Trends and Determinants of Up-to-date Status with Colorectal Cancer Screening in Tennessee, 2002-2008

Veeranki, Sreenivas P., Zheng, Shimin

01 July 2014

BACKGROUND: Screening rates for colorectal cancer (CRC) are increasing nationwide including Tennessee (TN); however, their up-to-date status is unknown. The objective of this study is to determine the trends and characteristics of TN adults who are up-to-date status with CRC screening during 2002-2008. METHODS: We examined data from the TN Behavioral Risk Factor Surveillance System for 2002, 2004, 2006 and 2008 to estimate the proportion of respondents aged 50 years and above who were up-to-date status with CRC screening, defined as an annual home fecal occult blood test and/or sigmoidoscopy or colonoscopy in the past 5 years. We identified trends in up-to-status in all eligible respondents. Using multivariable logistic regression models, we delineated key characteristics of respondents who were up-to-date status. RESULTS: During 2002-2008, the proportion of respondents with up-to-date status for CRC screening increased from 49% in 2002- 55% in 2006 and then decreased to 46% in 2008. The screening rates were higher among adults aged 65-74 years, those with some college education, those with annual household income ≥$35,000 and those with health-care access. In 2008, the respondents who were not up-to-date status with CRC screening included those with no health-care coverage (adjusted odds ratio [OR] 0.46, 95% confidence interval [CI] 0.33-0.63), those aged 50-54 years (OR 0.62, 95% CI 0.46-0.82) and those with annual household income CONCLUSIONS: TN adults who are up-to-date status with CRC screening are increasing, but not across all socio-demographic subgroups. The results identified specific subgroups to be targeted by screening programs, along with continued efforts to educate public and providers about the importance of CRC screening.

colorectal cancer

tenncare

Tennessee

up-to-date screening status

Biostatistics and Epidemiology

Behavior and Behavior Mechanisms

Biostatistics

Epidemiology

Faktory ovlivňující odpověď kolorektálního karcinomu na chemoterapeutickou léčbu / The study of the factors affecting colorectal cancer chemotherapy

Dolníková, Alexandra

January 2019

Application of cytotoxic chemotherapy still remains the essential treatment strategy in advanced colorectal cancer. The intrinsic and acquired drug resistance represents one of the reasons that may even lead to failure of cancer therapy. The DNA damage response pathways have been shown to play an important role in the development of chemoresistance. There is sufficient evidence showing the high-frequency deregulated expression of many DNA repair genes across multiple cancer types. An example of such gene in colorectal cancer is MRE11, which encodes protein known as a sensor of DNA double-strand breaks. In year 2016, there was a substantial study published by our group at The Department of Molecular Biology of Cancer (IEM CAS, Prague), the study analysed the association of polymorphisms in predicted microRNA target sites of double-strand breaks (DSBs) repair genes, including MRE11, and clinical outcome and efficacy of chemotherapy in colorectal cancer. Our hypothesis, based on the mentioned study, is that specifically and exactly defined microRNAs with ability to regulate certain DNA repair proteins may not only affect the survival of colorectal cancer cells, but also the sensitivity to chemotherapy. In practical part of the submitted thesis we have identified miR-140 as a potential regulator of...

Novel insights into MACC1 transcriptional regulation for identifying small molecule MACC1 inhibitors to restrict colorectal cancer progression

Juneja, Manisha

09 October 2014

MACC1 wurde als prognostischer Biomarker für die Tumorprogression und das Metastasen-freie Überleben im KRK sowie in anderen soliden Tumoren beschrieben. Das Gen induziert Zellmotilität und Proliferation in Zellkultur sowie die Metastasierung im Mausmodell. Damit stellt MACC1 ein vielversprechendes Ziel für die Intervention bei Tumorprogression und –metastasierung und damit für die Behandlung von KRK-Patienten dar. Unser Ziel war es, die Transkription von MACC1 zu inhibieren. Hierfür identifizierten wir zunächst die Promoter-Region von MACC1 und untersuchten MACC1s transkriptionelles Regulationsnetzwerk. Durch ortsgerichtete Mutagenese, Chromatin Immunopräzipitation und Electrophoretic Mobility Shift Assay ermittelten wir, dass Transkriptionsfaktoren wie Ap-1, Sp1, C/EBPs und GIPC1 an den MACC1-Promoter binden und die Transkription des MACC1-Gens kontrollieren. Darüberhinaus konnten wir durch Hochdurchsatz-Screening die bisher ersten Inhibitoren gegen MACC1 identifizieren: Rottlerin und Lovastatin. Wir zeigten, dass diese spezifisch auf den endogenen MACC1-Promoter wirken, was eine zeit- und konzentrationsabhängige Reduktion der MACC1-Expression zur Folge hatte. Beide Inhibitoren begrenzten das Expressionsniveau von Sp1 und interferierten mit der Bindung von c-Jun mit dem MACC1-Promoter, was in einer Inhibition der MACC1-Transkription resultierte. Ferner führte die tägliche Behandlung von Xenograft-Mausmodellen mit Rottlerin zu einer Inhibition der MACC1-Expression im Primärtumor und einer damit einhergehenden Begrenzung des Tumorwachstums. Zusammenfassend lässt sich festhalten, dass in der vorliegenden Arbeit zum ersten Mal der MACC1-Promoter und seine transkriptionelle Regulation beleuchtet wurden. Die neuen Erkenntnisse wurden zur Identifizierung der ersten Inhibitoren gegen MACC1 genutzt. Zur Behandlung von KRK-Patienten mit einem hohen Risiko für MACC1-induzierte Metastasierung könnten diese Inhibitoren Potential für die klinische Anwendung beherbergen. / MACC1 has been reported as a prognostic biomarker for tumor progression and metastasis-free survival in CRC along with other solid tumors. It induces cell motility and proliferation in cell culture and metastasis in mouse models. Consequently, targeting MACC1 to intervene in tumor progression and metastasis formation holds a promising approach to treat CRC patients. We designed a strategy to inhibit MACC1 via targeting its transcription. We first identified MACC1 gene promoter by creating various promoter-luciferase constructs. We then established that transcription factors such as Ap-1, Sp1, C/EBPs and GIPC1 bind to the MACC1 promoter and govern MACC1 transcription, expression and thus motility in vitro and in CRC patients. Using a high throughput screening targeting the MACC1 promoter, we identified small molecule MACC1 inhibitors, Rottlerin and Lovastatin. These inhibitors specifically restricted endogenous MACC1 promoter leading to reduced MACC1 expression in a time- and concentration-dependent manner. In vitro functional assays demonstrated the impact of the small molecule inhibitors on retarding cell proliferation and motility. Both inhibitors restricted Sp1 levels and interfered with the binding of c-Jun to the MACC1 promoter, thereby inhibiting MACC1 transcription. The study further described the effect of Rottlerin on a CRC-xenografted mouse model. Daily treatment of xenografted mice with Rottlerin resulted in the inhibition of MACC1 expression in the primary tumor accompanied with the restricted tumor growth. To summarize, this is the first study unraveling the MACC1 promoter, its transcriptional regulation and identification of newly identified MACC1 inhibitors. In clinical settings, inhibition of MACC1 expression using these inhibitors might provide immense potential for the treatment of CRC patients who are at high risk for MACC1-induced metastasis linked to shorter survival.

