Cross-talk between MAPK cascades and other cellular regulatory pathways can extensively influence MAPK/ERK signaling by dynamic and complex interactions [4, 36].

Illustrating such phenomena, cross-talk between MAPK/ERK and PI3K/AKT/mTOR pathways at different stages of signal propagation can amplify key target regulatory protein activities through cross-activation and/or substrate convergence [4, 36]. MAPK/ERK regulates PI3K, TSC, and mTOR activity by activating PI3K and mTORC1 and inhibiting TSC2 [4, 36]. In this case, an important positive loop involves PI3K activation and GAB docking proteins phosphorylation. Once phosphorylated, GAB interferes in RAS-GAP complex binding, decreasing RAS inactivation and leading to positive ERK upstream regulation [36]. Moreover, ERK, RSK, AKT, and S6K protein kinases, and the components of MAPK/ERK and PI3K/AKT/mTOR pathways, often phosphorylate the same substrate including FOXO and c-Myc transcription factors [4, 36].

It is also known that the WNT/β-catenin signaling pathway interferes in MAPK/ERK regulation. The active GSK3β in the destruction complex (binding to β-catenin, APC, and AXIN) phosphorylates RAS, which is consequently degraded. Aberrant activation of the WNT/β-catenin pathway leads to excessive dissociation of destruction complex with consequent accumulation of β-catenin and RAS proteins in the cytoplasm. This promotes the β-catenin translocation to the nucleus and facilitates MAPK/ERK downstream activity by increasing RAS availability [37, 38]. In that case, mutual deregulation in MAPK/ERK and hyperactivation of WNT/B-catenin seems to cooperatively act triggering tumorigenesis [37, 38].

Interactions between epithelial and ectomesenchymal cells govern tooth development during odontogenesis. The molecular mechanisms associated with odontogenesis involve intracellular signaling cascades, including MAPK, Hedgehog, and Wnt pathways, and alterations in these pathways have been associated with the pathogenesis of odontogenic lesions [2, 3]. It is beyond the scope of this review to discuss the Hedgehog and Wnt pathways and the molecular pathogenesis of odontogenic lesions related to them. Thereby, we focused on the prototypical MAPK/ERK signaling pathway and the odontogenic tumors associated with its disturbance.

MAPK/ERK signaling plays a role in odontogenesis [39]. Unlike humans, mice are monophyodonts and have intrinsic differences from humans. However, mice dentition is a useful model to study the mechanisms related to human dental development [39, 40]. Supporting a role for MAPK/ERK signaling in odontogenesis, mice carrying deletions in Sprouty genes, which encode negative regulators of MAPK/ERK pathway, have hyperactive MAPK/ERK pathway signaling and supernumerary teeth [39, 41]. Similarly, ribosomal protein S6 kinase (RSK) mutant mice develop supernumerary teeth and alteration in dental shape patterns [39, 40]. RSKs are protein kinases that act downstream of the MAPK/ERK cascade and seem to have a feedback inhibitory effect on MAPK/ERK signaling [39, 40]. It is notable that the mutations in RSK2 cause Coffin-Lowry syndrome (OMIM #303600), in which dental anomalies can be present [40].

In addition, experimental data support the association of MAPK/ERK with odontogenic tumors tumorigenesis through RAS genes. Notably, Hras-G12V mutant mice show defects in the differentiation and proliferation of ameloblasts and their precursors [42, 43], while Hras transgenic mice develop jaw tumors consistent with odontogenic tumors [44–46]. Further supporting a role for MAPK/ERK signaling in odontogenesis, KRAS, RAF1, MEK1, and ERK1/2 protein expressions have been detected in human tooth germs by immunohistochemistry [47].

