Classical monocytes from patients with pancreatic ductal adenocarcinoma exhibit a significantly altered transcriptome profile compared with healthy volunteers

Cook, Jenny Anne

January 2014

Pancreatic Ductal Adenocarcinoma (PDAC) affects approximately 8000 people every year in the UK and is the fifth leading cause of cancer related death. At a molecular level PDAC is characterized by a significant immune infiltrate. Tumour-associated macrophages (TAMs) infiltrate the tumour and contribute to a worse prognosis by promoting growth, metastasis and resistance to chemotherapy. TAMs are derived from circulating ‘classical’ CD14++ CD16- monocytes in the peripheral blood. Current work in murine models suggests targeting monocyte recruitment in PDAC can reduce TAM infiltration and disease burden therefore improving survival. This project aims to identify markers specific to monocytes from PDAC patients and to investigate their biological relevance and potential for therapeutic intervention. Gene expression and metabolomics analysis was carried out on classical CD14++ CD16- monocytes from locally advanced PDAC patients and age matched healthy donors. Transcriptomic profiling revealed a significantly altered gene expression profile in classical monocytes from patients and genes with the highest fold change difference were chosen for validation using qPCR. Validated gene targets were investigated further in vitro and large-scale gene expression analysis from pancreatic tumours assessed. The results from my work demonstrate that the gene expression profile of classical monocytes from PDAC patients is significantly different compared to healthy volunteers. Identification and validation of up-regulated genes and their biological relevance may represent a relevant novel novel biomarker or therapeutic strategyies to target monocytes and myeloid recruitment in cancer.

616.99

Mechanostimulation of integrin αvβ6 and fibronectin in DCIS myoepithelial cells

Hayward, Mary-Kate

January 2018

Alterations to the tumour microenvironment is a common feature of many cancers, including breast cancer, and there is increasing evidence that alterations to the microenvironment, including; increased integrin expression, ECM deposition and protease activity, promote cancer progression. Most invasive breast cancers arise from a preinvasive stage, ductal carcinoma in situ (DCIS). Previous work in our laboratory has shown the microenvironment of DCIS is altered, such that myoepithelial cells (MECs) switch to a tumour-promoting phenotype, associated with upregulation of integrin αvβ6 and fibronectin (FN) expression. Mechanisms by which integrin αvβ6 and FN expression are regulated is unclear. We show DCIS progression into invasion is accompanied by an increase in MEC expression of integrin αvβ6 and periductal FN deposition, and their expression were associated in DCIS. These findings were modelled in isolated primary DCIS-MECs, primary normal MECs and MEC lines, with and without integrin αvβ6 expression, where integrin αvβ6-positive MECs upregulating FN expression. We identified integrin αvβ6-positive DCIS ducts were larger than integrin αvβ6-negative DCIS ducts, and mechanical stretching of primary normal MECs and a normal MEC line led to upregulation of integrin αvβ6 expression and FN deposition in a TGFβ-dependent manner. We further show upregulation of integrin αvβ6 and FN by MECs mediate TGFβ-dependent upregulation of MMP13 which promotes breast cancer cell invasion in vitro. These data show altered tissue mechanics in DCIS and MEC expression of integrin αvβ6 and FN deposition are linked, and implicate TGFβ in their activation. These findings suggest integrin αvβ6 and FN may be used as markers to stratify DCIS patients.

Caracterização da expressão de microRNAs em carcinoma de mama receptores hormonais positivos e HER-2 negativo / Caracterização da expressão de microRNAs em carcinoma de mama receptores hormonais positivo e HER-2 negativo