MACC1

Kolorektales Karzinom

Metastase

Rottlerin

Lovastatin

Inhibitoren

Colorectal cancer

MACC1

Metastasis

Rottlerin

Lovastatin

Inhibitors

570 Biowissenschaften, Biologie

32 Biologie

XH 7200

ddc:570

Tumorantigen-gepulste dendritische Zellen zur Steigerung der Zytotoxizität immunologischer Effektorzellen bei Tumoren des gastroenteropankreatischen Systems

Märten, Angela

31 May 2000

Die Rationale für immuntherapeutische Ansätze zur Behandlung maligner Neoplasien geht davon aus, daß Tumore über spezifische Tumorantigene verfügen. Dendritische Zellen als die wichtigsten antigenpräsentierenden Zellen sind in der Lage, Tumorantigene naiven T-Zellen zu präsentieren und spezifische zytotoxische T-Zellen zu stimulieren. In der vorliegenden Arbeit wurden dendritische Zellen durch Stimulation mit Interleukin-4 (IL-4) und Granulozyten/ Makrophagen Koloniestimulierender Faktor (GM-CSF) aus peripheren mononukleären Blutzellen gesunder Spender und an Tumoren des gastroenteropankreatischen Systems erkrankter Patienten generiert. Mit den dendritischen Zellen cokultivierte immunologische Effektorzellen (Zytokin-induzierte Killerzellen, CIK-Zellen) wurden im Zytotoxizitätstest gegen kolorektale und pankreatische Karzinomzellen eingesetzt. CIK-Zellen sind zytototoxische Zellen, die durch Stimulation mit Zytokinen aus peripheren Blutlymphozyten erzeugt werden. Durch die Cokultivierung der Effektorzellen mit dendritischen Zellen konnte eine signifikante Steigerung der unspezifischen zytotoxischen Wirkung der CIK-Zellen bewirkt werden. Zur Steigerung der spezifischen Zytotoxizität wurden dendritische Zellen mit dem Gesamtprotein der tumor-assoziierten Antigene cancer associated antigen (CA 19-9) und carcinoembryonic antigen (CEA) gepulst. Effektorzellen zeigten nach der Cokultur mit gepulsten dendritischen Zellen zytotoxische Wirkung gegen Targetzellen, die das zum Pulsen verwendete Tumorantigen auf der Zelloberfläche exprimieren. Die Antigenspezifität der zytotoxischen Wirkung konnte durch eine signifikant verminderte Zellyse nach Blockade des Tumorantigens auf den Targetzellen belegt werden. Erstmals beschrieben ist hier das Pulsen dendritischer Zellen mit sowohl autologen als auch allogenen Seren von Patienten mit erhöhten Tumormarkerspiegeln. Eine Kultivierung dendritischer Zellen in tumormarkerhaltigem Serum bewirkte dosisabhängig eine verstärkte zytotoxische Wirkung cokultivierter Effektorzellen gegen Tumorzellen. Die verstärkte Zellyse zeigte sich unabhängig vom allogenem oder autologem Charakter des Serums. Der immunstimulierende Effekt des Patientenserums konnte durch eine vorhergehende Hitzeinaktivierung des Serums neutralisiert werden. Die höchsten Zellysen wurden durch eine Kultivierung dendritischer Zellen in tumormarkerhaltigem Serum und zusätzlichem Pulsen mit exogenem Tumorantigen erreicht. Unte rsuchungen an komplett autologen Systemen reproduzierten die an Zellkulturen erhobenen Befunde. Hierfür wurden erfolgreich Primärkulturen kolorektaler Tumore etabliert. Aus dem Blut von Tumorpatienten wurden dendritische Zellen generiert, die mit autologem Serum kultiviert wurden. Die cokultivierten autologen Effektorzellen erwiesen sich im Zytotoxizitätstest gegen autologe Tumorzellen als zytotoxisch. Die Cokultivierung der Effektorzellen mit den dendritischen Zellen bewirkte bei beiden Zellpopulationen Veränderungen. Dendritische Zellen zeigten nach der Cokultur eine verstärkte Expression antigenpräsentierender und costimulatorischer Moleküle. Bei den CIK-Zellen kam es zu einem Anstieg der Proliferationsrate. Bei Untersuchungen zur Antigenspezifität von T-Zellrezeptoren konnte vermehrt antigenspezifischer T-Zellrezeptor nachgewiesen werden. Des weiteren stieg das Verhältnis zwischen zytotoxischen T-Zellen und T-Helferzellen zugunsten der zytotoxischen T-Zellen. In ELISpot-Untersuchungen wurde eine Zunahme Interferon-gamma sezernierender CIK-Zellen nachgewiesen. Dendritische Zellen ließen sich erfolgreich mit inaktiviertem Adenovirus, an das kovalent Poly-L-Lysin gekoppelt ist, transfizieren. Die für den adenoviralen Gentransfer benötigten Oberflächenstrukturen konnten auf dendritischen Zellen nachgewiesen werden. Zur Verbesserung der Zytotoxizität wurden dendritische Zellen erfolgreich mit dem Gen für den Transaktivator CIITA transfiziert. CIITA- transfizierte dendritische Zellen exprimierten vermehrt MHC Klasse II-Moleküle. Die transduzierten dendritischen Zellen induzierten bei cokultivierten Effektorzellen eine erhöhte unspezifische Zytotoxizität. Mit Tumorantigen gepulste dendritische Zellen können bei der Entwicklung immuntherapeutischer Protokolle bei malignen Neoplasien von Bedeutung sein. / The immunotherapeutic approach against malignant neoplasias appreciates that tumours encode tumour rejection antigens, that enable them to induce protective immunity. Dendritic cells are major antigen-presenting cells and are able to present tumour antigens to naive T-cells and stimulate cytotoxic T-cells in a specific manner. In the present graduation-manuscript dendritic cells were generated in the presence of Interleukin-4 and granulocyte/macrophage colony-stimulating factor (GM-CSF) from peripheral mononuclear blood cells of healthy donors and tumour- patients. Immunological effector cells termed cytokine- induced killer cells (CIK cells) were co-cultured with dendritic cells and tested for their cytotoxic capacity against colorectal and pancreatic cancer cell-lines in a LDH-release assay. CIK cells are cytotoxic lymphocytes generated by incubation of peripheral blood lymphocytes with different cytokines. Co-culture of effector cells with dendritic cells led to a significant increase of the cytotoxic effect of CIK cells. For a further increase of specific cytotoxicity dendritic cells were pulsed with total protein of the tumour-associated antigens cancer associated antigen CA 19-9 and carcinoembryonic antigen (CEA). Co-cultured effector cells showed an increase in cytotoxicity against tumour-antigen expressing target cells, after co-culture with pulsed dendritic cells. The specificity of the cytotoxic effect could be shown by blocking the tumour-antigens with a monoclonal antibody. Autologous and allogenec untreated serums from patients with elevated tumour-marker levels were also used for pulsing of dendritic cells. Similar to the results when using total protein for pulsing, a cultivation in serum of patients with elevated tumour marker levels caused an intensified cytotoxic effect of effector cells against tumour cells in a dose-dependent manner. The intensified cytotoxicity was seen independent of the allogenec or autologous character of the serum. The immuno-stimulating effect of the patient serum could be neutralized by preceding heat inactivating. The highest cytotoxicity was achieved by a cultivation of dendritic cells in serum from patients with elevated tumour marker levels and additional pulsing with exogenous tumour antigen. Experiments with completely autologous systems reproduced the results made with cell-lines. Primary cultures of colorectal tumours were established. Dendritic cells were generated from the blood of tumour patients and were cultivated in autologous serum. Co-cultured autologous effector cells showed cytotoxicity when used against autologous tumour cells. Co-culturing of effector cells with dendritic cells caused modifications at both cell populations. Dendritic cells showed an increase expression of antigen-presenting and co-stimulatory molecules. CIK cells showed a higher proliferation-rate when co-cultured. They express more antigen-specific T-cell receptor, and the cytotoxic T-cells to T-helper cells ratio increased. ELISpot-assays showed an increase of interferon gamma producing cells. Dendritic cells were successfully transduced by using an inactivated adenovirus, which covalently binds poly-L- lysine. Dendritic cells express the molecules that enables adenoviral gene delivery on their surface. For the improvement of cytotoxicity dendritic cells were transduced with the gene encoding for the transactivator CIITA. CIITA transduced dendritic cells increases expression of MHC class II molecules. Cytotoxicity experiments with transduced dendritic cells resulted in an increased induction of non-specific cytolysis from co-cultured effector cells. DC pulsed with tumour-antigens may have a major impact on immunotherapeutic protocols for cancer patients.