The fibroblast growth factor receptor 1 (FGFR1), which is a receptor whose stimulation activates MAPK/ERK pathway, has a strong expression in mouse odontoblasts, in addition to FGFR2 (isoform IIIb) in ameloblasts. This suggests that the fibroblast growth factors (FGFs) have a role in the regulation of their differentiation and secretory functions [48]. Moreover, the expression patterns of different FGFs in dental epithelium and mesenchyme are dynamic, supporting the existence of regulatory signaling cascades between FGFs in both these tissues during odontogenesis [49]. Another receptor whose stimulation activates MAPK/ERK pathway is the epidermal growth factor receptor (EGFR). There is consistent evidence that EGFR expression during odontogenesis has an important role during this developmental process [50].

Collectively, the above-mentioned studies support a role for MAPK/ERK signaling pathway in odontogenesis regulation, and disturbance in this pathway may lead to either odontogenesis impairment or can give rise to odontogenic tumors in animal models.

Ameloblastoma is a locally aggressive benign epithelial odontogenic tumor occurring mainly in the posterior mandible. Although benign, this tumor can behave aggressively and recur. Surgical approaches to remove this tumor often lead to facial deformity and morbidity [1]. Ameloblastomas are differently categorized into ameloblastoma (conventional), unicystic type, extraosseous/peripheral type, and metastasizing ameloblastoma, with distinct biological behaviors [1].

In 2014, the pioneer study by the group of Heikinheimo reported for the first time recurrent activating BRAF p.V600E mutations in ameloblastomas [9]. Considering that MAPK/ERK signaling can be activated by stimulation of transmembrane receptors, including EGFR, and that overexpression of EGFR had previously been reported in ameloblastomas, when the investigators detected ameloblastoma cultured cells resistant to EGFR-targeted inhibition they screened these cells for BRAF p.V600E mutation [9]. After detecting the mutation in this index case, the study of Kurppa et al. (2014) detected BRAF p.V600E mutation in 62.5% (15/24) of ameloblastoma samples through Sanger sequencing [9]. In addition, the study of these authors demonstrated the utility of the BRAF p.V600E-specific monoclonal antibody VE1 to detect the BRAF p.V600E mutation in ameloblastomas by immunohistochemistry [9].

The study of Sweeney et al. carried out targeted next-generation sequencing (NGS) and/or Sanger sequencing and VE1 immunohistochemistry where they detected BRAF p.V600E mutation in 43% (12/28) of ameloblastoma samples [51]. Additionally, they detected another BRAF variant (p.L597R) in one sample [51]. The study of Brown et al. performed a combination of allele-specific PCR, NGS gene panel, and Sanger sequencing and showed BRAF p.V600E in 62% (31/50) of ameloblastoma cases [52]. They further reported the presence of BRAF p.V600E mutation in 67% (23/34) of ameloblastomas by using VE1 immunohistochemistry in cases not suitable for molecular evaluation [52]. Following these pieces of research, several studies have also assessed the presence of BRAF p.V600E in conventional ameloblastoma, either by molecular techniques or a combination of mutation screening and immunohistochemistry, with mutation frequencies varying from 55 to ~90% [10, 53–63]. In two studies with limited sample numbers, the mutation was detected in all samples [2/2 [64] and 4/4 [65]]. The frequency of BRAF p.V600E mutation in studies that have assessed the mutation only using immunohistochemistry varied from 33 to 79% [66–71]. Notably, although immunohistochemical expression of BRAF p.V600E has been used as a surrogate of BRAF p.V600E mutation, results must be interpreted with caution since there are false-positive cases detected by immunohistochemistry and not confirmed by molecular technique [73] as well as false-negative cases [63].

There is no consensus on the association of BRAF p.V600E mutation with ameloblastoma clinicopathological features, including location, age, histology, as well as clinical behavior. In the studies conducted by Sweeney et al. and Gültekin et al., they suggested the predominance of BRAF p.V600E ameloblastomas in mandible when compared to BRAF wild-type tumors [51, 55]. The studies of Brown et al., Bonacina et al., and Kelppe et al. have also suggested BRAF p.V600E positive cases mostly locate in the mandible and occur at earlier ages [52, 62, 69]. In agreement with that, the study of Gültekin et al. has also reported that BRAF p.V600E ameloblastoma cases occur at a much younger age than BRAF p.V600E wild-type ones [55]. Additionally, BRAF mutations have been reported by some authors to predominantly occur in non-plexiform histologic type ameloblastoma [51, 55, 71], while conversely others reported BRAF mutations predominance in plexiform type [67]. It is worth mentioning that in this last study [67], the authors have assessed the mutation using immunohistochemistry as a surrogate marker for the mutation. However, they used a different antibody clone other than VE1. Nonetheless, most studies reported recurrent BRAF p.V600E mutation regardless of histological type [9, 10, 56, 60, 66], mandibular/maxillary location [10, 56, 66], and the age of patients [9].

