Modeling and histopathological recognition of anoikis resistance in colorectal carcinoma

Patankar, M. (Madhura)

03 December 2019

Abstract Colorectal carcinoma (CRC) is an important cause of cancer-associated deaths. About 30–50% of CRCs show KRAS or BRAF mutation. In many cancers, anoikis, i.e. apoptosis induced by loss of extracellular matrix (ECM) contact, is disturbed. Anoikis resistance is essential for the formation of metastases, and since anoikis resistance assessment is based on in vitro cell cultures, the prognostic value of anoikis resistance is largely unknown. We aimed to identify the histopathological features indicating anoikis resistance in CRC and analyze their prognostic value. The roles of BRAF and KRAS mutations and survivin in anoikis resistance were analyzed and 3-D cell culture was used to model the histopathology of anoikis resistant (AR) structures. The two cohorts of CRC cases used in the study consisted of 62 (series 1) and 137 patients (series 2). Immunohistochemistry for ECM proteins enabled identification of tumor cells with and without ECM contact, and in both populations, apoptosis was determined with staining for caspase-cleaved keratin 18. Based on absence of ECM contact and decreased apoptosis rate, we identified micropapillary (MIP), cribriform and solid structures to represent the putative AR populations. High areal density of AR structures associated independently with short survival and was an independent prognostic factor. MIPs showed lower survivin expression, proliferation and apoptosis rates than non-MIP cells, and low apoptosis rate was associated with poor prognosis in stage I and II cases. For 3-D in vitro model of AR structures, we transfected Caco-2 cells with mutated KRAS or BRAF genes; both induced anoikis resistance as measured with Annexin V test in suspension culture. In 3-D cultures, native Caco-2 cells formed polarized cysts. In contrast, mutated cell lines formed partially filled cysts or solid structures, and inverted polarity in KRAS mutant cells. In conclusion, it is possible to identify putative AR structures by conventional histopathology and their number is associated with poor prognosis. MIPs represent a distinct subpopulation of CRC cells with features of quiescence. KRAS and BRAF mutations induce anoikis resistance in Caco-2 cells. In 3-D cultures, oncogenes KRAS and BRAF induce solid structures and cell piling, with structural resemblance to putative AR structures observed by histopathology. The mutated Caco-2 cells thus serve as a model to study the manifestation of anoikis resistance as a distinct histological feature with oncological significance. / Tiivistelmä Paksu- ja peräsuolisyöpä on yleinen syöpäkuoleman aiheuttaja. KRAS- tai BRAF-geenien mutaatio todetaan 30–50 prosentissa suolisyövistä. Anoikis tarkoittaa apoptoosia, jonka käynnistää solun irtoaminen soluväliaineesta. Anoikisresistenssi on etäpesäkkeen synnyn edellytys. Anoikisresistenssiä voidaan todeta vain soluviljelyssä, joten sen merkitystä syövässä in vivo ei ole aiemmin arvioitu. Tässä työssä pyrittiin tunnistamaan anoikisresistenssiin viittaavat muutokset histopatologisista suolisyöpänäytteistä ja selvittämään niiden vaikutusta potilaan ennusteeseen. Lisäksi tutkittiin BRAF- ja KRAS-mutaatioiden yhteyttä anoikisresistenssiin ja mallinnettiin anoikisresistenttejä (AR) rakenteita kolmiulotteisessa soluviljelmässä. Potilasaineisto koostui 199 suolisyöpäpotilaasta. Kudosleikkeistä värjättiin soluväliaineen komponentteja sekä määritettiin apoptoottiset ja jakautuvat solut (M30- ja Ki-67-värjäykset). AR-solupopulaatioiden tunnistamisessa käytettiin kriteereinä soluväliainekontaktin puuttumista ja vähentynyttä apoptoositiheyttä. AR-populaatioiksi osoittautuivat mikropapillaariset (MIP), seulamaiset ja solidit rakenteet. Näiden rakenteiden korkea kokonaisesiintyvyys osoittautui itsenäiseksi huonon ennusteen tekijäksi. MIP-rakenteissa surviviinin ilmentyminen ja apoptoosi- ja proliferaatiotiheys olivat vähentyneet muihin kasvainsoluihin verrattuna. Lisäksi apoptoottisten solujen pieni määrä MIP-rakenteissa liittyi huonoon ennusteeseen paikallisessa syövässä. Mallinnusta varten Caco-2 solut transfektoitiin mutatoiduilla KRAS- tai BRAF-geeneillä. Onkogeenien transfektion todettiin indusoivan anoikisresistenssiä. Kolmiulotteisessa soluviljelyssä polarisoituneet Caco-2 solut muodostivat säännöllisiä rauhasmaisia rakenteita. Onkogeeneillä transfektoidut solut muodostivat puolestaan osittain tai kokonaan täyttyneitä rakenteita ja KRAS-transfektio aiheutti solujen polariteetin kääntymistä. Havainnot osoittavat, että anoikisresistenssiä edustavat rakenteet voidaan tunnistaa kudosleikkeestä ja niiden runsas määrä viittaa huonoon ennusteeseen. MIP-rakenteissa todettiin lepotilan (quiescence) piirteitä. KRAS- ja BRAF-mutaatiot aiheuttavat Caco-2 soluissa anoikisresistenssiä. Kolmiulotteisissa soluviljelmissä onkogeenien vaikutus näkyy solujen pinoutumisena, mikä muistuttaa syöpäkudosnäytteissä todettuja AR-rakenteita. Tulosten perusteella modifioituja Caco-2 soluja voidaan hyödyntää anoikisresistenssin mallintamiseen ja tarkempien mekanismien tutkimiseen.

