). Recent studies have shown that E-cadherin expression is regulated by Snail, Slug, and SIP, and it is now known that over-expression of these transcription factors leads to down-regulation of E-cadherin, EMT, and increased invasion in vitro (Comijn et al., 2001; Bolos et al., 2002; Guaita et al., 2002; Yokoyama et al., 2003). Furthermore, Peinado et al.(2003) have recently showed that TGF-ß induces the Snail transcription factor in epithelial cell lines, resulting in repression of E-cadherin expression and the induction of EMT in vitro.
| (VI) Metastases |
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| (VII) Oral Cancer |
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(B) HUMAN ORAL CANCER
Along with others, we have been studying for some time the effects of TGF-ß in a series of malignant oral keratinocyte cell lines derived from human oral squamous cell carcinomas (SCC). Interestingly, the majority of these cells retain a full or partial response to the anti-proliferative effects of TGF-ß1 (Prime et al., 1994; Fahey et al., 1996; Malliri et al., 1996). Even in those lines that are not growth-inhibited by TGF-ß1, a restricted transcriptional response to the ligand is retained (Paterson et al., 1995, 2002). Further, despite the fact that p53 cooperates with Smad proteins to mediate certain TGF-ß signals (Cordenonsi et al., 2003), all of the human oral SCC lines that have been studied to date contain mutant p53, regardless of whether they are growth-inhibited or refractory to TGF-ß1. Experiments are currently in progress to determine the exact mechanism to account for why certain cell lines fail to respond to TGF-ß1, but one such mechanism is the failure to express Smad4 protein (Paterson et al., 2002). Intriguingly, over-expression of endogenous TGF-ß1 in Smad4-deficient cells leads to tumor suppression in vivo (Paterson et al., 2002). Analysis of our more recent data demonstrates that the tumor suppression in this context is not due to the inhibition of primary tumor formation but, rather, occurs as a result of tumor regression, possibly by the potentiation of mitochondria-regulated apoptosis (unpublished observations).
As the TGF-ß signal transduction pathways have become unraveled, genetic defects responsible for variations in TGF-ß responsiveness have been examined in oral carcinomas. Structural defects of TßRI (Chen et al., 2001; Knobloch et al., 2001) and TßRII (Garrigue-Antar et al., 1995; Wang et al., 1997), leading to a complete abrogation of TGF-ß signaling, have been reported, but such abnormalities have proved to be rare. The fact that most cell lines retain a ligand-induced transcriptional response suggests the occurrence of more subtle alterations in the majority of human oral cancers. During the transition from normality to malignancy and from carcinoma to metastases, TßR-II protein expression decreases significantly, suggesting that down-regulation of TßR-II, rather than gene mutations, is important in the pathogenesis of the disease (Paterson et al., 2001). To examine the functional significance of decreased TßR-II activity in oral cancer, we transfected dominant-negative TßR-II cDNA into a human malignant oral keratinocyte cell line. The results demonstrated reduction of TGF-ß-induced growth inhibition but retention of ligand-induced transcriptional responses. The partial inhibition of TßR-II signaling in these circumstances not only induced a metastatic phenotype in vivo, but also was associated with an enhanced growth rate, increased migration and invasion in vitro, and a loss of tumor cell differentiation (Huntley et al., 2004).
In contrast to carcinomas from glandular tissues (Dalal et al., 1993; Friess et al., 1993; Picon et al., 1998), the level of TGF-ß1 protein in oral cancer remains unchanged during the progression from normality to lymph node metastases (Paterson et al., 2001); other studies report increased TGF-ß1 expression in head and neck cancers (Pasini et al., 2001). Malignant human oral keratinocytes in vitro produce less TGF-ß1 than their normal counterparts, most probably due to adaptation to cell culture conditions (Fahey et al., 1996). Analysis of recent data indicates that while TGF-ß1 expression is not a useful biomarker of prognosis in patients with head and neck cancer (Logullo et al., 2003), it does act in an autocrine capacity to stimulate cell motility (Hasina et al., 1999).