The association between the presence of BRAF p.V600E and ameloblastoma aggressiveness is unclear. While some studies had reported earlier recurrence and increased recurrence rates in BRAF wild-type tumors [52, 55, 58], others had observed a more aggressive behavior with poor disease-free survival and higher recurrence rate in ameloblastomas harboring BRAF p.V600E mutation; in these cases, assessed by immunohistochemistry only [66, 67]. In recent times, no difference has been found in relapse-free intervals between BRAF p.V600E positive and wild-type ameloblastoma cases [62].

Mutations in 28 genes have been assessed by an NGS targeted panel, in addition to smoothened frizzled class receptor (SMO) mutations, assessed by Sanger sequencing [55]. Mutations have been detected in approximately 90% of the ameloblastomas, comprised of conventional, unicystic, and peripheral cases, with BRAF p. V600E corresponding to 60% of mutation-positive cases [55]. SMO mutations have been detected in 14% of cases, in a mutually exclusive pattern with BRAF mutations. Additionally, NRAS, HRAS, and EGFR somatic mutations have been detected in one case each, mutually exclusive with BRAF and SMO mutations. In a few cases, BRAF or SMO mutations co-occurred with mutations in other genes. Importantly, the authors reported high recurrence rate in ameloblastomas harboring multiple gene mutations (higher mutational burden) detected either by targeted NGS or Sanger sequencing. At the same time, a low risk for relapse was observed in tumors with a single BRAF mutation [55]. It is notable that the presence of two or three gene mutations, including somatic mutations in KRAS, PIK3CA, PTEN, FGFR, CDKN2A, and CTNNB1 in the background of either BRAF or SMO mutation-positive ameloblastomas, exclusively occurred in solid/conventional tumors [55]. Further studies may help to clarify if these associations between tumor mutation burden and aggressiveness hold.

The study of Diniz and co-workers in 2015 tested whether the BRAF p.V600E mutation was a signature of conventional ameloblastoma or if unicystic lesions also harbored this mutation. BRAF p.V600E was detected in 83% (5/6) of unicystic ameloblastomas [10]. In the later study of Heikinheimo et al., they reported BRAF p.V600E mutation in 94% (29/31) of mandibular unicystic ameloblastomas and higher homogeneity of mutations than that of conventional ameloblastomas, since rare samples carried a mutation other than BRAF [58]. The mutational screening of BRAF by molecular assays has been shown to be useful for the differential diagnosis between unicystic ameloblastomas and odontogenic cysts [64, 73]. Furthermore, a consistent homogeneous profile for BRAF mutational status has been shown in unicystic ameloblastomas, with BRAF p.V600E detection by allele-specific qPCR in all areas with different histological appearances from the same neoplasm, including those areas resembling other odontogenic lesions [64]. Other studies that reported BRAF p.V600E mutation in the unicystic variant by molecular screening and/or immunohistochemistry are listed in Table 1.

A small number of studies have assessed genetic mutations in peripheral ameloblastomas [54, 55, 62, 69, 71]. The BRAF p.V600E was also the most common mutation among them, and it was detected in 62.5% (10/16) of cases [54, 55, 62, 69, 71]. Additionally, single somatic mutations in NRAS [54] and SMO [55] have also been detected in one peripheral ameloblastoma sample each in a mutually exclusive manner with the BRAF mutation.

