Chronic Disruption of the Late Cholesterol Synthesis Leads to Female-Prevalent Liver Cancer

Cokan, Kaja Blagotinšek, Urlep, Žiga, Lorbek, Gregor, Matz-Soja, Madlen, Skubic, Cene, Perše, Martina, Jeruc, Jera, Juvan, Peter, Režen, Tadeja, Rozman, Damjana

13 April 2023

While the role of cholesterol in liver carcinogenesis remains controversial, hepatocellular carcinoma generally prevails in males. Herein, we uncover pathways of female-prevalent progression to hepatocellular carcinoma due to chronic repression of cholesterogenic lanosterol 14α-demethylase (CYP51) in hepatocytes. Tumors develop in knock-out mice after year one, with 2:1 prevalence in females. Metabolic and transcription factor networks were deduced from the liver transcriptome data, combined by sterol metabolite and blood parameter analyses, and interpreted with relevance to humans. Female knock-outs show increased plasma cholesterol and HDL, dampened lipid-related transcription factors FXR, LXRα:RXRα, and importantly, crosstalk between reduced LXRα and activated TGF-β signalling, indicating a higher susceptibility to HCC in aging females. PI3K/Akt signalling and ECM-receptor interaction are common pathways that are disturbed by sex-specific altered genes. Additionally, transcription factors (SOX9)2 and PPARα were recognized as important for female hepatocarcinogenesis, while overexpressed Cd36, a target of nuclear receptor RORC, is a new male-related regulator of ECM-receptor signalling in hepatocarcinogenesis. In conclusion, we uncover the sex-dependent metabolic reprogramming of cholesterol-related pathways that predispose for hepatocarcinogenesis in aging females. This is important in light of increased incidence of liver cancers in post-menopausal women.

info:eu-repo/classification/ddc/610

ddc:610

Genetic Variants in the Promoter Region of the Macrophage Migration Inhibitory Factor are Associated with the Severity of Hepatitis C Virus-Induced Liver Fibrosis

Wirtz, Theresa Hildegard, Fischer, Petra, Backhaus, Christina, Bergmann, Irina, Brandt, Elisa Fabiana, Heinrichs, Daniel, Koenen, Maria Teresa, Schneider, Kai Markus, Eggermann, Thomas, Kurth, Ingo, Stoppe, Christian, Bernhagen, Jürgen, Bruns, Tony, Fischer, Janett, Berg, Thomas, Trautwein, Christian, Berres, Marie-Luise

31 January 2024

Two polymorphisms in the promoter region of macrophage migration inhibitory factor (MIF)—rs755622 and rs5844572—exhibit prognostic relevance in inflammatory diseases. The aim of this study was to investigate a correlation between these MIF promoter polymorphisms and the severity of hepatitis C virus (HCV)-induced liver fibrosis. Our analysis included two independent patient cohorts with HCV-induced liver fibrosis (504 and 443 patients, respectively). The genotype of the single nucleotide polymorphism (SNP) -173 G/C and the repeat number of the microsatellite polymorphism -794 CATT5–8 were determined in DNA samples and correlated with fibrosis severity. In the first cohort, homozygous carriers of the C allele in the rs755622 had lower fibrosis stages compared to heterozygous carriers or wild types (1.25 vs. 2.0 vs. 2.0; p = 0.03). Additionally, 7 microsatellite repeats were associated with lower fibrosis stages (<F2) (p = 0.04). Comparable tendencies were observed in the second independent cohort, where fibrosis was assessed using transient elastography. However, once cirrhosis had been established, the C/C genotype and higher microsatellite repeats correlated with impaired liver function and a higher prevalence of hepatocellular carcinoma. Our study demonstrates that specific MIF polymorphisms are associated with disease severity and complications of HCV-induced fibrosis in a stage- and context-dependent manner.

info:eu-repo/classification/ddc/610

ddc:610

HEPATOCYTE DIFFERENTIATION AND HEPATOCELLULAR CARCINOMA: RATIONALE FOR P53 INDEPENDENT THERAPY

Enane, Francis Obunyakha

02 June 2017

No description available.

