The expression and role of Migration Stimulating Factor (MSF) in oral tumours

Aljorani, Lateef Essa

January 2012

Migration Stimulating Factor (MSF) is an oncofoetal protein which is constitutively produced by both epithelial and stromal cells during foetal development, not expressed by the majority of their normal adult counterparts, but re-expressed during pathological processes such as cancer and wound healing. Scotland has the highest occurrence of oral cancers in the UK; the incidence is still increasing, but patient survival remains very poor. The expression of MSF in oral tumours has not been previously reported. The aims of this study were: • To determine the effects of MSF on the migration of oral tumour cell lines and normal stromal cells in culture (chapter 3), • To ascertain the possible presence, diagnostic and prognostic value of MSF in oral squamous cell carcinoma (OSCC; chapter 4), and salivary gland tumours (SGT; chapter 5). • To identify the putative MSF receptors in oral tumour cell lines (chapter 6). For tissue culture studies, the effects of rhMSF (wild type and mutant proteins) were examined on human cell lines TYS, HSG, Endo 742 and FSF44. These cells were derived from OSCC, SGT, microvascular endothelial cells and skin fibroblasts, respectively. For ex-vivo studies, paraffin embedded archival specimens of OSCC and SGT were stained with specific MSF antibodies and the level of staining was assessed by consensus of 2-4 independent observers. The association between MSF expression and patient survival was determined by Kaplan-Meier and log-rank tests. Results presented in this thesis indicate that TYS and HSG cells secrete bioactive MSF in culture. rhMSF stimulated the migration of these tumour cells. The use of mutant proteins demonstrated marked differences among the cells examined: Five bioactive motifs (4x IGD and 1x HEEGH) were required for MSF bioactivity on TYS and HSG cells, whereas only one of these motifs was required for Endo 742 and two for FSF44. MSF+aa and MSF-aa showed the same migration-stimulating activity, but differ in their interaction with the MSF-inhibitor Neutrophil Gelatinase-Asscciated Lipocalin (NGAL). NGAL was shown to bind to and inhibit MSF+aa, but not MSF-aa. The bioactivity of MSF+aa and MSF-aa was inhibited by Insulin-like Growth Factor Binding Protein-7 (IGFBP7), MSF-function-neutralising antibody and antibody to the integrin avß3. This integrin was identified in the cell membrane material bound to MSF, suggesting that avß3 is a receptor for MSF.

616.994

Análise da via do Akt em neoplasias benignas e malignas de glândulas salivares / Analisys of Akt pathway in benign and malignant salivary galnd tumours

Marques, Yonara Maria Freire Soares

01 October 2010

A proteína Akt modula a função de numerosos substratos envolvidos na regulação da sobrevivência celular, progressão do ciclo celular e crescimento celular. Estudos prévios realizados em nosso laboratório demonstraram a superexpressão de Akt em adenoma pleomórfico, mioepitelioma e carcinoma adenóide cístico. O objetivo deste estudo foi analisar a via da proteína Akt através da avaliação da expressão das proteínas NFkB e PTEN em neoplasias benignas e malignas de glândulas salivares através das técnicas de imunohistoquímica, western blotting e imunofluorescência, e a possível interação protéica direta entre p-Akt/Mdm2 e p-Akt/PTEN em linhagem de carcinoma adenóide cístico. A superexpressão nuclear na proteína PTEN foi encontrada nas duas neoplasias malignas estudadas. Além disso, não foi observada interação direta entre as proteínas p-Akt/Mdm2 e p-Akt/PTEN, as quais apresentam localização nuclear em neoplasias de glândulas salivares. / The Akt protein modulates the function of numerous substrates involved in the regulation of cell survival, cell cycle progression and cell growth. Previous studies from our laboratories showed overexpression of Akt and Mdm2 followed by the lack of p53 expression in pleomorphic adenoma, myoepithelioma and adenoid cystic carcinoma. The aim of this study was to analyze the Akt pathway through evaluation of expression of NFkB and PTEN proteins in pleomorphic adenoma, carcinoma ex pleomophic adenoma and adenoid cystic carcinoma by western blotting, immunofluorescence and immunohistochemical techniques, and we have intended to analyse a possible direct interaction between p-Akt/Mdm2 and p-Akt/ PTEN protein in salivary gland tumours. Overexpression of nuclear PTEN was present in both carcinomas studied. In addition, there was no direct interaction between p-Akt/Mdm2 and p-Akt/ PTEN protein, which presents a nuclear localization in salivary gland tumours.

Akt

Akt

Mdm2

Mdm2

Neoplasias de glândulas salivares

NFkB

NFkB

PTEN

PTEN

Salivary gland tumours

Análise da via do Akt em neoplasias benignas e malignas de glândulas salivares / Analisys of Akt pathway in benign and malignant salivary galnd tumours

Yonara Maria Freire Soares Marques

01 October 2010

A proteína Akt modula a função de numerosos substratos envolvidos na regulação da sobrevivência celular, progressão do ciclo celular e crescimento celular. Estudos prévios realizados em nosso laboratório demonstraram a superexpressão de Akt em adenoma pleomórfico, mioepitelioma e carcinoma adenóide cístico. O objetivo deste estudo foi analisar a via da proteína Akt através da avaliação da expressão das proteínas NFkB e PTEN em neoplasias benignas e malignas de glândulas salivares através das técnicas de imunohistoquímica, western blotting e imunofluorescência, e a possível interação protéica direta entre p-Akt/Mdm2 e p-Akt/PTEN em linhagem de carcinoma adenóide cístico. A superexpressão nuclear na proteína PTEN foi encontrada nas duas neoplasias malignas estudadas. Além disso, não foi observada interação direta entre as proteínas p-Akt/Mdm2 e p-Akt/PTEN, as quais apresentam localização nuclear em neoplasias de glândulas salivares. / The Akt protein modulates the function of numerous substrates involved in the regulation of cell survival, cell cycle progression and cell growth. Previous studies from our laboratories showed overexpression of Akt and Mdm2 followed by the lack of p53 expression in pleomorphic adenoma, myoepithelioma and adenoid cystic carcinoma. The aim of this study was to analyze the Akt pathway through evaluation of expression of NFkB and PTEN proteins in pleomorphic adenoma, carcinoma ex pleomophic adenoma and adenoid cystic carcinoma by western blotting, immunofluorescence and immunohistochemical techniques, and we have intended to analyse a possible direct interaction between p-Akt/Mdm2 and p-Akt/ PTEN protein in salivary gland tumours. Overexpression of nuclear PTEN was present in both carcinomas studied. In addition, there was no direct interaction between p-Akt/Mdm2 and p-Akt/ PTEN protein, which presents a nuclear localization in salivary gland tumours.

Akt

Mdm2

Neoplasias de glândulas salivares

NFkB

PTEN

Akt

Mdm2

NFkB

PTEN

Salivary gland tumours