Mendes, Daniele Carvalho Calvano

27 January 2015

Introdução: O câncer de mama é, em sua essência, uma doença genética. O acúmulo de alterações moleculares no genoma das células somáticas é a base para a progressão do câncer. Além de ter biologia natural mais favorável, os tumores com alta expressão de receptores de estrogênio têm terapia-alvo bem estabelecida. Apesar disso, as pacientes podem apresentar resistência medicamentosa, recidiva e óbito. Os microRNAs (miRNAs) são uma classe de pequenas moléculas não codificadoras de proteínas que regulam a expressão gênica durante a etapa de tradução. Esta regulação é feita pelo pareamento de bases com o mRNA-alvo (RNA mensageiro), resultando na supressão da tradução ou na clivagem do mRNA. Se os miRNAs têm como alvo genes supressores de tumor ou oncogenes, podem atuar como supressores tumorais ou oncogenes. OBJETIVO: avaliar a expressão de microRNAs, por PCR em tempo real, no carcinoma mamário ductal invasivo (CDI) com receptores hormonais positivos e HER-2 negativo (luminal A). MÉTODOS: Foram avaliados materiais em parafina de 33 pacientes com tumores luminal A, bem como tecido mamário histologicamente normal. Foram utilizados kit para extração de RNA de amostras fixadas e parafinadas - miRNeasy FFPE; kit para síntese de cDNA - miScript II RT; kit miScript SYBR Green PCR e miScript miRNA PCR Arrays para análise de 84 sequências de miRNA de câncer humano. Analisaram-se dados clínicos, como idade, paridade, amamentação, estado menopausal; variáveis histológicas, como tamanho do tumor, estado linfonodal, invasão linfática; características imunoistoquímicas, como expressão de Ki-67. Para a análise estatística utilizou-se o software miScript miRNA PCR Array Data Analysis, que emprega o método de quantificação relativa ??Ct. RESULTADOS: A análise comparativa dos 33 casos de CDI luminal A com os 15 casos de parênquima mamário normal revelou haver microRNAs hiperexpressos, sendo eles: miR-96-5p (fold-regulation = 9,245, p = 0,000192), miR-182-5p (fold-regulation = 6,4813, p = 0,00024), miR-21-5p (fold-regulation = 6,3129, p = 0,000001), miR- 210-3p (fold-regulation =4,3584, p =0,001002) e. miR-7-5p (fold-regulation = 4,0166, p = 0,036407). Apontou, ainda, microRNAs com hipoexpressão, a saber: miR-204-5p (Fold-regulation = -8,2104, p = 0,000000), miR-125b-5p (Fold-regulation = --6,332, p=0,000000), let-7c-5p (Fold-regulation: -4,5142, p=0,000000) e let-7e-5p (Fold-regulation = -4,059, p = 0,011625): CONCLUSÕES: CDI luminal A apresentou hiperexpressão de miR-96-5p, miR-182-5p, miR-21-5p, miR-210-3p e miR-7-5p. Apontou, ainda, hipoexpressão do miR-204-5p, miR-125b-5p, let-7c-5p e let-7e-5p, permitindo diferenciá-lo do tecido normal / INTRODUCTION: Breast cancer is a genetic disease and the accumulation of molecular alterations in the genome of somatic cells is the basis for cancer progression. Besides having a more favorable natural biology, tumors with high expression of estrogen receptor have a well established targeted therapy. Nevertheless, patients may present with resistance and eventually relapse and death. MicroRNAs (miRNAs) are a class of small non-coding protein molecules that regulate gene expression during the translation stage. This adjustment is made by base pairing with the mRNA (messenger RNA) target resulting in suppression of translation or cleavage of the mRNA. Depending on whether miRNAs target tumor suppressor genes or oncogenes, they can act as tumor suppressors or oncogenes. OBJECTIVE: evaluate the expression of microRNAs by RT-PCR in positive hormonal receptors, negative HER 2 (luminal A) invasive ductal carcinoma (IDC). METHODS: Paraffin embedded tumor material from 33 patients with luminal A IDC, and histologically normal breast tissue. Were used: Kit for RNA extraction from fixed and paraffin embedded samples - miRNeasy FFPE; cDNA synthesis kit - miScript II RT; miScript SYBR Green PCR Kit and miScript miRNA PCR Arrays for analysis of 84 miRNA sequences of human cancer. Clinical data such as age, parity, breastfeeding, menopausal status; histological variables such as tumor size, lymph node status, lymphatic invasion; immunohistochemical characteristics, such as expression of Ki-67, were evaluated. For statistical analysis the miScript miRNA PCR Array Data Analysis software, which uses the method of relative quantification ??Ct, was used. RESULTS: A comparative analysis of 33 cases of luminal A IDC with 15 cases of normal breast parenchyma defined microRNAs overexpressed, as follows: miR-96-5p (fold-regulation = 9,245, p = 0,000192), miR-182-5p (fold-regulation = 6,4813, p = 0,00024), miR-21-5p (fold-regulation = 6,3129, p = 0,000001), miR- 210-3p (fold-regulation =4,3584, p =0,001002) and miR-7-5p (fold-regulation = 4,0166, p = 0,036407). Furthermore, microRNAs with reduced expression, as follows:. miR-204-5p (Fold-regulation = -8,2104, p = 0,000000), miR-125b-5p (Fold-regulation = -6,332, p=0,000000), let-7c-5p (Fold-regulation: -4,5142, p=0,000000) and let-7e-5p (Fold-regulation = -4,059, p = 0,011625): CONCLUSION: Luminal A CDI breast cancer has shown overexpression of miR-96-5p, miR-182-5p, miR-21-5p, miR-210-3p and miR-7-5p. Also has shown,downregulation of miR-204-5p, miR-125b-5p, let-7c-5p e let-7e-5p, allowing differentiating it from normal tissue