anoikis resistance

apoptosis

carcinoma

colon

extracellular matrix

proliferation

survivin

anoikisresistanssi

apoptoosi

karsinooma

kooolon

proliferaatio

soluväliaine

BRAF

KRAS

Molekulární mechanismy nádorové patogeneze signální cesty Hedgehog u vybraných nádorových typů / Molecular mechanisms of tumor pathogenesis of Hedgehog signaling pathway in selected tumor types

Kreisingerová, Kateřina

January 2021

The presented doctoral thesis is focused on the role of the Hedgehog (HH) signaling pathway in cancer pathogenesis. HH signaling pathway is an evolutionarily conserved signaling pathway that plays an essential role in embryonic development. Its activity is strictly limited to stem and progenitor cells for example in brain, lung, skin or prostate. HH pathway also plays a key role in tissue homeostasis and regeneration. Aberrantly activated HH pathway is essential in cancer progression. The aim of the presented thesis was to elucidate new details about the HH signaling pathway. We identified a new target gene of the HH pathway - the anti-apoptotic protein survivin. Survivin is considered to be an important tumor marker associated with a poor prognosis of patients. We showed that the inhibitor of HH pathway effectors GLI1 and GLI2 GANT61 reduced the survivin level in cancer cells. Subsequently, we used GANT61 and the inhibitor of the anti-apoptotic BCL2 protein family obatoclax to inhibit melanoma cells growth. We showed that the combination of these inhibitors was very effective in the eradication of melanoma cells in vitro. We also proved that GANT61 triggers the process of apoptosis in melanoma cells. We found out that the HH signaling pathway is canonically activated in many cell lines of various...

In vitro 3D fluorescent cell-based assay reporting gene regulation for high-throughput drug screening

Li, You

27 September 2022

No description available.

Chemical Engineering

Biology

3D cell culture

drug screening

survivin

telomerase reverse transcriptase

fluorescent protein

reporter gene assay

Computational Simulations of Protein-Ligand Molecular Recognition via Enhanced Samplings, Free Energy Calculations and Applications to Structure-Based Drug Design

Park, In-Hee

13 September 2010

No description available.

Biomedical Research

Biophysics

Chemistry

enhanced sampling

free energy calculation

structure-based drug design

ligand-induced-fit simulation

survivin

Avaliação da transfecção de células dendríticas com RNA tumoral como estratégia para indução de imunidade específica em pacientes com leucemia linfóide crônica. / Evaluation of dendritic cell transfection with tumor RNA as a strategy to induce specific immunity in chronic lymphoid leukemia patients.