Immuntherapie

Gastrointestinale Tumore

Dendritische Zellen

CIITA

Immunotherapy

colorectal cancer

dendritic cells

CIITA

570 Biowissenschaften, Biologie

32 Biologie

XH 7100

ddc:570

Mutated in colorectal cancer (MCC): a putative tumour suppressor gene in colorectal cancer

Sigglekow, Nicholas David, Garvan Institute of Medical Research, Faculty of Medicine, UNSW

January 2009

Colorectal cancer (CRC) remains a significant burden in contemporary society due to an aging population, unhealthy dietary choices and an increasingly sedentary lifestyle. While the underlying defects for many hereditary forms of CRC have been determined, many genetic and epigenetic changes promoting common sporadic CRCs have yet to be identified. The Mutated in Colorectal Cancer (MCC) gene, identified in 1991, was initially thought to be responsible for the hereditary form of CRC, familial adenomatous polyposis, before the discovery of the susceptibility gene Adenomatous Polyposis Coli (APC), which then became the focus of intense research. Recent data, however, suggests that MCC may also be important in the development of CRC. I have investigated the mechanism of MCC gene silencing, the putative structure, and multiple functions of MCC. MCC was frequently silenced by promoter hypermethylation in CRC cell lines and primary tumours. MCC methylation showed strong molecular and clinicopathological associations with hallmarks of the serrated neoplasia pathway. Furthermore, MCC methylation was more frequent in serrated precursor lesions compared with adenomas, thus occurring early during carcinogenesis. MCC is highly conserved in complex multicellular organisms. Re-introduction of MCC in CRC cell lines resulted in partial G1 to S phase, and G2/M phase cell cycle blocks, potentially by upregulating cell cycle inhibitor gene transcription and interfering with the process of mitotic checkpoints and division, respectively. Changes in MCC levels also modulated NF?B pathway signalling, the pathway required for maintaining cell viability and proliferation in colonic epithelial cells. In particular, MCC overexpression suppressed both TNF? and LPS-induced NF?B activation, decreasing both the magnitude and rate of cellular responses. Overexpression also resulted in downregulation of proteins involved in canonical NF?B pathway signalling, while increasing the transcription of non-canonical NF?B genes. Therefore, MCC may direct activation of this pathway to a specific subset of NF?B-regulated genes. These data provide a molecular basis for the role of MCC as a tumour suppressor gene in CRC. MCC may have multiple functions, regulating cell cycle progression and modulating NF?B pathway signalling, either through direct involvement in pathway signalling cascades, or by providing a scaffold on which signalling events can occur.

Tumour suppressor.

Mutated in colorectal cancer.

MCC.

Promoter hypermethylation.

Colon cancer.

NF-kappaB.

Cell cycle.

G1/S block.

G2/M block.

Serrated neoplasia pathway.