Medicine

Molecular Biology

Biochemistry

Genetics

REAL-TIME ASSESSMENT OF THERMAL TISSUE DAMAGE USING DIFFUSE REFLECTANCE SPECTROSCOPY

Nagarajan, Vivek Krishna

January 2017

No description available.

Biomedical Engineering

Biophysics

Medical Imaging

Optics

Functional and Structural Analysis of Decellularized Liver Tissue Matrix, with Potential Applications in Cancer Tissue Engineering

Hansen, Ryan

30 August 2017

No description available.

Biomedical Engineering

tissue engineering

liver

decellularization

extracellular matrix

ecm

liver cancer

hcc

hepatocellular carcinoma

patient-derived xenograft

pdx

Comparison of proteins of the endoplasmic reticulum from control rat liver with proteins of the endoplasmic reticulum from dissected liver tumor nodules

Abdou, Eman

January 2008

Mémoire numérisé par la Division de la gestion de documents et des archives de l'Université de Montréal.

Réticulum endoplasmique

Carcinome hépatocellulaire

Immunobuvardage

Protéomique

Spectrométrie de masse

Protéines phosphorylées

Protéines inconnues

Biomarqueurs

Endoplasmic reticulum

Hepatocellular carcinoma

Immunoblot

Proteomics

Mass spectrometry

Phosphorylated proteins

Unknown proteins

Biomarkers

Voies de la glycosylation et carcinome hépatocellulaire

Borentain, Patrick

07 December 2012

La glycosylation est un processus enzymatique permettant l'ajout de sucres à des composés (sucres, lipides ou protides), modifiant ainsi leurs propriétés. La glycosylation est impliquée dans la détoxification des xénobiotiques et des variations d'activité des enzymes responsables ont été identifiées comme facteur de risque de cancer en particulier dans les organes exposés aux xénobiotiques. Dans la première partie de notre travail nous étudions l'impact des polymorphismes génétiques de certaines enzymes responsables de la détoxification (UGT1A7, GST et XRCC1) sur le risque de carcinome hépatocellulaire. Nous montrons que la combinaison de certains polymorphismes génétiques peut entraîner une augmentation du risque de CHC. Des modifications d'expression des glycoprotéines de surface ont été observées dans les cellules cancéreuses jouant un rôle dans leurs interactions avec le microenvironnement. Dans la seconde partie, nous étudions l'effet de l'inhibition des interactions des cellules de CHC/cellules endothéliales par le blocage du couple sialyl Lewis x/E-sélectine sur la croissance tumorale. Ce blocage est obtenu, d'une part par transfert du gène de la Fucosyl-transferase I, inhibant l'expression de sLex à la surface des cellules de CHC, et d'autre part, par utilisation de cimétidine ou d'amiloride permettant une inhibition de l'expression de la E-sélectine par les cellules endothéliales. Nous obtenons une inhibition de la croissance tumorale in vivo par blocage de la néoangiogénèse. Ces travaux permettent donc d'identifier des facteurs de risque génétiques de CHC et d'envisager une autre voie de traitement du CHC. / Glycosylation is an enzymatic process that consists of the addition of glycosyl groups to compounds (sugars, lipids or proteins), thus modifying their properties. Glycosylation is involved in the detoxification of xenobiotics and variations in activity of enzymes responsible have been identified as a potential risk factor for cancer in particular in organs in contact with the external environment. In the first part of our work we study the impact of polymorphisms of detoxification enzyme (UGT1A7, GST and XRCC1) on the risk of hepatocellular carcinoma. We show that the combination of genetic polymorphisms of such enzymes may increase the risk of HCC. Modifications in the expression of surface glycoproteins have been observed in cancer cells and play a role in their interactions with the tumoral microenvironment. In the second part, we study the effect of inhibition of interactions of HCC cells / endothelial cells on tumor growth by blocking the interaction between sialyl Lewis x and E-selectin. First, we achieved the inhibition of the expression of sLex on the surface of HCC cells by introducing fucosyl transferase- I gene in HCC cells. In a second part of our work we used cimetidine and amiloride to inhibit the expression of E-selectin by endothelial cells. This approach resulted in inhibition of HCC cells / endothelial cells interaction and thereby tumor growth inhibition in vivo. This effect is mediated by an inhibition of tumor neoangiogenesis. This work therefore identifies genetic risk factors for HCC and allows considering another way of treatment of HCC.

