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Metastasizing Maxillary Ameloblastoma: Report of a Case with Molecular Characterization J Oral Maxillofac Res 2016;7(1):e5 doi:10.5037/jomr.2016.7105 |
Metastasizing Maxillary Ameloblastoma: Report of a Case with Molecular Characterization
1Department of Surgery and Translational Medicine, Section of Anatomic Pathology, University of Florence, Italy.
2Second Otolaryngology Head and Neck Surgery Clinic, Azienda Ospedaliera Universitaria Careggi, Florence, Italy.
Corresponding Author:
Department of Surgery and Translational Medicine
University of Florence
Largo Brambilla 3, 50134, Firenze
Italy
Phone: +39 055 4478102
Fax: +39 055 4379868
E-mail: franchi@unifi.it
ABSTRACT
Background: Ameloblastoma is a benign odontogenic tumour that may exhibit aggressive biological behaviour with local recurrence and metastasis following initial surgical resection. Surgery is the most acceptable modality of treatment, even if a biological approach is currently on study. We report a case of maxillary ameloblastoma with development of neck and brain metastases after repeated local recurrences. Molecular analysis was performed with the aim to better characterize this neoplasm and its peculiar behaviour.
Methods: We investigated the status of tumour protein p53 (TP53), epidermal growth factor receptor (EGFR), B-Raf proto-oncogene (BRAF) and human epidermal growth factor receptor 2 (HER2) genes with immunohistochemical, fluorescent in situ hybridization and/or direct sequencing in order to clarify their possible role in the development of this neoplasm and the possibility of a targeted treatment.
Results: The histological appearance of the tumour was the same in the primary lesion, in the recurrence and in the metastases. EGFR positivity was present in the recurrence and the brain metastasis, while HER2 was negative in all samples tested. Fluorescent in situ hybridization analysis for EGFR showed disomy of neoplastic cells. Direct DNA sequencing of TP53 gene exons 5 - 9 was carried out in tumour samples from the infratemporal recurrence and brain metastasis, with no mutational alteration detected. Similarly, sequencing analysis of BRAF exon 15 (V600) and EGFR gene showed wild type results in all samples tested.
Conclusions: Further studies are needed to identify molecular pathways that may provide an opportunity of alternative treatments and/or new potential predictive markers of local and distant spread of this rare tumour.
J Oral Maxillofac Res 2016;7(1):e5
doi: 10.5037/jomr.2016.7105
Accepted for publication: 29 March 2016
Keywords: ameloblastoma; human EGFR protein; human HER2 protein; metastasis; tumor suppressor protein p53.
INTRODUCTION
Ameloblastoma is a rare tumour of odontogenic epithelial origin, which accounts for approximately 1% of all mandibular tumours and cysts [1-2]. It has high propensity for local recurrence if not adequately removed and although the tumour may appear microscopically benign, the development of distant metastasis is possible. Classification as a benign or malignant lesion has generated much debate because ameloblastoma has different histopathologic patterns and displays a wide spectrum of biologic behaviours. In the WHO classification, a clear distinction between ameloblastoma, metastasizing ameloblastoma and ameloblastic carcinoma was made. Here, metastasizing ameloblastoma is defined as an ameloblastoma that metastasize in spite of a benign histology [3]. This occurrence is estimated in approximately 2% of the cases [4], and the most common site for metastasis is the lung (75 - 80%) [5], followed by the cervical lymph nodes, the diaphragm, the liver and the brain. On the other hand, ameloblastic carcinoma shows combined histologic features of ameloblastoma with cytologic atypia, regardless of the presence of metastasis [6]. This report describes a patient who presented a long history of local recurrence and distant metastasis of ameloblastoma. Molecular analysis was performed with the aim to better characterize this neoplasm and its peculiar behaviour.