Optimisation of Chemotherapy Treatment in Advanced Colorectal Cancer

Berglund, Åke

January 2002

<p>Colorectal cancer is one of the most common malignant diseases in Sweden – more than 5000 new cases are diagnosed each year. The overall five-year survival is about 60% and in cases of recurrence the prognosis is poor.</p><p>In a phase III study in advanced colorectal cancer the response rate was doubled when 5-FU was given as a bolus injection versus as a short infusion. The toxicity was similar and time to progression was longer in the injection group. However, overall survival was not significantly different. Dose-effect relationships of 5-FU were studied in another phase III study recruiting 312 patients. A decrease from 500 mg/m² to 400 mg/m² worsened the treatment results. A low incidence of severe toxicity was seen in both groups. An increase to 600 mg/m² worsened the toxicity without any improvement of the results.</p><p>A cytotoxic drug sensitivity test in different tumour types, mainly gastrointestinal cancer, poorly predicted treatment outcome in a phase II study.</p><p>The conventional Nordic Flv regimen was split in a phase I/II trial. An escalation of dose was possible and the response rate was 20%.</p><p>Thymidylate synthase (TS) and the gene expression of p53 were investigated by immunohistochemical technique in the primary tumours of 132 patients. None of the markers predicted the later palliative chemotherapy result. However, TS significantly predicted time to recurrence.</p><p>Serum markers were analysed before and during FLv treatment to early predict outcomes among 87 patients. TPS is promising, both as a predictive marker before start of treatment and after a short period of treatment. In the same setting, CEA had lower predictive value. S-VEGF and S-bFGF did not yield any prognostic information of later outcome. In all studies B-haemoglobin values, performance status and subjective response were strong markers, both for prediction of objective response and for survival.</p>

Oncology

Colorectal cancer

chemotherapy

5-fluorouracil

dose-effect relationship

ex vivo assay

thymidylate synthase

p53

CEA

TPS

VEGF

bFGF.

Onkologi

Oncology

Onkologi

Untersuchungen zur chemischen Transformation von intestinalen Epithelzellen der Ratte und des Menschen durch 2-Hydroxyamino-1-methyl-6-phenylimidazo(4,5-b)pyridin / Investigations to chemical transformation of rat and human intestinal epithelial cells by 2-hydroxyamino-1-methyl-6-phenylimidazo(4,5-b)pyridine

Fuchs, Iris Judith

January 2006

Die Zahl der Kolonkarzinome in den westlichen Industrieländern steigt in den letzten Jahren stetig an. Zu den Verbindungen, die mit der Zubereitung der Nahrung entstehen, mit ihr aufgenommen werden und die Kolonkanzerogenese möglicherweise begünstigen, gehört das heterozyklische aromatische PhIP, das bei der Erhitzung proteinreicher Nahrungsmittel entsteht. Neben zahlreichen Fütterungsversuchen an Nagern existieren auch Zellkulturmodelle zur Untersuchung der molekularen Mechanismen der PhIP-induzierten Kolonkanzerogenese. Die chemische Transformation von Zellen sollte durch wiederholte Exposition gegenüber dem hydroxylierten Metaboliten des Kanzerogens (N2-OH-PhIP) erzielt werden. Es wurden IEC-18-Zellen der Ratte und HCEC-Zellen des Menschen zur Untersuchung verwendet. Die Behandlung der IEC-18-Zellen führt nach 25 Behandlungszyklen mit Konzentrationen von 5 bis 20 µM nicht zur Transformation der Zellen. Die Anwesenheit von N2-OH-PhIP führt zu einer zehnfach erhöhten Induktion der GST-Aktivität, insbesondere der Untereinheiten GST-A1, -A3, -Pi und -T2, die für die effiziente Detoxifizierung des N-Acetoxy-Metaboliten vom N2-OH-PhIP verantwortlich sind. Bereits nach drei Behandlungen mit 1,5 µM N2-OH-PhIP konnte eine maligne Transformation der HCEC-Zellen erzielt werden. Die Zellen zeigten die charakteristischen Zeichen der Transformation: veränderte Wachstumseigenschaften wie klonales dreidimensionales Zellwachstum („pilling up“), Hemmung der Zell-Zell-Kontaktinhibierung, verkürzte Populationsverdopplungszeiten und tumorigene und metastasierende Eigenschaften. Außerdem exprimierten die N2-OH-PhIP-exponierten humanen Kolonzellen mit steigender Anzahl der Behandlungen größere Mengen des trunkierten APC-Proteins. Die bekannten PhIP-spezifischen Mutationen im APC-Gen resultieren in der Expression eines trunkierten Proteinproduktes und werden als frühe Ereignisse in der Kolonkanzerogenese betrachtet. Die zusammenfassende Betrachtung aller Ergebnisse zeigt, dass die IEC-18-Zelllinie zur chemischen Transformation durch N2-OH-PhIP ungeeignet ist. Dagegen wurde erstmalig eine vollständige chemische Transformation von Humandickdarmepithelzellen in vitro durch Exposition der humanen Kolonepithelzelllinie HCEC gegenüber dem Kolonkarzinogen N2-OH-PhIP erzielt. / In the last few years a strong increase in the incidence of colorectal cancer has been observed. As to the specific components in processed food responsible for the induction of colon cancerogenesis / it has been suggested that heterocyclic aromatic amines (HAA), e.g. the most abundant HAA 2-amino-1-methyl-6-phenylimidazo[4,5-b]pyridine (PhIP), which is formed in protein rich food, when it is cooked at high temperatures or over an open flame, might be involved in this process. Whereas a number of in vivo-models to study PhIP-mediated colon carcinogenesis are known, only a limited number of cell culture systems to study the HAA-mediated transformation of intestinal epithelial cells do in fact exist. In the present study IEC-18 cells (rat intestinal epithelial cells) and HCEC cells (human colon epithelial cells) were incubated with N2-OH-PhIP, the N-hydroxylated metabolite of PhIP. The IEC-18 cells could not be transformed despite 25 treatment cycles with 5 to 20 µM N2-OH-PhIP. This might be due to the fact that GST activity as well as the expression of the GST -A1, -A3, -Pi and -T2 units, which are responsible for the detoxication of the N-acetoxy derivative of PhIP were strongly induced by N2-OH-PhIP. In contrast, HCEC cells were malignantly transformed when exposed three times to 1.5 µM N2-OH-PhIP. The chemically-treated cells showed a reduced population doubling time, they lost cell-cell contact inhibition and started pilling up. Furthermore, if HCEC cells were injected subcutaneously into SCID mice tumors developed at the site of injection in all animals tested. The transformed HCEC cells also express high amounts of truncated APC protein, which in vivo appears at an early stage of colon cancerogenesis. Taken together, it has been shown that IEC-18 cells are not suitable for chemical transformation studies with the HAA metabolite N2-OH-PhIP. For the first time it has been shown that the HAA metabolite N2-OH-PhIP is indeed able to malignantly transform human colon epithelial cells in vitro.