Carcinome hépatocellulaire

Glycosylation

Enzymes de détoxification

Polymorphismes génétiques

Sélectines

Sialyl Lewis

Néoangiogénèse

Amiloride

Cimétidine

Hepatocellular carcinoma

Glycosylation

Detoxification enzymes

Genetic polymorphisms

Selectins

Sialyl Lewis

Neo angiogenesis

Amiloride

Cimetidine

Sítios polimórficos do gene hfe em estudos populacionais e em doenças hereditárias ou adquiridas que cursam com sobrecarga de ferro / Population study of polymorphic loci in HFE gene in hereditary or acquire disease course to iron overload

Campos, Wagner Narciso de

31 July 2013

Mutações no gene HFE têm sido apontadas como um dos principais fatores para o desenvolvimento de sobrecarga de ferro, especialmente os SNPs (single nucleotide polymorphism) clássicos C282Y e H63D. A sobrecarga de ferro pode ser primária, atribuída diretamente a mutações do gene HFE (hemocromatose hereditária - HH) ou adquirida em decorrência de fatores genéticos e de comorbidades, particularmente, infecção pelo vírus da hepatite C (HCV) e carcinoma hepatocelular (CHC). Desequilíbrio de ligação entre os SNPs principais do gene HFE com alelos dos genes HLA-A e HLA-B podem contribuir com alterações da função das células do sistema imunológico. Neste trabalho, sequenciamos a região codificadora do gene HFE (éxon 2, 3, 4 e 5) de pacientes que apresentam ou não sobrecarga de ferro primária ou adquirida. Assim, estudamos 130 pacientes com hepatite C, 60 pacientes com CHC, 14 pacientes com HH e 100 indivíduos saudáveis. Foram encontrados sete SNPs no gene HFE no sentido 5\' para 3\': i) H63D C>G no éxon 2 (rs1799945); ii) IVS2(+4)T>C no íntron 2 (rs2071303); iii) íntron 3 C>G (rs807209); iv) C282Y G>A no éxon 4 (rs1800562); v) íntron 4 G>A (rs2794717); vi) IVS4(-44) T>C (rs1800708); vii) no íntron 5 a deleção G>del, ainda não foi descrita na literatura. Foram realizadas as reconstruções de haplótipos da região codificadora e os haplótipos estendidos englobando o gene HFE e dez outros loci (HLA-A, HLA-B, HLA-C, HLA-DRB1, HLA-DQB1, TNFa, TNFb, TNFc, TNFd e HLA-G-14pb). Também, normatizamos a nomenclatura do gene de acordo com as regras do The International ImMunoGeneTics Information System - IMGT (http://www.imgt.org/). Diversas ferramentas foram utilizadas para avaliar a associação entre os sítios polimórficos do gene HFE com a sobrecarga de ferro, incluindo testes de associações avaliando alelos, genótipos, desequilíbrio de ligação, haplótipos e diplótipos, testes de diversidades e neutralidade. Finalmente, comparamos os SNPs do gene HFE encontrados na população saudável do presente trabalho com as diversas populações mundiais, disponíveis no sítio 1000genomes (http://www.1000genomes.org/). Os resultados demonstraram que a nossa a população estava mais próxima das populações europeias e americanas, sendo parcialmente próxima das populações africanas e distante das populações asiáticas. O alelo C282Y G, contido no haplótipo da região codificadora HFE*01:03, conferiu susceptibilidade a HH na população brasileira testada, concordando com os achados observados em outras populações mundiais. O diplótipo HFE*01:02:01:01/HFE*01:01:01:05 conferiu susceptibilidade para o desenvolvimento de sobrecarga de ferro em pacientes com CHC causado pelo HCV. Detectamos forte desequilíbrio entre os alelos H63D G e IVS2(+4) C no éxon 2 do gene HFE, e concomitantemente, desequilíbrio desses alelos com alelo HLA-B*44, aparentemente, sem associação com sobrecarga de ferro, mas com aparente origem histórica. Finalmente, o