Breast neoplasms/pathology

Carcinoma ductal breast/genetics

Carcinoma ductal breast/pathology

Carcinoma ductal de mama/genética

Carcinoma ductal de mama/patologia

Expressão gênica

Gene expression

Genes supressores de tumor

Genes tumor suppressor

Immunohistochemistry

Imuno-histoquímica

Marcadores biológicos de tumor/análise

MicroRNAs

MicroRNAs

Neoplasias da mama/patologia

Prognosis

Prognóstico

Real-time polymerase chain reaction

Tumor markers biological/analysis

Expressão imuno-histoquímica da topoisomerase III? nos carcinomas mamários / Prognostic significance of topoisomerase III immunohistochemical expression in breast carcinomas

João Paulo Oliveira da Costa

17 August 2010

Topoisomerases são enzimas nucleares que participam na regulação da estrutura do DNA nas células eucarióticas. A topoisomerase III é o mais novo membro da família das topoisomerases. Seu papel no desenvolvimento dos tumores mamários ainda necessita ser investigado. O objetivo do presente estudo foi avaliar a imunoexpressão da topoisomerase III nos carcinomas mamários, e comparar sua expressão com dados clinicopatológicos e marcadores imunohistoquímicos clássicos de importância prognóstica nos carcinomas mamários. Utilizando-se tissue microarrays contendo 171 casos de carcinomas ductais mamários primários, foi analisada a expressão imunohistoquímica de topoisomerase III, receptor de estrógeno, receptor de progesterona, HER-2, Ki67, p53 e BRCA-1. Positividade para topoisomerase III foi encontrada em 33,9% dos casos, e sua expressão relacionou-se com metástases à distância (p=0.036) e óbito (p=0.006). Negatividade para topoisomerase III relacionou-se com negatividade para HER=2 (p<0.001), p53 (p<0.001) e BRCA-1 (p=0.001), e com baixa expressão de Ki-67 (p<0.001). Na Análise de Riscos Múltiplos de Cox, a expressão de topoisomerase III foi um significante preditor de sobrevida [razão de risco 3.006 (intervalo de confiança a 95%: 1.582-5.715); p=0.001]. Concluindo, a topoisomerase III pode ser útil na avaliação do prognóstico de pacientes com câncer de mama, além de ser um fator independente de predição da sobrevida. / Topoisomerases are ubiquitous nuclear enzymes that regulate DNA structure in eukaryotic cells. The role of topoisomerase III, the newest member of the topoisomerase family, in the clinical outcome of breast cancer is still poorly understood. This study aims to investigate the immunoexpression of topoisomerase III in breast cancer and its relationships with clinicopathological features and immunohistochemical markers of prognostic significance in breast pathology. Using tissue microarrays containing 171 cases of primary invasive breast cancer, we analyzed the immunoexpression of topoisomerase III, estrogen receptor, progesterone receptor, HER-2, Ki67, p53 and BRCA-1. Immunostaining for topoisomerase III was found in 33.9% of breast carcinomas, and immunopositivity was related with distant metastasis (p=0.036) and death (p=0.006). Decreased expression of topoisomerase III was related with negativity with HER-2 (p<0.001), p53 (p<0.001) and BRCA1 (p=0.001) and low expression of Ki67 (p<0.001). In the multivariate analysis, topoisomerase III expression was a significant predictor of survival [hazard ratio 3.006 (95% confidence interval 1.582-5.715); p=0.001]. In conclusion, topoisomerase III expression can be a useful marker in assessing the prognosis of patients with breast cancer and is an independent predictor of survival.