CASE DESCRIPTION AND RESULTS
A 29-year-old male presented a swelling of the oral cavity without any symptoms. The radiographic examination showed diffuse opacity of the right nasal fossa and maxillary sinus, with destruction of the medial and inferior walls of the maxillary sinus, and thinning of the pavement of the orbita (Figure 1A). He underwent extended right maxillectomy with resection of a portion of the hard palate with a histologic diagnosis of ameloblastoma. In the following years, his medical history was significant for an adenocarcinoma of the colon and an acute myocardial infarction. After a disease-free interval of 20 years, the tumour recurred locally in the right maxillary sinus (Figure 1B), and the diagnosis of ameloblastoma was confirmed histologically. One year later a computed tomography highlighted a recurrence involving the right orbita (Figure 1C) and the hard palate (Figure 1D). The patient underwent hemifacial resection with orbital exenteration. After 10 months, twenty-seven years after the onset of the primary lesion, the patient referred frontal headache, postural instability, disorientation and bewilderment with impaired short-term memory. magnetic resonance imaging revealed a recurrence in the infratemporal fossa (Figure 1E) and a single metastasis in the right temporal area of the brain (Figure 1F). These were surgically removed, and the sphenoidal-orbital region and the right temporal lobe were also treated with radiation therapy (60 Gray total dose). Nine months later the patient developed a further metastatic deposit in the right neck, which was surgically removed. The patient is currently alive with disease localized in the brain.
Figure 1 |
Histopathology
The histological appearance of the tumour was the same in the primary lesion, in the recurrence and in the metastases. The tumour mainly presented a plexiform pattern, characterized by a proliferation of basal cells organized in anastomosing strands with an inconspicuous stellate reticulum (Figure 2). The basal cells were columnar and hyperchromatic, with nuclei displaced away from the basement membrane. In the primary lesion, focal areas of the tumour displayed cystic changes (Figure 2). There were no cytologic atypia, mitotic activity and areas of necrosis in any of the specimens.
Figure 2 |
Immunohistochemistry
The results of the immunohistochemical stainings are illustrated in Figure 3. Staining for epidermal growth factor receptor (EGFR) conducted on the infratemporal recurrence and on the brain metastasis, showed strong membrane and cytoplasmic positivity of neoplastic cells. Tumour protein p53 (TP53) nuclear immunostaining was detected in the majority of neoplastic cells. Conversely, human epidermal growth factor receptor 2 (HER2) was negative in all samples tested.
Figure 3 |
Fluorescent in situ hybridization (FISH) analysis
The analysis was conducted on the infratemporal recurrence. Neoplastic cells showed disomy, with an average ratio of EGFR gene to chromosome 7 centromere signals (CEP7) signals per cell of 0.8.
Molecular studies
Direct DNA sequencing of TP53 gene exons 5 - 9 was carried out in tumour samples from the infratemporal recurrence and brain metastasis, with no mutational alteration detected. Similarly, sequencing analysis of B-Raf proto-oncogene (BRAF) exon 15 (V600) and EGFR showed wild type results in all samples tested.
DISCUSSION
According to the current WHO classification, metastasizingameloblastoma shows the same histological features of non-metastasizing ameloblastoma, and therefore the diagnosis can be made only retrospectively, when metastasis has occurred [5]. Thus, it is difficult to predict the behaviour of this neoplasm, which has always an uncertain malignant potential. Generally accepted risk factors for the development of metastasis include large primary lesion, late diagnosis of the initial tumour, multiple local recurrences, inadequate surgical treatment, radio-chemotherapy treatment and plexiform pattern [7], even if the exact nature and the role played by each factor is not clear [8]. In addition, long-term follow-up is recommended [2], because metastasis may occur after a very long disease-free interval, which may be up to 42 years after the treatment of the primary lesion [7], with an average time to metastasis of 18 years [9]. Indeed, in the present case the first recurrence occurred 20 years after the primary lesion, and 7 years later two metastases were detected. However, according to Van Dam et al. [9], in the absence of malignant cytologic transformation of the metastatic lesion, the clinical course of the metastatic tumour is relatively indolent, with an average survival of 10 years after the diagnosis of metastasis.
In the recent past, several studies attempted to elucidate the complex aspects of ameloblastoma biology, in order to improve treatment and outcome of the patients. Currently, radical surgery is the elective therapy both for primary and secondary lesions. In addition, patients must be followed strictly with instrumental exams and punctual follow-up to prevent recurrence [1]. Radiotherapy and chemotherapy are reserved for the palliative setting and inoperable tumours [10].
Recently, several molecular studies have been undertaken in order to improve our understanding of the pathogenesis of this neoplasm, and to identify possible targets for alternative treatments, to potentially reduce the need for extensive and repeated surgery. The status of different genes has been evaluated, including transmembrane tyrosine kinase EGFR, BRAF, HER2 and TP53.
Epidermal growth factor and EGFR participate in the differentiation of ameloblasts and in the control of their cellular function [11]. EGFR regulates the proliferation of both normal and neoplastic cells, it is expressed by normal odontogenic epithelium and the presence of alterations of this gene has been investigated both with immunohistochemical [11-13] and molecular analysis [14].