teste de diversidade encontrou diferenças apenas na amostra de HH e o teste de neutralidade não encontrou pressões seletivas na população controle do presente trabalho. Concluindo, este é o primeiro trabalho, avaliando grande segmento da região codificadora do gene HFE em diversas amostras de pacientes apresentando ou não sobrecarga de ferro e em indivíduos controle. / Mutations at the HFE gene have been identified as a major factor for the development of iron overload, especially the classical single nucleotide polymorphism (SNP) C282Y and H63D. Primary iron overload can be directly attributed to mutations in the HFE gene (hereditary hemochromatosis - HH), whereas secondary overload may be acquired due to genetic factors and comorbidities, particularly infection with hepatitis C virus (HCV) and hepatocellular carcinoma (HCC). Linkage disequilibrium between major SNPs at the HFE gene with HLA-A and HLA-B alleles may contribute to alterations in the function of immune cells. We sequenced the coding region of the HFE gene (exon 2, 3, 4 and 5) of patients exhibiting primary or secondary iron overload. Thus, we studied 130 patients with hepatitis C, 60 patients with HCC, 14 patients with HH and 100 healthy individuals. We observed seven SNPs in the HFE gene in 5 \'to 3\' sequence: i) H63D C>G at exon 2 (rs1799945); ii) IVS2(+4)T>C at intron 2 (rs2071303); iii) intron 3 C>G (rs807209); iv) C282Y G>A at exon 4 (rs1800562); v) intron 4 G>A (rs2794717); vi) IVS4(-44) T>C (rs1800708); vii) at intron 5 we detected a yet undescribed G>deletion. We performed haplotype reconstruction of the coding region and extended haplotypes comprising the HFE gene and ten other loci (HLA-A, HLA-B, HLA-C, HLA-DRB1, HLA-DQB1, TNFa, TNFb, TNFc, TNFd and HLA-G14bp). In addition, we normatized the nomenclature of the HFE gene, according to the rules of the International ImMunoGeneTics Information System - IMGT (http://www.imgt.org/). Several tools were used to evaluate the association between HFE polymorphic sites with iron overload, including tests assessing associations of alleles, genotypes, linkage disequilibrium, haplotype and diplotypes, diversity and neutrality tests. Finally, we compare the SNPs at the HFE gene observed in the healthy population with those observed in diverse worldwide populations available at the 1000genomes site (http://www.1000genomes.org/) the results showed that our population was closer to American and European populations, partially close the populations of African and distant of Asian populations. The C282Y allele G, contained in the coding region HFE * 01:03 haplotype, conferred susceptibility to HH in the Brazilian population tested, agreeing with the findings observed in other worldwide populations. The HFE*01:02:01:01/HFE* 01:01:01:05 dyplotype conferred susceptibility to the development of iron overload in patients with HCC caused by HCV. A strong linkage disequilibrium was detected between the H63D G and IVS2 (+4) C alleles in exon 2 of the HFE gene, and concomitantly, a linkage between these alleles with HLA-B*44, apparently not associated with iron overload, but with apparent historical origin. Finally, the test of diversity revealed differences only in the HH sample and the neutrality test detected no selective pressures on the control population of this study. In conclusion, this is the first study evaluating a large segment of the coding region of the HFE gene in several samples of patients exhibiting or not iron overload and in control subjects.