maligne Transformation

Kolonkrebs

heterozyklische aromatische Amine

intestinale Epithelzellen

colorectal cancer

heterocyclic aromatic amines

intestinal epithelial cells

malignant transformation

Natural sciences and mathematics

Optimisation of Chemotherapy Treatment in Advanced Colorectal Cancer

Berglund, Åke

January 2002

Colorectal cancer is one of the most common malignant diseases in Sweden – more than 5000 new cases are diagnosed each year. The overall five-year survival is about 60% and in cases of recurrence the prognosis is poor. In a phase III study in advanced colorectal cancer the response rate was doubled when 5-FU was given as a bolus injection versus as a short infusion. The toxicity was similar and time to progression was longer in the injection group. However, overall survival was not significantly different. Dose-effect relationships of 5-FU were studied in another phase III study recruiting 312 patients. A decrease from 500 mg/m2 to 400 mg/m2 worsened the treatment results. A low incidence of severe toxicity was seen in both groups. An increase to 600 mg/m2 worsened the toxicity without any improvement of the results. A cytotoxic drug sensitivity test in different tumour types, mainly gastrointestinal cancer, poorly predicted treatment outcome in a phase II study. The conventional Nordic Flv regimen was split in a phase I/II trial. An escalation of dose was possible and the response rate was 20%. Thymidylate synthase (TS) and the gene expression of p53 were investigated by immunohistochemical technique in the primary tumours of 132 patients. None of the markers predicted the later palliative chemotherapy result. However, TS significantly predicted time to recurrence. Serum markers were analysed before and during FLv treatment to early predict outcomes among 87 patients. TPS is promising, both as a predictive marker before start of treatment and after a short period of treatment. In the same setting, CEA had lower predictive value. S-VEGF and S-bFGF did not yield any prognostic information of later outcome. In all studies B-haemoglobin values, performance status and subjective response were strong markers, both for prediction of objective response and for survival.

Oncology

Colorectal cancer

chemotherapy

5-fluorouracil

dose-effect relationship

ex vivo assay

thymidylate synthase

p53

CEA

TPS

VEGF

bFGF.

Onkologi

Oncology

Onkologi

Genetic and epidemiological studies of hereditary colorectal cancer

Cederquist, Kristina

January 2005

Lynch syndrome (Hereditary Nonpolyposis Colorectal Cancer, HNPCC) is the most common hereditary syndrome predisposing to colorectal cancer, accounting for 1-3% of all colorectal cancer. This multi-organ cancer predisposition syndrome is caused by mutations in the mismatch repair (MMR) genes, especially MLH1 and MSH2, and to lesser extents MSH6 and PMS2, which lead to widespread genetic instability and thus microsatellite instability (MSI). Hereditary cancer often manifests in two or more tumours in a single individual; 35-40% of Lynch syndrome patients have synchronous or metachronous tumours of the two major Lynch syndrome-related cancers: colorectal and endometrial. The main purposes of the work underlying this thesis were to identify persons at risk of Lynch syndrome or other types of hereditary colorectal cancer, to estimate the cancer risks associated with these predispositions and to identify the underlying genetic causes. A population-based cohort of 78 persons with double primary colorectal or colorectal and endometrial cancer was identified. Cancer risks in their 649 first-degree relatives were estimated in relation to tumour MSI status (positive or negative) and age at diagnosis (before or after 50 years of age) in the probands. The overall standardised incidence ratio was 1.69 (95% CI; 1.39-2.03). The highest risks for Lynch syndrome-associated cancers: (colorectal, endometrial, ovarian and gastric) were found in families with young MSI-positive probands, likely representing Lynch syndrome families. Importantly, no overall risk was found in families with old probands, irrespective of MSI status. Blood samples were available from 24 MSI-positive patients for mutation screening of MLH1, MSH2 and MSH6. Sequence variants or rearrangements predicted to affect protein function were found in 16 patients. Six novel variants were found: two large rearrangements, two truncating and two missense mutations. The missense mutations were found to segregate in the families. Studies of allele frequencies, MSI and loss of immunostaning in tumours from family members further supports the hypothesis that these missense changes play a role in Lynch syndrome, as do the non-conservative nature and evolutionary conservation of the amino acid exchanges. Five families had mutations in MLH1, five in MSH2, and six in MSH6. The unexpectedly large impact of MSH6 was in genealogical studies shown to be due to a founder effect. Cumulative risk studies showed that the MSH6 families, despite their late age of onset, have a high lifetime risk for all Lynch syndrome-related cancers, significantly higher in women (89% by age 80 years) than in men (69%). The gender differences are in part due to high endometrial (70%) and ovarian cancer risk (33%) in addition to the high colorectal cancer risk (60%). These findings are of great importance for counselling and surveillance of families with MSH6 mutations. Finally, in a large family with MSI-negative hereditary colorectal cancer for which the MMR genes and APC had been excluded as possible causes, a genome-wide linkage analysis was performed, resulting in a suggested linkage to chromosome 7. Conclusions: Relatives of probands with MSI-positive, double primary colorectal and endometrial cancer diagnosed before the age of 50 years have significantly increased risks of Lynch syndrome-related cancers. MSH6 mutations, which have unusually high impact in this study population due to a founder effect, confer high cumulative risks of cancer despite the generally late age of onset.