Carcinomas mamários

Fator prognóstico

Imuno-histoquímica

Sobrevida

topoisomerases

Breast ductal carcinoma

Imunohistochemistry

Prognosis

Topoisomerase III

Association of Oct4, Sox2, Nanog and Lin28 Protein Expression Levels with the Prognosis of Invasive Mammary Ductal Carcinoma Patients

Huang, Sheng-feng

30 August 2012

Breast cancer is the most common cancer in Taiwanese women and the invasive ductal carcinoma (IDC) is the most common type. Increasing evidence shows that cancer stem cells (CSCs) have been implicated in tumorigenesis, tumor progression, and drug-resistance. In addition, four reprogramming factors (Octamer-binding Protein 4 (Oct4), Sex-determining Region Y (SRY)-related Box 2 (Sox2), Nanog and Lin28) employed to induce induced pluripotent stem (iPS) cells are associated with CSCs formation. The purpose of this study was to investigate the relationship of the protein expression levels of the reprogramming factors (Oct4, Sox2, Nanog and Lin28) with the tumorigenesis, clinicopathologic outcomes and prognosis of breast IDC patients. Immunohistochemistry (IHC) assay of tissue microarrays, made by 309 IDC and 20 breast fibrosis paraffin embedded samples, were used to examine the protein expression levels of Oct4, Sox2, Nanog and Lin28 in normal mammary ductal tissues, tumor adjacent normal mammary ductal tissues, ductal carcinoma in situ (DCIS), IDC and recurrence tissues. Our IHC results showed that Sox2 and Lin28 were expressed in half of breast IDC patients¡¦ tumor tissue (49.6% and 49.7%, respectively), but Oct4 and Nanog are less expressed (13.5% and 24.7%, respectively). The protein expression levels of the four proteins were positively correlated with each other. In addition, the expression levels of the four proteins were upregulated in tumor adjacent normal tissue as compared to breast fibrosis pateints¡¦ normal mammary ductal tissue. To compare the expression levels of the four proteins in different tissues; such as tumor adjacent normal, DCIS, IDC and recurrence tissues, the expression levels of the four protiens gradually decreased when tumor developed and progressed. However, their expression levels were comparable between IDC and recurrence tissues. Additionally, the high expression levels of four proteins were high in two good clinicopathological characteristics and a biomarker of breast cancer; such as nuclear Sox2 and Lin28 in those with pathology stage I; nucleus expression of the four proteins in those with well and moderate cell differentiation; and Sox2 in those with positive estrogen receptor. However, the four proteins¡¦ expression levels were not correlated with IDC patients¡¦ survival. In conclusion, the reprogramming factors: Oct4, Sox2, Nanog and Lin28 may play an important role in tumorigenesis of breast IDC, but their impacts on tumor progression were quite small.

reprogramming factor

induce induced pluripotent stem cell

tissue microarray

Invasive ductal carcinoma

Gene expression profiling of the breast tumour microenvironment : characterization of gene expression heterogeneity in the breast tumour microenvironment and its influence on clinical outcome

Finak, Grzegorz.