C Hepatitis

Carcinoma hepatocelular

Gene HFE

Haplótipo

Haplotype

Hemocromatose hereditária

Hepatite C

Hepatocellular Carcinoma

Hereditary hemochromatosis

HFE gene

Iron overload

SNPs

SNPs

Sobrecarga de ferro

Modelo experimental para indução de esteatose hepática e esteatohepatite: estudo em ratos / Experimental model for induction of steatosis and steatohepatitis - study in rats

Silva, Eliana Pinheiro da

29 October 2012

Introdução: A Doença Hepática Gordurosa Não Alcoólica (DHGNA) tem sido considerada atualmente a forma mais comum de doença hepática no mundo ocidental, relacionada principalmente ao aumento da prevalência da obesidade.A DHGNA abrange um largo espectro de doença, desde casos de esteatose simples (EH) até esteato-hepatite não alcoólica (EHNA) e fibrose, podendo evoluir para cirrose e carcinoma hepatocelular (CHC). Embora se conheçam os fatores predisponentes para o desenvolvimento de EHNA, sua patogênese, assim como tratamento eficaz, permanecem pouco conhecidos.Os lípides, principalmente gorduras neutras, fosfolipídios e colesterol, são componentes fundamentais das células, assim como as proteínas e os hidratos de carbono. Embora aumentos marcantes de proteínas e hidratos de carbono não produzam quaisquer alterações macroscópicas no fígado, um acúmulo de gordura é prontamente reconhecido pela coloração amarelada e pelo aumento de volume do órgão. Várias dietas tem sido usadas em animais de laboratórios, principalmente camundongos e ratos no sentido de induzir esteatose, esteatohepatite e fibrose hepática, embora nenhuma delas consiga reproduzir na totalidade os componentes essenciais da doença humana. Não encontramos em nenhum trabalho da literatura a utilização da dieta deficiente em colina e hiperlipídica (DCH), por nós utilizada. Objetivo: O objetivo deste estudo foi avaliar o efeito de uma dieta deficiente em colina e hiperlipídica (DCH) para desenvolver esteatose hepática, esteatohepatite e fibrose hepática no rato. Métodos: A doença hepática foi induzida em ratos Sprague-Dawley machos pesando de 300 a 350 gramas, hospedados em gaiolas padrão e recebendo água à vontade. Foi usado dieta deficiente em colina e hiperlipídica (DCH). Os animais foram distribuídos por meio de tabela sequencial randomizada em dois grupos. No grupo 1 dez ratos receberam a dieta por 4 meses e no grupo 2 dez ratos receberam a dieta durante 8 meses. Após o tempo estipulado das dietas os animais foram anestesiados e sacrificados. Os fígados dos animais foram retirados, pesados e enviados para estudo histopatológico de acordo com os critérios estabelecidos por Kleiner. Os animais foram pesados no início do experimento e por ocasião do sacrifício. Resultados: o peso dos animais do grupo 1 (DCH - 4 meses) no início do experimento variou de 305 a 350 gramas com média de 329,9 gramas e no fim do experimento de 529 a 615 gramas com média de 579,2 gramas. O percentual de ganho de peso dos animais variou de 60 a 86,93% com média de 75,72%. O peso dos animais do grupo 2 (DCH - 8 meses) no início do experimento variou de 320 a 353 gramas com média de 339,4 gramas e no fim do experimento variou de 661,5 a 783 gramas com média de 705,6 gramas. O percentual do ganho de peso dos animais variou de 95,58 a 123,71% com média de 107,78%. O peso do fígado dos animais do grupo 1 no fim do experimento variou de 24,5 a 29,5 gramas. O percentual do peso do fígado em relação ao peso dos animais do grupo 1 variou de 4,16 a 5,54% com média de 4,75%. O peso do fígado