Genetics

Lynch syndrome

HNPCC

colorectal cancer

endometrial cancer

cancer risk

MSI

MLH1

MSH2

MSH6

genome-wide scan

Genetik

Clinical genetics

Klinisk genetik

Διερεύνηση μοριακών προγνωστικών παραγόντων στον καρκίνο του παχέος εντέρου

Γρίβας, Πέτρος

14 December 2009

Ο καρκίνος του παχέος εντέρου αποτελεί ένα από τα συχνότερα κακοήθη νεοπλάσματα παγκοσμίως, προκαλώντας σημαντική νοσηρότητα και θνητότητα. Η συστηματική διερεύνηση της παθογένειας συντελεί σημαντικά στην πρόληψη, έγκαιρη διάγνωση, θεραπεία και πρόγνωση της νόσου. Στην εποχή της μοριακής ιατρικής, η κατανόηση των μοριακών μηχανισμών καρκινογένεσης έχει αναδείξει το ρόλο ενδοκυττάριων σηματοδοτικών μονοπατιών, τα οποία ρυθμίζουν κυτταρικές διαδικασίες, όπως πολλαπλασιασμός, διαφοροποίηση, απόπτωση, αγγειογένεση, διήθηση. Κομβικά συστατικά τέτοιων μοριακών δικτύων αποτελούν οι υποδοχείς αυξητικών παραγόντων, όπως ο Human Εpidermal Receptor-1 (ΗΕR-1/EGFR), ο ρόλος του οποίου έχει τεκμηριωθεί στο αδενοκαρκίνωμα παχέος εντέρου, επιτείνοντας το ενδιαφέρον στη διευκρίνηση του ρόλου γειτονικών υποδοχέων, όπως του Human Εpidermal Receptor-3 (HER-3). O HER-3 συνιστά μεμβρανικό υποδοχέα που συμμετέχει σε μοριακά μονοπάτια ενδοκυτταρικής σηματοδότησης. Επομένως, ποσοτικές μεταβολές στην έκφρασή του αλλά και ποιοτικές αλλαγές στη δομή του, συντελούν δυνητικά στην κυτταρική εξαλλαγή. Τα δεδομένα από τη μελέτη του HER-3 στο αδενοκαρκίνωμα παχέος εντέρου είναι περιορισμένα και ο ρόλος του στην παθογένεια, πρόγνωση και θεραπεία της νόσου παραμένει ασαφής. Αντίστοιχα με τους μεμβρανικούς υποδοχείς, πυρηνικοί υποδοχείς ενέχονται σε διαδικασίες ρύθμισης γονιδιακής έκφρασης. Οι οιστρογονικοί υποδοχείς (ER) α και β διαμεσολαβούν την επίδραση των οιστρογόνων σε κυτταρικό επίπεδο, μεταποιώντας τα επίπεδα των ορμονών σε μεταβολές γονιδιακής έκφρασης. Οι διαφορές στην επίπτωση του καρκίνου του παχέος εντέρου ανάμεσα στα δύο φύλα καθώς και πρόσφατα βιβλιογραφικά δεδομένα έχουν αναδείξει τη σημασία της έκφρασης αυτών των υποδοχέων στην καρκινογένεση του παχέος έντερου. Παράλληλα, η εξειδίκευση της οιστρογονικής δράσης σε επίπεδο ιστού και κυττάρου εξασφαλίζεται μέσω της δράσης συγκεκριμένων συμπαραγόντων (ενεργοποιητών/καταστολέων). Αυτές οι πρωτεΐνες είναι ειδικοί μεταγραφικοί παράγοντες, οι οποίοι συνδεόμενοι με τους οιστρογονικούς αλλά και άλλους υποδοχείς «εξατομικεύουν» την ορμονική επίδραση στο γονιδίωμα. Ο proline-, glutamic acid-, and leucine-rich protein 1 (PELP1), γνωστός και ως modulator of non-genomic activity of ER (MNAR), ο amplified in breast cancer-1 (AIB1) και ο transcriptional intermediary factor-2 (TIF2) είναι σημαντικοί συμπαράγοντες οιστρογονικών υποδοχέων, με συνέπεια η μελέτη τους να αποτελεί αναπόσπαστο μέρος της διερεύνησης οιστρογονο-εξαρτώμενων μηχανισμών. Η συνεχής αλληλεπίδραση HER- και ER-εξαρτώμενων μονοπατιών έχει περιγραφεί σε ποικίλλους ιστούς. Σκοπός της παρούσας μελέτης είναι η διερεύνηση του ρόλου της (υπερ)έκφρασης του μεμβρανικού υποδοχέα HER-3, των οιστρογονικών υποδοχέων (ER) και των συμπαραγόντων PELP1/MNAR, AIB-1 και TIF-2 στον καρκίνο του παχέος εντέρου. Υλικά και μέθοδοι Στην παρούσα μελέτη χρησιμοποιήθηκαν ιστικά δείγματα, μονιμοποιημένα σε φορμόλη και εκλεισμένα σε παραφίνη από 140 ασθενείς με αδενοκαρκίνωμα παχέος εντέρου. Η έκφραση των επιπέδων HER-3 mRNA εκτιμήθηκε με τη μέθοδο της ποσοτικής αλυσιδωτής αντίδρασης πολυμεράσης (RT-PCR) σε 54 αδενοκαρκινώματα και 29 δείγματα φυσιολογικού βλεννογόνου. Η έκφραση των επιπέδων της φωσφορυλιωμένης (pHER-3) και μη φωσφορυλιωμένης HER-3 πρωτείνης εκτιμήθηκε με τη μέθοδο της ανοσοιστοχημείας σε 110 δείγματα φυσιολογικού βλεννογόνου, 24 αδενώματα και 140 αδενοκαρκινώματα. Η έκφραση των επιπέδων του οιστρογονικού υποδοχέα α και β και του PELP1/ΜΝΑR εκτιμήθηκε με τη μέθοδο της ανοσοιστοχημείας σε 113 αδενοκαρκινώματα, 30 αδενώματα και 88 δείγματα φυσιολογικού βλεννογόνου. Αντίστοιχα η έκφραση των επιπέδων του ΑΙΒ1 και TIF-2 εκτιμήθηκε με τη μέθοδο της ανοσοιστοχημείας σε 110 αδενοκαρκινώματα, 30 αδενώματα και 83 δείγματα φυσιολογικού βλεννογόνου. Αποτελέσματα Η πρωτεΐνη HER-3 εκφράζεται στο κυτταρόπλασμα και στον πυρήνα επιθηλιακών κυττάρων παχέος εντέρου σε φυσιολογικό βλεννογόνο, αδενώματα και αδενοκαρκινώματα και φαίνεται να μεταβάλλεται τοπογραφικά (από τον πυρήνα στο κυτταρόπλασμα) κατά τη διαδικασία της καρκινογένεσης. Ωστόσο, η έκφραση της πρωτεΐνης HER-3 σε αδενοκαρκινώματα δε φαίνεται να συσχετίζεται σημαντικά με τις κλινικοπαθολογικές παραμέτρους της νόσου. Η φωσφορυλιωμένη μορφή της πρωτεΐνης HER-3 (pHER-3) εκφράζεται στον πυρήνα και τη μεμβράνη επιθηλιακών και λείων μυικών κυττάρων παχέος εντέρου σε φυσιολογικό βλεννογόνο, αδενώματα και αδενοκαρκινώματα. Η πυρηνική έκφραση pHER-3 δε διαφέρει σημαντικά ανάμεσα σε φυσιολογικό βλεννογόνο, αδενώματα και αδενοκαρκινώματα. Ωστόσο, αυξημένα επίπεδα πυρηνικής έκφρασης pHER-3 συσχετίζονται σημαντικά με μεγαλύτερο στάδιο της νόσου, χωρίς να συσχετίζονται με τα επίπεδα έκφρασης της μη φωσφορυλιωμένης μορφής. Τα επίπεδα έκφρασης του γονιδίου ΗER-3 δε φαίνεται να αυξάνουν σημαντικά κατά την καρκινογένεση. Ωστόσο, αυξημένα επίπεδα HER-3 mRNA στα αδενοκαρκινώματα σχετίζονται με μεγαλύτερη ηλικία