STAT3 gene expression in ameloblastomas and odontogenic keratocysts

Author:

de Araújo1,Andrade de2,Schlaepfer Sales3,Carneiro Braúlio4,Martins Marília Trierveiler5,Freitas Valéria6,Aquino Xavier1,Cury Patrícia2,Gurgel Clarissa2,dos Santos7

Affiliation:

1. Federal University of Bahia, School of Dentistry, Laboratory of Surgical Pathology, Salvador, Bahia, Brazil

2. Federal University of Bahia, Program Dentistry and Health, Salvador, Bahia, Brazil

3. Federal University of Bahia, Department of Biomorphology, Salvador, Bahia, Brazil

4. South University of Bahia, Department of Oral and Maxillofacial Surgery, Jequié, Bahia, Brazil

5. University of São Paulo, Department of Oral and Maxillofacial Pathology, São Paulo, São Paulo, Brazil

6. State University of Feira de Santana, Department of Health, Feira de Santana, Bahia, Brazil

7. Federal University of Bahia, School of Dentistry, Laboratory of Surgical Pathology, Salvador, Bahia, Brazil + Federal University of Bahia, Program Dentistry and Health, Salvador, Bahia, Brazil

Abstract

Introduction/Objective. STAT3 (signal transducers and activators of transcription) is involved in different physiological processes, including cell proliferation and survival. High expression of this protein is observed in various types of cancer. This study aimed to investigate the gene and protein expression of STAT3 in a series of odontogenic cysts and tumors to provide more information about their biological profile. Methods. The STAT3 gene expression at mRNA was quantified by real-time quantitative polymerase chain reaction (RT-qPCR) in 23 odontogenic keratocysts (OKCs) and seven ameloblastomas (AMs), and compared to the non-neoplastic oral mucosa. We also assessed the expression of STAT3 gene at protein levels, using immunohistochemistry, in 43 OKCs and 47 AMs. Results. STAT3 transcripts were found in 96.6% of the tumors studied; however, the gene was downregulated in OKC and AM compared to the non-neoplastic oral mucosa. The STAT3 gene expression at mRNA level was higher in sporadic OKC than in syndromic OKC (p = 0.04). There was no difference in STAT3 gene expression at mRNA level between OKCs and AMs (p = 0.88). Immunostaining of STAT3 revealed no significant difference between sporadic and syndrome OKC (p > 0.05), nor between conventional and unicystic AMs (p > 0.05). Ameloblastomas exhibited significantly higher STAT3 immunostaining than OKCs (p = 0.03). In OKC and AM, STAT3 immunostaining was predominantly cytoplasmic and no difference in the cellular localization of STAT3 was observed between these lesions (p = 0.58). Conclusion. Our findings showed low expression of STAT3 gene in OKCs and AMs in relation to nonneoplastic oral mucosa. However, higher STAT3 immunostaining was observed in AMs compared to OKCs.

Publisher

National Library of Serbia

Subject

General Medicine

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