dos animais do grupo 2 no fim do experimento variou de 31 gramas a 39 gramas com média de 33,8 gramas. O percentual do peso do fígado em relação ao peso dos animais do grupo 2 variou de 4,63% a 5,07%, com média de 4,78%. A análise histopatológica dos animais do grupo 1 demonstrou intensa balonização e esteatose microgoticular com inflamação lobular; o estadiamento de fibrose foi discreto nestes animais. O estudo histopatológico dos animais do grupo 2 revelou intensa esteatose microgoticular e balonização com inflamação lobular; alguns animais apresentaram esteatose macrogoticular. Os animais deste grupo 2 apresentaram fibrose com grande variação individual. Os animais de ambos os grupos experimentais desenvolveram esteatohepatite, pois apresentaram o índice de atividade da doença hepática gordurosa não alcoólica (NAS)>=5. A análise comparativa demonstrou não haver diferença estatística no valor do NAS entre os dois grupos experimentais. Em relação ao estadiamento da fibrose na esteatohepatite não alcoólica, os animais do grupo 2 apresentaram uma tendência de escores mais elevados do que os animais do grupo 1. No entanto não houve diferença estatística entre os grupos devido a grande variação individual (p=0,2755). Conclusões: A dieta DCH administrada durante 4 e 8 meses induziu nos ratos aumento considerável de peso corpóreo e do peso do fígado. Os animais do grupo 1 apresentaram intensa balonização, esteatose microgoticular e inflamação lobular com discreta fibrose hepática. Os animais do grupo 2 apresentaram intensa balonização, esteatose macro e microgoticular, inflamação lobular e maior grau de fibrose hepática, bem estabelecida com formação de colágeno e expansão fibrosa nos espaços vasculares. A dieta deficiente em colina e hiperlipídica (DCH) induziu no rato esteatose hepática e esteatohepatite com fibrose, servindo de modelo experimental para proporcionar melhor entendimento para procedimentos terapêuticos futuros desta importante patologia do fígado. / Introduction: Nonalcoholic Fatty Liver Disease (NAFLD) has currently been regarded as the most common form of liver disease in the western world, mainly related to the increased prevalence of obesity. NAFLD covers a broad spectrum of diseases, since cases of simple steatosis (HS) to steatohepatitis (EHNA) and fibrosis, and may evolve to cirrhosis and hepatocellular carcinoma (CHC). Although the predisposing factors for the development of EHNA are well established, there is little knowledge on its pathogenesis as well as the effective treatment options. Lipids, especially phospholipids, neutral fats and cholesterol, are fundamental cell components, as well as proteins and carbohydrates. Although striking increases of proteins and carbohydrates do not produce liver macroscopic changes, fat build up can be rapidly recognized by the yellow coloring and increased organ volume. Many diets have been used in laboratory animals, mainly rats although none of them can fully reproduce the fundamental components of the human disease. We could not find in the literature any study on the use of choline-deficient and hiperlipidic diet (CHD), used in the present study. Goal: The objective of this study was to evaluate the effect of a cholinedeficient and hiperlipidic diet (CHD) on the development of steatosis, steatohepatitis and hepatic fibrosis in rats. Methods: The liver disease was induced in male Sprague-Dawley rats, weighing from 300 to 350 grams, hosted in standard cages and receiving water ad libitum