των ασθενών, εντόπιση του όγκου στο αριστερό κόλον και το ορθό και με λεμφαδενική διήθηση. Επίσης, συχετίστηκαν με αυξημένη πιθανότητα υποτροπής της νόσου και μειωμένο χρονικό διάστημα ως την υποτροπή. Ο ERα εκφράζεται σπάνια στο παχύ έντερο σε αντίθεση με τον ERβ, ο οποίος εκφράζεται συχνά στον πυρήνα επιθηλιακών αλλά και στρωματικών κυττάρων. Η έκφραση της πρωτεΐνης ERβ καθίσταται πιο έντονη κατά τη διάρκεια της καρκινογένεσης σε άνδρες, και στα αδενοκαρκινώματα συσχετίζεται με την πιθανότητα υποτροπής της νόσου. Ο συμπαράγοντας PELP1/MNAR ανιχνεύεται στον πυρήνα επιθηλιακών αλλά και στρωματικών κυττάρων του παχέος εντέρου και η έκφρασή του αυξάνει κατά την καρκινογένεση και στα αδενοκαρκινώματα συσχετίζεται με την έκφραση του ERβ. Ωστόσο, η υπερέκφραση του PELP1/MNAR στα ERβ θετικά αδενοκαρκινώματα συσχετίζεται με μεγαλύτερη συνολική επιβίωση των ασθενών. Ο AIB1 και ο TIF2 ανιχνεύονται στον πυρήνα επιθηλιακών αλλά και στρωματικών κυττάρων του παχέος εντέρου. Η έκφραση του ΑΙΒ1 αυξάνει κατά την καρκινογένεση και συσχετίζεται με τοπική ανάπτυξη του όγκου. Ωστόσο, στην πολυπαραγοντική ανάλυση ο ΑΙΒ1 αναδεικνύεται ως ανεξάρτητος ευνοϊκός προγνωστικός παράγοντας ως προς τη συνολική επιβίωση. Η έκφραση του ΤΙF2 αυξάνει κατά την καρκινογένεση και στα αδενοκαρκινώματα συσχετίζεται με την έκφραση του AIB1. Ωστόσο, η έκφρασή του στα αδενοκαρκινώματα δε σχετίζεται με κλινικοπαθολογικές παραμέτρους της νόσου. Το πρότυπο έκφρασης των συμπαραγόντων AIB1 και TIF2 δε σχετίζεται σημαντικά με εκείνο του ERβ. Συζήτηση-συμπεράσματα-προοπτικές Η παρούσα μελέτη αναδεικνύει τη σημασία της έκφρασης και φωσφορυλίωσης του ΗΕR3 στην καρκινογένεση του παχέος εντέρου, υποστηρίζοντας τον πιθανό ρόλο τους στην πρόγνωση της νόσου. Τα ευρήματα της μελέτης συμφωνούν με συγκεκριμένα βιβλιογραφικά δεδομένα ως προς τη συχνότητα ανίχνευσης του υποδοχέα στον παχύ έντερο, ενώ είναι η πρώτη η οποία αναδεικνύει τα επίπεδα HER-3 mRNA ως πιθανό προγνωστικό βιοδείκτη. Η διερεύνηση της έκφρασης του οιστρογονικού υποδοχέα β (ERβ1) ανέδειξε αύξηση των επιπέδων του κατά την καρκινογένεση, εύρημα που βρίσκεται σε συμφωνία με μερικά και σε αντιδιαστολή με άλλα βιβλιογραφικά δεδομένα. Η προγνωστική σημασία της έκφρασης των πυρηνικών υποδοχέων εξαρτάται από ποικίλους παράγοντες, όπως τα επίπεδα ειδικών συμπαραγόντων, ομοιοπολικές τροποποιήσεις, την τοπογραφία τους μέσα στο κύτταρο και τα επίπεδα συγκεκριμένων συγκεντρώσεων προσδέτη/ορμόνης. Η αύξηση των επιπέδων των συμπαραγόντων του οιστρογονικού υποδοχέα PELP1/MNAR, ΑΙΒ1 και ΤΙF2 κατά την καρκινογένεση υποδηλώνει πιθανή συμμετοχή τους σε οιστρογονοεξαρτώμενη ογκογόνο σηματοδότηση. Ωστόσο, η απουσία ισχυρής συσχέτισης ανάμεσα στα επίπεδα έκφρασής τους και στα επίπεδα έκφρασης του οιστρογονικού υποδοχέα (ERβ1) υπογραμμίζει την πλειοτροπική τους δράση και τον επιπρόσθετο ρόλο τους σε οιστρογονο-ανεξάρτητη ενδοκυττάρια σηματοδότηση. Περισσότερες μελέτες σε μεγάλο αριθμό ασθενών, κατάλληλα σχεδιασμένες και εκτελεσμένες, με τη χρήση ευαίσθητων και ειδικών πειραματικών τεχνικών καθώς και μεθόδων στατιστικής ανάλυσης απαιτούνται για την επιβεβαίωση των ευρημάτων της παρούσας μελέτης. Στην εποχή της μεταγονιδιωματικής ιατρικής, η αναζήτηση χρήσιμων μοριακών βιοδεικτών δύναται να συντελέσει στη βελτίωση της πρόγνωσης και της ποιότητας ζωής των ασθενών με καρκίνο του παχέος εντέρου. / Colorectal cancer is a major cause of cancer-related morbidity and mortality in the western world and has a significant impact on the health care systems. The deep understanding of molecular mechanisms that underline cellular transformation and tumor progression leads to the identification of key-molecules that are appropriate targets for sophisticated therapy in cancer. One such targeted approach exploits the presence of specific biomarkers that could be considered essential for tumor development. The role of such a biomarker, Human Εpidermal Receptor-1 (ΗΕR-1/EGFR), has been established in the development of colorectal cancer, suggesting the potential involvement of neighboring receptors, such as Human Εpidermal Receptor-3 (HER-3). HER-3 is a membranic receptor implicated in intracellular cell proliferation signaling. Thus, quantitative modifications in its expression and/or qualitative changes in its structure may contribute to cellular malignant transformation. The significance of HER3 expression, localization and phosphorylation remains elusive and data regarding its role in the pathogenesis, diagnosis, prognosis and management of colorectal cancer is limited. Apart from their mebranic counterparts, nuclear receptors are implicated in the regulation of gene transcription. Estrogen receptors (ER) α and β mediate the estrogen actions in the subcellular microenvironment. Differences in the incidence of colorectal cancer in the two genders have underlined the significance of ER expression in colorectal carcinogenesis. The specificity of estrogen activities in various cell types is mediated by the presence of tissue-specific coregulators (coactivators/corepressors). These proteins are specific transcription factors that bind to nuclear receptors, orchestrating their actions on the genome. Frequently, such