January 2008

Breast cancer is a very heterogeneous disease. This heterogeneity can be observed at many levels, including gene expression, chromosomal aberrations, and disease pathology. A clear understanding of these differences is important since they impact upon treatment efficacy and clinical outcome. Recent studies have demonstrated that the tumour microenvironment also plays a critical role in cancer initiation and progression. Genomic technologies have been used to gain a better understanding of the impact of gene expression heterogeneity on breast cancer, and have identified gene expression signatures associated with clinical outcome, histopathological breast cancer subtypes, and a variety of cancer-related pathways and processes. However, little work has been done in this context to examine the role of the tumour microenvironment in determining breast cancer outcome, or in defining breast cancer heterogeneity. Additionally, little is known about gene expression in histologically normal tissue adjacent to breast tumour, if this is influenced by the tumour, and how this compares with non-tumour-bearing breast tissue. By applying laser--capture microdissection and gene expression profiling to clinical breast cancer specimens the research presented in this thesis addresses these questions. / We have generated gene expression profiles of morphologically normal epithelial and stromal tissue, isolated using laser capture microdissection, from patients with breast cancer or undergoing breast reduction mammoplasty. We determined that morphologically normal epithelium and stroma exhibited distinct expression profiles, but molecular signatures that distinguished breast reduction tissue from tumour-adjacent normal tissue were absent. Stroma isolated from morphologically normal ducts adjacent to tumour tissue contained two distinct expression profiles that correlated with stromal cellularity, and shared similarities with soft tissue tumors with favourable outcome. Adjacent normal epithelium and stroma from breast cancer patients showed no significant association between expression profiles and standard clinical characteristics, but did cluster ER/PR/HER2-negative breast cancers with basal-like subtype expression profiles with poor prognosis. Our data reveal that morphologically normal tissue adjacent to breast carcinomas has not undergone significant gene expression changes when compared to breast reduction tissue, and provide an important gene expression data set for comparative studies of tumour expression profiles. / We compared gene expression profiles of tumour stroma from primary breast tumors and derived signatures strongly associated with clinical outcome. We present a new stroma-derived prognostic predictor (SDPP) that stratifies disease outcome independently of standard clinical prognostic factors and published expression-based predictors. The SDPP predicts outcome in several published whole tumour--derived expression data sets, identifies poor-outcome individuals from multiple clinical subtypes, including lymph node--negative tumors, and shows increased accuracy with respect to previously published predictors, especially for HER2-positive tumors. Prognostic power increases substantially when the predictor is combined with existing outcome predictors. Genes represented in the SDPP reveal the strong prognostic capacity of differential immune responses as well as angiogenic and hypoxic responses, highlighting the importance of stromal biology in tumour progression. / We show that gene expression in the breast tumour microenvironment is highly heterogeneous, identifying at least six different classes of tumour stroma with distinct expression patterns and distinct biological processes. Two of these classes recapitulate the processes identified in the stroma-derived prognostic predictor, while the others are new classes of stroma associated with distinct clinical outcomes. One of these is associated with matrix remodelling and is strongly associated with the basal molecular subtype of breast cancer. The remainder are independent of the previously published molecular subtypes of breast cancer. Additionally, based on independent data from over 800 tumors, the combinations of stroma classes and breast cancer subtypes identify new subgroups of breast tumors that show better discrimination between good and poor outcome individuals than the molecular breast cancer subtypes or the stroma classes alone, suggesting a novel classification scheme for breast cancer. This research demonstrates an important role for the tumour microenvironment in defining breast cancer heterogeneity, with a consequent impact upon clinical outcome. Novel therapies could be targeted at the processes that define the stroma classes suggesting new avenues for individualized treatment.

Breast Neoplasms -- pathology.

Carcinoma, Ductal, Breast -- pathology.

Stromal Cells -- physiology.

Prognosis.

Gene Expression Profiling.