and fed with a choline-deficient and hiperlipidic diet (CHD). The experimental animals were distributed by means of a random sequential table in two groups. In Group 1 ten rats received the diet for four months and in Group 2 ten rats received the same diet for eight months. After these predetermined feeding time periods the animals were anesthetized and sacrificed. The animal livers were then removed, weighed and sent to histopathological study according to the criteria established by Kleiner. All the animals were weighed at the beginning of the experiment and by the time of the sacrifice. Results: The weight of Group 1 animals (4 months CHD) at the beginning of the experiment varied from 305 to 350 grams with an average of 329.9 grams and at the end of the experiment from 529 to 615 grams averaging 579.2 grams. The percentage of weight gain in animals of this group ranged from 60% to 86.93% with an average of 75.72%. The weight of Group 2 animals (8 months CHD) at the start of the experiment varied from 320 to 353 grams with an average of 339.4 grams and at the end of the experiment from the 661.5 to 783 g with an average of 705.6 grams. The percentage of weight gain in animals of this group varied from 95.58% to 123.71%, averaging 107.78%. The liver weight of Group 1 animals at the end of the experiment varied from 24.5 to 29.5 grams. The percentage of liver weight in relation to the animals\' weight, in Group 1, ranged from 4.16% to 5.54%, with an average of 4.75%. The liver weight of Group 2 animals at the end of the experiment varied from 31gramas to 39 grams, with an average of 33.8 gram. The percentage of liver weight in relation to the animals\' weight, in Group 2, ranged from 4.63% to 5.07%, with an average of 4.78%. Liver histopathological analysis in Group 1 animals showed marked ballooning degeneration and microgoticular steatosis with lobular inflammation; fibrosis staging was discreet in these animals. Liver histopathological study in animals of Group 2 showed an intense microgoticular steatosis and ballooning with lobular inflammation; some animals of this group presented macrogoticular steatosis. The amount of hepatic fibrosis in animals of this group was extremely variable. Animals of both experimental groups developed steatohepatitis, as they presented the activity index of nonalcoholic fatty liver disease (NAS) >= 5. Statistical analysis did not show a significant difference between the NAS values of the two experimental groups. Fibrosis staging analysis in non-alcoholic steatohepatitis showed a trend toward higher scores in animals of Group 2 as compared to Group 1 animals. However there was no statistical difference between the groups due to a large individual variation (p = 0.2755). Conclusions: CHD diet administered for four and eight months induced considerable increases in the rats\' body weight and liver weight. Animals in Group 1 showed intense liver ballooning, steatosis and lobular inflammation with discrete microgoticular fibrosis. Animals in Group 2 presented intense ballooning, steatosis macro and microgoticular, lobular inflammation and a higher degree of well-established hepatic fibrosis, with collagen formation with fibrotic expansion in vascular spaces. Choline-deficient and hiperlipidic diet (CHD) in the rat induced hepatic steatosis and steatohepatitis with fibrosis, representing an experimental model, which can provide a better knowledge for future therapeutic procedures of this important liver pathology.