Mutually exclusive and less common mutations affecting other MAPK-related genes, such as KRAS, NRAS, HRAS, and FGFR2 (a receptor whose stimulation activates MAPK/ERK pathway) have been reported in BRAF wild-type ameloblastomas [51, 52, 54, 55, 58, 62, 72]. It is notable that the KRAS p.G12R mutation, which occurs in adenomatoid odontogenic tumors [12], has been reported in 4/50 (8%) [52] and 4/28 (14%) [51] of BRAF wild-type ameloblastoma cases. Furthermore, in addition to the above-mentioned mutations in MAPK pathway genes, somatic EGFR mutation has been detected in one single case of maxillary ameloblastoma [55]. Mutations in FGFR2 have been described in 4/28 (14%) [51], 3/50 (6%) [53], and 2/39 (5%) [58] of BRAF wild-type conventional ameloblastomas. The study of Bartels et al. assessed BRAF wild-type ameloblastomas by targeted NGS and identified FGFR2 mutations in 4/7 (57%) of them, including one FGFR2/TP53/PTEN-triple-mutant case [72]. Additionally, increased proliferation through MAPK/ERK activation of ameloblastomas cultured cells has been shown after treatment with FGF ligands [77], reinforcing the role of FGF signaling in the tumorigenesis of ameloblastomas.

Other cancer-associated mutations not directly involved in the MAPK pathway have also been detected in ameloblastomas [51, 52, 54, 55, 57, 58, 72, 78]. Among them, SMO mutations have been detected in between 13 and 39% of ameloblastomas, occurring in a mutually exclusive pattern with BRAF p.V600E [51, 52, 55]. SMO mutations often occur along with an additional RAS family or FGFR2 mutation [51, 52, 55]. Interestingly, the study of Sweeney et al. proposed site-specific BRAF and SMO mutations in mandible and maxilla, respectively [51]. This finding was later supported by the study of Gültekin et al. in a larger cohort [55]. However, the site-specificity of these mutations has not been confirmed by other groups [10, 58]. Aside from the SMO mutations, APC mutations have been detected in 3/6 ameloblastomas [78], and CTNNB1, PIK3CA, SMARCB1, PTEN, CDKN2A mutations have been reported in a few cases and tend to occur in a non-mutually exclusive manner with BRAF p.V600E mutation and with each other [52, 54, 55]. Protein products of some of these genes, e.g., APC, β -catenin encoded by CTNNB1, and PI3K encoded by PI3KCA, are components of pathways that cross-talk with MAPK/ERK, as discussed in the “MAPK/ERK signaling pathway cross-talk” topic.

Recently, two studies performed whole-exome sequencing to assess coding mutations in ameloblastomas and reported uncommon mutations in several other genes occurring in the background of BRAF p.V600E mutation [57, 65]. The study of Guan et al. reported BRAF p.V600E mutation in 82% (9/11) of samples and proposed intratumor heterogeneity in ameloblastomas based on different variant allele frequencies (VAF) of BRAF p.V600E and other detected mutations [57]. Mutations in the CDC73 gene, which encodes parafibromin, have been detected in 2/11 samples [57]. It is worth mentioning that CDC73 germline mutation causes hyperparathyroidism-jaw tumor syndrome (OMIM #145001), in which ossifying fibromas may occur. The study of Shi et al. suggested a “two-hits” mechanism contributing to ameloblastoma tumorigenesis, with BRAF p.V600E (detected in all four assessed samples) corresponding to the first hit and mutations in genes belonging to the gene network of cell proliferation, such as HSAP4, corresponding to the second hit [65]. However, further investigations in larger cohorts and using other methodologies for evaluating tumor clonality and the role of the detected mutations in ameloblastoma development, if any, are needed to confirm these findings. Currently, the evidence is still insufficient to draw any conclusions about further mutations other than BRAF p.V600E participating as drivers of ameloblastoma pathogenesis.

The BRAF p.V600E mutations have been reported in benign mixed odontogenic tumors [13, 52, 53, 63], namely ameloblastic fibroma [13, 52, 53, 63], ameloblastic fibrodentinoma [13, 52], and ameloblastic fibro-odontoma [13, 53, 63].