Validation of Candidate Biomarkers for the Development of a Multi-Parametric Panel for Early Detection of Pancreatic Ductal Adenocarcinoma (PDAC)

Chan, Alison Hui-Wai

21 November 2013

High-throughput mass spectrometry has discovered a plethora of candidates in the biomarker field, however, subsequent verification and validation studies are urgently needed to assess the potential of novel biomarkers in the detection of pancreatic cancer. We have conducted extensive verification and validation studies on two of our most promising biomarkers CUZD1 and LAMC2 with a total of 715 blood samples. In our study, both markers demonstrated consistent diagnostic ability of early- and CA19.9 negative-PDAC cases. When used in combination with CA19.9, CUZD1 and LAMC2 were shown to significantly improve the performance of CA19.9 alone in the diagnosis of PDAC patients. We speculate that CUZD1 and LAMC2 may be good candidates to be used in a panel for monitoring PDAC patients who do not express CA19.9 levels as well as for an aid in screening high risk populations. Further validation of these two proteins is warranted.

pancreatic cancer

early diagnosis

pancreatic ductal adenocarcinoma

biomarker

validation

0992

0571

Validation of Candidate Biomarkers for the Development of a Multi-Parametric Panel for Early Detection of Pancreatic Ductal Adenocarcinoma (PDAC)

Chan, Alison Hui-Wai

21 November 2013

High-throughput mass spectrometry has discovered a plethora of candidates in the biomarker field, however, subsequent verification and validation studies are urgently needed to assess the potential of novel biomarkers in the detection of pancreatic cancer. We have conducted extensive verification and validation studies on two of our most promising biomarkers CUZD1 and LAMC2 with a total of 715 blood samples. In our study, both markers demonstrated consistent diagnostic ability of early- and CA19.9 negative-PDAC cases. When used in combination with CA19.9, CUZD1 and LAMC2 were shown to significantly improve the performance of CA19.9 alone in the diagnosis of PDAC patients. We speculate that CUZD1 and LAMC2 may be good candidates to be used in a panel for monitoring PDAC patients who do not express CA19.9 levels as well as for an aid in screening high risk populations. Further validation of these two proteins is warranted.

pancreatic cancer

early diagnosis

pancreatic ductal adenocarcinoma

biomarker

validation

0992

0571

Modelo experimental de lesões intra-epiteliais e de adenocarcinoma ductal pancreático induzidos por 7,12-dimetilbenzantraceno em camundongos