Carcinoma hepatocelular

Esteato hepatite

Fatty liver

Fibrose hepática

Fígado gorduroso

Hepatic fibrosis

Hepatocellular carcinoma

Ratos Sprague-Dawley

Sprague - Dawley rats

Steato hepatitis

Estudo da região promotora do gene do colágeno XVIII humano / Study of human collagen XVIII promoter region

Correa, Lucia Maria Armelin

29 June 2007

O colágeno XVIII é um componente das membranas basais com diversos domínios funcionais, como a endostatina e o domínio frizzled, que têm importante papel em processos celulares como proliferação e diferenciação. COL18A1 possui dois promotores alternativos: o promotor 1, que regula a síntese da variante NC11-303, e o promotor 2 responsável pelas variantes NC11- 728 e NC11-493, expressas por hepatócitos. Existe uma variação interindividual da endostatina circulante e da expressão do colágeno XVIII no fígado. A expressão do colágeno XVIII/endostatina foi correlacionada com a progressão tanto do hepatocarcinoma (HCC), quanto da fibrose/cirrose hepática. Elucidar a regulação da expressão de COL18A1 pode auxiliar na compreensão dessa variação interindividual e da progressão dessas doenças. Neste trabalho demos início a caracterização do promotor 2 do COL18A1. Identificamos na seqüência predita como promotora cinco regiões conservadas entre humanos e camundongos. A análise in silico e funcional dessas regiões revelou que os fatores de transcrição, Sp1, Sp3, YY1, Oct-1, C/EBP&#945; e C/EBP&#946;, interagem com as mesmas. Demonstramos que C/EBP&#946;&#61472;aumenta a taxa de transcrição do promotor 2 em hepatócitos, e que existe uma correlação positiva da expressão de NC11-493 com C/EBP&#945;&#61472;e C/EBP&#946;&#61472;em tecido hepático cirrótico e tumoral. As expressões de C/EBP&#945;&#61472;em tecido hepático cirrótico e tumoral estão diretamente correlacionadas, enquanto que os níveis de NC11-493 nos tumores estão inversamente correlacionados com o tamanho dos mesmos. Mostramos a existência de diversos SNPs no promotor 2. O SNP-700T/G, funcional in vitro, afeta a interação de Sp3 e YY1 com essa região regulatória. A deleção da região do SNP indicou que ela possui elementos importantes para a transcrição em hepatócitos, apesar deste SNP não estar relacionado com o nível de expressão do colágeno XVIII em fígado fibrótico ou com susceptibilidade a HCC. O SNP- 700T/G está em desequilíbrio de ligação com o SNPc.1135C/T, no domínio frizzled do colágeno XVIII. Não foi possível elucidar a funcionalidade do SNPs c.1135C/T in vitro, mas os haplótipos formados por esses dois SNPs têm diferentes frequências entre descendentes de europeus e de africanos. Nosso trabalho traz importantes contribuições e abre novas perspectivas para a compreensão da regulação do colágeno XVIII em fígado humano, tanto em situações fisiológicas, quanto em processos fibrogênicos e tumorigênicos¶ / Collagen XVIII is a basal membrane component with several funcional domains, such as endostatin and frizzled domains, which have important roles in cellular processes such as proliferation and differentiation. COL18A1 has two promoter regions: promoter 1, that regulates the synthesis of NC11-303 isoform, and promoter 2, localized in intron 2, responsible for NC11-728 and NC11-493 isoforms expressed by hepatocytes. There is a large interindividual variation in circulating endostatin and in collagen XVIII liver expression. Collagen XVIII/endostatin levels were correlated with hepatocellular carcinoma (HCC) progression, as well as liver fibrosis/cirrhosis, conditions that precede HCC. Elucidating the mechanisms that regulate COL18A1 expression in hepatocytes may help understanding its variation among individuals and liver disease stages, as well as contribute to new treatment strategies. In this work we began to characterize COL18A1 promoter region 2. We identified in the predicted promoter sequence five conserved regions between human and mouse. The in silico and functional analysis of these regions revealed that transcription factors Sp1, Sp3, YY1, Oct-1, C/EBP&#945; and C/EBP&#946; interact with them. We have demonstrated that C/EBP&#946; increases promoter 2 transcription rate in hepatocytes, and that there is a positive correlation of NC11-493 expression with that of C/EBP&#945; and C/EBP&#946; in cirrhotic and tumor liver samples. Non-tumor and tumor C/EBP&#945; expressions positively correlate between themselves, while NC11-493 tumor expression inversely correlates with tumor size. We also showed that there are several SNPs in COL18A1 promoter 2 region. SNP-700T/G, functional in vitro, affects Sp3 and YY1 interaction with the promoter 2 region and deletion of the SNP region indicated that this sequence has important hepatocyte regulatory elements. Our results suggest that this SNP does not significantly affects COL18A1 expression in fibrotic/cirrhotic liver and is not associated with HCC susceptibility. SNP-700T/G is in linkage disequilibrium with SNPc.1135C/T, at collagen XVIII frizzled domain. We could not elucidate SNPc.1135C/T functionality in vitro, but the haplotypes formed by these two SNPs have different frequencies in European and African descendants. In conclusion, our work brings important contributions and opens new perspectives for the comprehension of collagen XVIII regulation in human liver in physiological situations, as well as in fibrotic/cirrhotic and tumorigenic process.

Colágeno XVIII

Collagen XVIII

Fatores de transcrição

Fibrose/cirrose hepática

Hepatocarcinoma

Hepatocellular carcinoma

Liver fibrosis/cirrhosis

Polimorfismo de base única

Promoter Region

Região Promotora

Single Nucleotide Polymorphisms

Transcription factors