Collectively, these studies reported BRAF p.V600E mutations in 45.8% (11/24) of ameloblastic fibromas [13, 52, 53, 63], 60% (3/5) of ameloblastic fibrodentinomas [13, 52], and 34.6% (9/26) of ameloblastic fibro-odontomas [13, 53, 63], whereas all nine odontoma samples investigated were wild-type for BRAF p.V600E [13, 63]. These results suggested that at least a subset of ameloblastic fibromas, ameloblastic fibrodentinomas, and ameloblastic fibro-odontomas are pathologic entities distinct from odontomas. However, this subject is still debatable.

It was suggested that the BRAF p.V600E mutation was limited to the epithelial component of the four mutant cases of mixed tumors which had the two components tested separately, i.e., 1/1 mutant ameloblastic fibroma and 3/3 mutant ameloblastic fibro-odontomas [53]. However, our group has recently dealt with this issue using a straightforward methodology. We have subjected mixed odontogenic tumor samples to laser capture microdissection before molecular testing in an attempt to avoid epithelial-mesenchymal cross-contamination and using allele-specific quantitative PCR, a high sensitivity mutation detection assay, we detected the BRAF p.V600E mutation in the mesenchymal component of all mutation-positive mixed odontogenic tumors (9/9) [13]. Notwithstanding, BRAF p.V600E positive status was additionally detected in the epithelial components in two cases, which are one ameloblastic fibroma and one ameloblastic fibro-odontoma [13]. While this positivity in the epithelial and mesenchymal components of these two samples may have occurred due to cross-contamination and detected using a high-sensitivity molecular technique, it may also represent the true mixed nature of such lesions.

The molecular pathogenesis of odontogenic sarcomas, namely ameloblastic fibrosarcoma, has been explored recently [13, 75]. The BRAF p.V600E mutation has been detected in 71% (5/7) [75] and 67% (2/3) [13] of cases. Consistent with the histopathologic features of the ameloblastic fibrosarcoma, in which malignancy is restricted to the mesenchymal component, the BRAF p.V600E mutation was restricted to the sarcomatous areas of the two mutant ameloblastic fibrosarcoma cases tested in our cohort [13]. The mutation was further detected in the benign mesenchymal component of the ameloblastic fibroma-like area in one of the ameloblastic fibrossarcoma positive cases [13]. This finding reinforces the malignant transformation from a previous ameloblastic fibroma in some cases [13]. In addition to BRAF mutations, NRAS p.Q61K has been detected in a BRAF wild-type ameloblastic fibrosarcoma sample [75].

Although the rarity of this tumor precludes extensive knowledge about its molecular pathology, the current results could support the role of the MAPK/ERK pathway in its pathogenesis and pave the way for further investigation on targeted therapy.

Ameloblastic carcinomas, the malignant counterpart of ameloblastomas, also harbor BRAF p.V600E mutations, but with reported frequencies varying from 25 to 40% [10, 53, 63]. Such frequencies are lower than those reported for the same mutations for ameloblastomas (64% in conventional, 81% in unicystic, and 63% in peripheral), as shown in Table 1. It is worth noting that the lower frequency of BRAF p.V600E mutation in ameloblastic carcinomas compared with ameloblastomas is similar to what is observed in other benign tumors and their malignant counterparts [6]. For instance, BRAF p.V600E mutation is detected in approximately 80% of benign melanocytic nevi, 60% of dysplastic nevi, and only in 40–45% of melanomas, suggesting that the functional effects of the mutation are context-dependent [6]. Additionally, oncogene-induced senescence may limit the proliferation status of nevi in the tumorigenic process [79]. However, BRAF p.V600E mutation has been recently reported in 5/5 ameloblastic carcinoma cases submitted to molecular screening [76]. These results could encourage targeted therapy as a new direction in the future.