Loss of heterozygosity at chromosome 18q has been reported frequently in head and neck squamous cell carcinoma (van Dyke et al., 1994; Frank et al., 1997; Jones et al., 1997), suggesting that defects in Smad2 and Smad4 would be a common finding. Data to verify this proposal, however, are limited and somewhat controversial. One immunohistochemical study has shown consistent expression of Smad2, Smad3, and Smad4 protein (Muro-Cacho et al., 2001), while others have demonstrated normal expression of Smad2 and Smad3 but loss of Smad4 (Yan et al., 2000). To complicate matters further, Muro-Cacho et al.(2001) demonstrated normal expression of Smad2 but defective Smad2 phosphorylation in tissue specimens, the significance of which remains unclear. Analysis of our own data shows that Smad2 and Smad3 mRNA and protein are expressed in 14 of 14 oral carcinoma cell lines, but in two lines, Smad4 mRNA expression is markedly reduced, and Smad4 protein is undetectable, which results in loss of TGF-ß-induced growth inhibition but retention of transcriptional responses (Paterson et al., 2002); transfection with wild-type Smad4 cDNA restores ligand-induced growth inhibition (unpublished observations). The mechanism of Smad4 loss in these two cell lines is currently under investigation, but it does not appear to be due to inactivating mutations in the coding sequence of the gene, and suggests the involvement of epigenetic events or promoter mutations.
Evidence is emerging to show that alterations in transcriptional regulators may also play a role in abrogating Smad signaling in head and neck cancer. A mutation in the p300 co-activator gene, for example, was recently described in a human oral carcinoma cell line, and transfection of the wild-type p300 restored TGF-ß-induced Smad-dependent transcriptional activation (Suganuma et al., 2002).
We have shown that TGF-ß1 induces EMT in human oral carcinoma cell lines (even in cells that are markedly growth-inhibited by the ligand), that the response is dependent on the presence of mutant Ras, and that the phenomenon involves Erk, PI3 kinase, and p38 (unpublished observations). Further, we have preliminary data to show that the AP-1 complex is involved in EMT, suggesting that the TGF-ß and Ras signaling pathways converge on AP-1 to drive transdifferentiation.
The biological consequences of TGF-ß1-induced EMT in oral cancer are unclear, but if it functions to promote tumor progression, investigators will have to be cognizant of the use of retinoids as a therapeutic modality. The effects of the synthetic retinoid N-(4-hydroxyphenyl)retinamide (4-HPR or Fenretinide), for example, which has been shown to be an effective chemopreventive agent in ongoing clinical trials of different cancers, including head and neck cancer (Oridate et al., 1996), appear to be mediated, albeit in part, by TGF-ß (Roberson et al., 1997; Herbert et al., 1999; Borger et al., 2000; La et al., 2003), which raises the possibility that Fenretinide may have dual effects, depending on the presence of oncogenic Ras. Significantly, Ras is rarely mutated in oral cancer of Western origin, but in Asia, abnormalities leading to activated Ras occur frequently (Paterson et al., 1996). It is conceivable, therefore, that the use of Fenretinide for the treatment of pre-malignant oral lesions in India and southeast Asia could have disastrous clinical consequences. Interestingly, a Phase III chemoprevention trial involving some 47,447 smokers treated with ß-carotene had to be stopped because of the increase in lung cancer and patient mortality (ATBC Cancer Prevention Study, 1994; Omenn et al., 1996); smoking-induced lung cancer is known to be associated with a high incidence of K-Ras mutations (Minamoto et al., 2000).
| (VIII) Concluding Remarks |
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As noted leaders in the field have stated, "The perceived role of TGF-ß in carcinogenesis has undergone more plot twists than an Agatha Christie mystery" (Roberts and Wakefield, 2003). It seems likely that TGF-ß will continue to intrigue and tantalize the scientific community for some years to come.
| Acknowledgments |
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