Osvaldt, Alessandro Bersch

January 2004

INTRODUÇÃO: O adenocarcinoma de pâncreas apresenta um mau prognóstico. A utilização de modelos experimentais é necessária para a compreensão do comportamento biológico tumoral, principalmente das lesões precoces (neoplasias intra-epiteliais pancreáticas - NIPan) e para o desenvolvimento de opções terapêuticas. OBJETIVO: Avaliar a carcinogênese pancreática induzida por 7,12-dimetilbenzantraceno (DMBA), em camundongos, aplicando a classificação das neoplasias intra-epiteliais pancreáticas. MÉTODOS: 90 camundongos machos, mus musculus, da cepa CF1, foram submetidos à laparotomia mediana e 1 mg de DMBA foi implantado na porção cefálica do pâncreas. Os animais foram divididos em dois grupos, com eutanásia em 30 e 60 dias. Em seguida, o pâncreas foi retirado, fixado em formalina e foram confeccionadas lâminas coradas com hematoxilina eosina. Os cortes histológicos foram avaliados por dois patologistas de acordo com os seguintes critérios: pâncreas normal, hiperplasia reacional, NIPan 1A, NIPan 1B, NIPan 2, NIPan 3 e carcinoma. As alterações inflamatórias também foram analisadas. RESULTADOS: A avaliação patológica evidenciou, no grupo de 30 dias: 4 (16,7%) animais com hiperplasia reativa, 16 (66,6%) com NIPan e 4 (16,7%) com adenocarcinoma. No grupo de 60 dias: 10 (27,1%) animais com hiperplasia reativa, 13 (35,1%) com NIPan e 14 (37,8%) com adenocarcinoma. A diferença entre os grupos apresentou significância estatistística (P < 0,05 – teste exato de Fisher). A prevalência de alterações inflamatórias em 30 dias foi: pancreatite aguda (n=11), pancreatite crônica (n=5) e inflamação dependente da bolsa (n=8). No grupo de 60 dias 11 espécimes apresentavam pancreatite aguda e 26 pancreatite crônica. CONCLUSÕES: O modelo experimental com DMBA em camundongos, induz neoplasia intra-epitelial pancreática e adenocarcinoma ductal histologicamente semelhantes ao carcinoma pancreático em humanos. Este modelo pode ser utilizado na investigação da carcinogênese com enfoque na progressão molecular das lesões precursoras até o adenocarcinoma. / BACKGROUND: Pancreatic adenocarcinoma has a dismal long-term prognosis. Experimental models are necessary to understand its biological behavior mainly the early pancreatic lesions termed pancreatic intraepithelial neoplasia (PanIN) and to develop new treatments. OBJECTIVE: The aim of this study is to evaluate pancreatic carcinogenesis induced by DMBA implantation in mice according to PanIN classification system. METHODS: 90 male, mus musculus, CF1 mice were submitted to a median laparotomy and 1 mg of DMBA was implanted in the head of the pancreas holded with a purse-string suture. Euthanasia was done after 30 and 60 days. After, the excised pancreata were fixed in formalin, embedded in paraffin and stained with haematoxylin and eosin for histology. The specimens were evaluated by two pathologists according to the following criteria: normal ducts, reactive hyperplasia, PanIN 1A, PanIN 1B, PanIN 2, PanIN 3 and carcinoma. The inflammatory changes were also analyzed. RESULTS: The pathologic evaluation showed for 30 days group 4 (16.7%) reactive hyperplasia, 16 (66.6%) PanIN and 4 (16.7%) adenocarcinomas. In the 60 days group there were 10 (27.1%) specimens with reactive hyperplasia, 13 (35.1%) with PanIN lesions and 14 (37.8%) with adenocarcinomas. The difference between groups was statistically significant (P < 0,05; Fisher exact test). The prevalence of inflammatory changes in 30 days groups were: acute pancreatitis (n=11), chronic pancreatitis (n=5) and DMBA pocket dependent (n=8). In the 60 days groups, 11 had acute pancreatitis and 26 had chronic pancreatitis. CONCLUSIONS: DMBA experimental model in mice induces characteristic pancreatic intraepithelial neoplasia and ductal adenocarcinoma histologically similar to human pancreatic cancer. This model is useful for the study of pancreatic carcinogenesis emphasizing the molecular progression of early pancreatic lesions.