Immunohistochemical studies have shown positivity for EGFR both in primary lesions and in metastases, although this marker did not predict recurrence [15]. In agreement, in the present case we observed EGFR cytoplasmic and membranous immunostaining in both the recurrence and the brain metastasis. In the molecular study performed by Kurppa et al. [14], an over-expression of EGFR was observed in ameloblastomas studied with real-time reverse transcription polymerase chain reaction (RT-PCR), while in the present case, FISH analysis did not demonstrate gene amplification. Moreover, gene sequencing did not identify any activating mutation of the EGFR gene. Therefore, data from literature indicate that anti-EGFR targeted therapy could be potentially used in the treatment of recurrent disease, especially in cases where the surgical approach is limited [15]. Indeed, as reported by Vered et al. [11], EGFR treatment is recommended in aggressive ameloblastomas not only in monotherapy, but also in combination with conventional radiotherapy. The administration of anti-EGFR agents could be also intralesional, to avoid the adverse events of the treatment. Recently, new anti-EGFR monoclonal antibodies were developed, and the target therapy with these drugs showed clinically successful results, underlying the possibility to control the disease also in advanced cases [11].
BRAF is a potent activator of the mitogen activated protein kinase (MAPK) cascade, which in turn phosphorylate and activate extracellular signal-regulated kinases 1 and 2 (ERK1/ERK2) [16,17]. ERK regulates the expression of several genes through the phosphorylation of nuclear transcription factors or by targeting other intracellular signalling molecules. Thus, through the stimulation of ERK signalling, BRAF is capable to induce proliferation and to promote transformation. More than 40 different mutations are identified in BRAF gene human cancer [18]. Ninety percent of B-RAF mutations are represented by a missense mutation at residue 600 that substitutes a glutamine with a valine (V600E), resulting in constitutively activation of the gene. In a study of BRAF V600E mutation in 24 ameloblastomas [14], 15 tumours (63%) resulted positive for the mutation, without significant association with specific ethnicity, sex or age of the patients, or tumour histology. This mutation has been associated with resistance to EGFR-targeted drugs in primary ameloblastoma cells, similar to what happens in colorectal cancer.
HER2, also known as c-erb or HER2/neu, is a human epidermal growth factor receptor belonging to the same family of EGFR and its protein overexpression has been found in several carcinomas [19]. Previous studies showed that immunoreactivity for HER2 in ameloblastoma is significantly lower than in normal dental follicles [15,19] and, albeit with some differences, all variants of ameloblastoma resulted negative or weakly positive for HER2. This is in agreement with the present case, which showed no immunohistochemical expression of HER2 protein, neither in the primary or metastatic lesions.
TP53 suppressor gene is situated on chromosome 17p13 and is one of the most frequently altered genes in tumours [20]. Mutation or loss of heterozygosity in the p53 gene or accumulation of its protein is associated with increased cellular proliferation and malignant transformation [21]. Ameloblastoma shows variable reactivity to p53 depending on the histological types, with plexiform variant being more frequently positive than follicular variant [15,20]. In our study, direct sequencing of TP53 did not show any alteration of the gene, while immunohistochemistry showed positive nuclear staining of neoplastic cells. This is in agreement with the results of the study by Kumamoto et al. [20], who observed no TP53 gene alteration in a series of 11 ameloblastomas, including a metastasizing example. However, these Authors found a higher expression of p53, MDM2 and p14ARF in benign and malignant ameloblastomas than in tooth germs, supporting the hypothesis that these factors may be involved in the malignant transformation of odontogenic epithelium, while TP53 gene mutation is likely to play a minor role.
CONCLUSIONS
We report a case of ameloblastoma with metastatic spread to the brain and the neck after repeated local recurrences. Further studies are needed to identify molecular pathways that may provide an opportunity of alternative treatments and/or new potential predictive markers of local and distant spread of this rare tumour.
ACKNOWLEDGMENTS AND DISCLOSURE STATEMENTS
The authors report no conflicts of interest related to this study.
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To cite this article: Metastasizing Maxillary Ameloblastoma: Report of a Case with Molecular Characterization J Oral Maxillofac Res 2016;7(1):e5 URL: http://www.ejomr.org/JOMR/archives/2016/1/e5/v7n1e5ht.htm |
Received: 4 February 2015 | Accepted: 29 March 2016 | Published: 31 March 2016
Copyright: © The Author(s). Published by JOMR under CC BY-NC-ND 3.0 licence, 2016.