Mutations in other genes which are not related to MAPK/ERK, such as TP53, CTNNB1, and APC, have also been reported in ameloblastic carcinomas [72, 78, 80]. The detection of TP53 mutation in the malignant area of a tumor arising from preexisting ameloblastoma [80] and observation of TP53 and CTNNB1 in a BRAF p.V600E wild-type ameloblastic carcinoma [72] suggest that mutations in these genes might play a role in the malignant transformation process of ameloblastomas.

Odontogenic carcinoma with dentinoid, which is an odontogenic carcinoma that has not yet been fully recognized as a unique entity, has also been shown to harbor pathogenic mutation in CTNNB1 and APC [81]. Although these genes are not part of the MAPK/ERK pathway, they belong to WNT/β-catenin, which is well known to cross-talk with MAPK/ERK. Inactivating APC mutation and CTNNB1 activating mutation leads to strong and aberrant cellular β-catenin accumulation [37, 38, 78, 81], and such phenomena have been observed in some odontogenic epithelial tumors, including ameloblastoma and odontogenic carcinoma [78, 81].

Clear cell odontogenic carcinoma has also been shown to harbor BRAF p.V600E [10]. However, since a single sample was screened, future studies including a larger cohort of samples may clarify if such mutations are frequent in this tumor.

An adenomatoid odontogenic tumor is a benign epithelial odontogenic tumor predominantly affecting the maxilla. It is often encapsulated and has an indolent clinical behavior [1, 82]. Adenomatoid odontogenic tumors most often occur sporadically. However, multiple adenomatoid odontogenic tumors can occur in patients with Schimmelpenning syndrome (OMIM#163200) [83, 84]. This syndrome is caused by postzygotic mutations in RAS genes [85]. Based on that knowledge, we screened an adenomatoid odontogenic tumor sample from a Schimmelpenning syndrome patient as well as two sporadic cases for mutations in a NGS panel comprising 50 tumor suppressor genes and oncogenes, including RAS family genes, by using Ion AmpliSeq^TM Cancer Hotspot Panel v2 (Life Technologies, Carlsbad, USA). The KRAS c.35G > T mutation leading to p.G12V was detected in all three samples, and it was further interrogated in additional samples. The mutation was detected in 78% (7/9) of tumors evaluated [11].

Following the aforementioned study, we assessed KRAS codon 12 mutations by allele-specific qPCR and screened codons 12, 13, and 61 by Sanger sequencing in a larger cohort of samples. We detected recurrent KRAS p.G12V (n = 15/38) or p.G12R mutations (n = 12/38) in 27 out of 38 adenomatoid odontogenic tumors (71%) regardless of the age of the patient, tumor size, tumor location, follicular or extrafollicular variants, and fibrous capsule thickness [12]. Confirming our findings, the study of Bologna-Molina et al. also reported KRAS codon 12 mutations in 78% (7/9) of cases, with either p.G12V (n = 2/9) or p.G12R (n = 4/9) mutations reported in 6/9 samples and p.G12D in a single case (1/9) [74].

Further than investigating point mutations, we have also investigated the copy-neutral loss of heterozygosity (cnLOH), as well as copy number alterations (CNAs) in a sporadic adenomatoid odontogenic tumor and a sample from a Schimmelpenning syndrome patient [11]. The sporadic tumor showed two rare CNAs, being one at 6p15 and the other at 7p15.3, covering the IGF2BP3 gene, while the tumor from the syndromic patient only harbored common gains and losses [11]. The deletion only encompasses an intronic portion of the gene, and the significance of these findings in the context of tumorigenesis is unclear.

While the BRAF p.V600E mutation emerged as a molecular signature for ameloblastomas and has also been shown to be frequent in other tumors with ameloblastic differentiation, KRAS codon 12 mutations seem to be a marker of adenomatoid odontogenic tumors [11, 12, 74]. Even tumors wild-type for KRAS showed MAPK/ERK pathway activation, demonstrated by the immunoexpression of the surrogate marker ERK1/2 phosphorylated form [12]. Therefore, whole-exome sequencing of the KRAS wild-type cases may provide information on the genetic signatures of the remaining 30% of cases for which KRAS mutations have not been detected.