Adenocarcinoma

Neoplasias pancreáticas

Carcinoma ductal pancreático

Modelos animais

Camundongos

9,10-Dimetil-1,2-benzantraceno

ROLES OF LIPOGENESIS IN BREAST CANCER PROGRESSION

Pandey, Puspa Raj

01 May 2012

Elevated level of lipogenic enzymes and overall lipogenesis have been reported in a wide variety of cancers and blocking the lipogenic pathway by chemical inhibitors or RNA interference causes tumor cell death by apoptosis which provides a strong rationale for targeting lipogenic pathway for the treatment and prevention of cancer however the exact role of lipogenesis as a cause, facilitator or consequence is not yet clearly understood. Therefore in this dissertation research, we set up to determine the mechanism of tumor cell death by inhibiting lipogenesis and to determine the role of increased lipogenesis in the breast cancer progression. In the first part of this study, we investigated the status of fatty acid synthase (FAS) gene which is regarded as the key lipogenic gene in fatty acid biosynthetic pathway and is responsible for the synthesis of lipid molecules by facilitating the condensation reaction between acetyl-CoA and malonyl-CoA in the presence of NADPH. We observed that normal breast epithelial cells MCF10A cells have very low level of FAS expression whereas breast cancer cell lines MCF7, MDA MB231 and MDA MB231 LM have significant overexpression. Next, we observed the similar trend of FAS overexpression in breast cancer stem-like cells (CSCs) isolated from the MCF7, MDA MB231 and MDA MB231 LM cell lines using cell surface markers (CD24-/CD44+/ESA+). These cells were previously transplanted into the mammary fat pad of nude mice and the results of our limiting dilution analysis indicate that CSCs had a significantly higher ability of forming breast cancer in the injected animals which explains our rationale to use CSCs in our research. In order to exploit this lipogenic pathway for the treatment and chemoprevention of breast cancer, we then examined the effects of resveratrol on breast cancer cells. Resveratrol is a natural polyphenolic compound and has been shown to exhibit cardio-protective as well as anti-neoplastic effects on various types of cancers. However, the exact mechanism of its anti-tumor effect is not clearly defined. We observed that resveratrol significantly reduced the cell viability by inducing apoptosis in parental cells as well as in CSCs. Resveratrol also inhibited mammosphere formation which is an inherent property of CSCs. This inhibitory effect of resveratrol is accompanied by a significant reduction in lipid synthesis which is caused by the down-regulation of the FAS gene followed by up-regulation of pro-apoptotic genes, DAPK2 and BNIP3. The activation of apoptotic pathway in the cancer stem-like cells was suppressed by FAS overexpression suggesting that resveratrol-induced apoptosis is indeed through the modulation of FAS-mediated cell survival signaling. Importantly, resveratrol was able to significantly suppress the growth of CSC in an animal model of human breast cancer xenograft without showing apparental toxicity. Taken together, our results indicate that resveratrol is capable of inducing apoptosis in the CSCs through suppression of lipogenesis by modulating FAS expression, which highlights a novel mechanism of anti-tumor effect of resveratrol. Taken together, our results indicate that resveratrol is capable of inducing apoptosis in the cancer stem-like cells through suppression of lipogenesis by modulating FAS expression, which highlights a novel mechanism of anti-tumor effect of resveratrol. In the second part of research, we tried to determine the role of elevated level of lipogenesis in normal to ductal carcinoma in situ (DCIS) progression. For this, we first analyzed the expression profile of various lipogenic genes using an expression microarray and found that CSCs from DCIS.com showed significantly higher level of ATP-citrate lyase (ACLY), acetyl-CoA carboxylase (ACC) and FAS than the normal non-tumorigenic stem-like cells obtained from MCF10A. The result was also confirmed by qRT-PCR and Western blot as well as in clinical specimens of DCIS by immunohistochemistry. In the next step, we detected that SREBP1, the master regulator of lipogenic genes, is also upregulated in DCIS and further identified that SREBP1 regulates the co-ordinate expression of ACLY, ACC and FAS ultimately resulting in the elevation of lipogenesis. In order to determine the role of SREBP1 overexpression in normal to DCIS transition, we overexpressed the SREBP1 in MCF10A cells which induced a significant increase in the downstream key lipogenic genes ACLY, ACC1 and FAS which resulted in the clear upregulation of total lipid content in the cells. Furthermore, we found that this elevation of lipogenesis in MCF10A-SREBP1 stem-like cells confers proliferative advantage as well as a significant increase in mammosphere forming ability and anchorage independent growth (3D culture). Thus, our results showed a possibility that increased lipogenesis in normal stem-like cells may be responsible for providing oncogenic transformation properties which can be confirmed at least in our in vitro model. We then examined the effects of resveratrol on CSCs sorted from DCIS.com. We found that resveratrol decreased the cell viability and increased apoptosis by reducing the total lipid content by inhibiting the expression of SREBP1 and downstream lipogenic genes. Resveratrol also hindered the stemness of the DCIS CSCs by inhibiting its mammosphere forming ability. When DCIS CSCs were transplanted into mammary fat pad of nude mice which were on resveratrol treatment, we observed that resveratrol significantly suppressed the formation of DCIS by downregulating lipogenic genes and by upregulating pro-apoptotic genes, DAPK2 and BNIP3. Collectively, our results indicate that lipogenic genes SREBP1 co-ordinately regulates the overexpression of ACLY, ACC1 and FAS in DCIS CSCs at an early stage of breast tumorigenesis and thus confer proliferative and survival advantages. Anti-growth effect of resveratrol on DCIS CSCs also provides us with a strong rationale to use this agent for chemo-prevention against DCIS.

Breast cancer

Cancer stem cells

Chemoprevention

Ductal carcinoma in situ

Lipogenesis

Resveratrol