coregulators are located in the cytoplasm, regulating the non genomic activity of the estrogens. Proline-, glutamic acid-, and leucine-rich protein 1 (PELP1), also known as modulator of non-genomic activity of ER (MNAR), amplified in breast cancer-1 (AIB1) and transcriptional intermediary factor-2 (TIF2) are considered major ER-coregulators. Thus, the investigation of their expression is inherent to the evaluation of estrogen-mediated mechanisms. The dynamic cross-talk between HER- and ER-driven signaling pathways has been described. The aim of this study is the investigation of the role of HER3, ER and coregulators PELP1/MNAR, AIB-1, TIF-2 (over)expression in the pathogenesis and prognosis of colorectal cancer. Material and Methods Sections from formalin-fixed, paraffin-embedded colorectal tissue blocks, derived from 140 patients with colorectal cancer, were used. HER-3 mRNA levels of expression were assessed by quantitative RT-PCR in 54 colorectal adenocarcinomas and 29 normal mucosa specimens. The expression levels of both phosphorylated and unphosphorylated HER-3 protein were assessed by immunohistochemistry in 110 normal mucosa specimens, 24 adenomas and 140 adenocarcinomas. The expression levels of ER α and β, PELP1/ΜΝΑR were assessed by immunohistochemistry in 88 normal mucosa specimens, 30 adenomas and 113 adenocarcinomas. Additionally, the expression levels of ΑΙΒ1 and TIF-2 protein were assessed by immunohistochemistry in 83 normal mucosa specimens, 30 adenomas and 110 adenocarcinomas. Results HER-3 was detected both in the cytoplasm and nucleus, whereas pHER-3 was observed in the nucleus and membrane of cells. A possible switch in HER-3 topography from the nucleus to the cytoplasm during colorectal tumorigenesis is suggested. The expression of pHER-3 did not differ significantly in normal tissue, adenomas and carcinomas, but was related to disease stage. HER-3 mRNA overexpression was significantly associated with decreased time to disease progression. It was also correlated with higher median age, left colon and rectal tumour sites and lymph node involvement. ERα expression was extremely rare in colorectal tissue of our cohort and its expression did not appear to be associated with colorectal carcinogenesis. ERβ and PELP1/MNAR were detected in the nucleus of epithelial, endothelial, inflammatory, smooth muscle cells and myofibroblasts. When intensity of staining was taken into account, the expression of both proteins was significantly increased in epithelial cells of carcinomas compared to normal mucosa. ERβ expression in epithelial cells was correlated with decreased disease progression-free survival. PELP1/MNAR overexpression in epithelial cells was found to be an independent favorable prognostic factor. AIB1 and TIF2 were detected in the nucleus of epithelial, endothelial, inflammatory, smooth muscle cells and myofibroblasts. The expression of both proteins was significantly increased in epithelial cells of carcinomas compared to normal mucosa. In carcinomas, a significant correlation between the levels of expression of AIB1 and TIF2 was noted, but there was no correlation between the expression patterns of these two proteins and ERβ. Although AIB1 overexpression was associated with local tumor invasion, it was also found to correlate independently with prolonged overall survival. TIF2 overxpression did not appear to correlate with clinicopathological parameters. Conclusion/Discussion This study highlights the significance of ΗΕR3 expression and phosphorylation in colorectal carcinogenesis, supporting also its potential prognostic significance. This study supports literature data regarding HER3 expression in colorectal tissue, while is the first to imply a possible prognostic significance of HER-3 mRNA expression levels and to suggest a topographic switch of HER3 protein during colorectal carcinogenesis. ERβ1 protein levels were found to increase during colorectal carcinogenesis, a finding which corresponds only to a small portion of literature data. The prognostic role of nuclear receptors depends on a number of factors, such as coregulator expression levels, chemical modifications, subcellular localization and ligand/hormone levels. The concomitant increase in the expression levels of coregulators PELP1/MNAR, ΑΙΒ1 and ΤΙF2 during colorectal carcinogenesis might imply their potential participation in estrogen-mediated signaling. However, the characteristic absence of strong correlation between their expression pattern and ERβ1 expression pattern underlines their pluripotent role and their possible contribution to estrogen-independent signaling. Further studies with a large number of patients, appropriately designed and conducted using sensitive experimental and statistical methods, are required for the confirmation of our hypothesis generation results. In the post-genomic era, identification of useful molecular biomarkers might contribute to the improvement of the management and prognosis of patients with colorectal cancer.

Καρκινογένεση

Συμπαράγοντες

616.994 347

Colorectal cancer

Carcinogenesis

Estrogen receptor

Coregulators

HER3

ER

AIB1

TIF2

PELP1/MNAR