Toniolo, Patrícia Argenta

07 December 2010

O desenvolvimento da imunoterapia do câncer baseada em células dendríticas (DCs) é alvo de vários estudos. Para tumores sólidos, a abordagem baseada no uso de DCs alogenêicas fundidas com células tumorais tem se mostrado relativamente eficaz. Por outro lado, esta estratégia necessita uma massa tumoral considerável de cada paciente para a geração das células híbridas. Para contornar este problema o uso de DCs transfectadas com mRNA tumoral, o qual pode ser amplificado in vitro a partir de uma pequena amostra inicial do tumor, tem sido investigado. Para isto, uma transfecção eficiente e tradução correta do mRNA tumoral nas DCs são etapas críticas. Sabendo-se que as DCs de pacientes com câncer possuem atividade aloestimuladora defeituosa, DCs derivadas de doadores saudáveis poderiam ser uma alternativa para induzir uma resposta imune mais eficiente. Assim, este trabalho pretendeu aprimorar a metodologia de transfecção de DCs alogenêicas, derivadas de monócitos de doadores saudáveis, com mRNA de antígenos tumorais (survivina e RPSA) super-expressos na leucemia linfóide crônica (LLC) e avaliar sua capacidade em estimular a resposta linfocitária. Ao mesmo tempo, foram estabelecidas as metodologias para amplificação e síntese do RNA destes antígenos tumorais específicos, assim como do RNA mensageiro total, contidos nas células tumorais de pacientes com LLC. Os resultados mostraram ser possível a amplificação do mRNA total extraído das células leucêmicas com manutenção da expressão dos antígenos tumorais. Ainda, várias condições de transfecção com mRNA da survivina, transcrito in vitro, foram testadas, encontrando-se na lipofecção, a melhor maneira de transfectar as DCs. A lipofecção mostrou-se com baixa toxicidade quando comparada à técnica de eletroporação. Observou-se uma eficiência em torno de 40% de células transfectadas num intervalo de tempo entre 12 e 48 horas. Estas células foram usadas como estimuladoras em ensaios de proliferação usando-se linfócitos T alogenêicos como células respondedoras. As células transfectadas com mRNA da survivina foram capazes de estimular resposta linfoproliferativa com maior produção de IFN-gama, avaliado por ELISA. Além disso, a transfecção não alterou o padrão de expressão dos marcadores de superfície característicos das DCs. Estes dados mostram que a transfecção das DCs com mRNA pode afetar a resposta imune induzida por estas APCs. Nossos resultados suportam o uso de DCs transfectadas com mRNA para produção de vacinas anti-tumorais e mostram a survivina como um potente antígeno indutor da resposta linfocitária. / The development of dendritic cell (DC)-based cancer immunotherapy has been the target of many studies. For solid tumors, a promising approach based in allogeneic DCs fused to tumor cells has been relatively effective. On the other hand, this approach needs large tumor samples to generate enough DC-tumor cell hybrids. To overcome this problem, tumor mRNA-transfected DCs can be used, since mRNA can be amplified in vitro and allow unlimited vaccine production. For this, efficient transfection and optimal translation of tumor mRNA in DCs are critical. Moreover, DC derived from cancer patients has defective alostimulatory activity. In this case, DC derived from healthy donors may be an alternative to induce immune response more efficiently. Here, we established the methodology of allogeneic DC transfection with mRNA for tumor antigens (survivin and RPSA) overexpressed in chronic lymphocytic leukemia (CLL), and evaluated their ability for T cell stimulation. At the same time, we established mRNA amplification and mRNA in vitro transcription methodology for specific tumor antigens and total messenger RNA, present in CLL tumor cells. Our results showed it to be possible to amplify total mRNA derived from leukemic cells maintaining tumor antigen expression. Moreover, several transfection conditions using survivin mRNA obtained from in vitro transcript reactions were evaluated, defining lipofection as the better way to transfect DC. We obtained nearly 40% of transfected DCs between 12 and 48 hours. Transfected DCs were used as stimulator cells in proliferation assays using allogeneic T cells as responder cells. Survivin mRNA transfected DCs were able to stimulate T cell proliferation with increased IFN-gama production, measured by ELISA. Furthermore, the transfection did not change the pattern of surface molecules expression characteristic of DC. These data show that mRNA DC transfection can affect immune responses induced by these APCs. These findings support the use of tumor mRNA transfected DCs for anti-cancer vaccine production and show survivin as a potent antigen to induce T cell responses.

Cellular immunology

Células cultivadas de tumor

Células dendríticas

Cultured tumor cells

Dendritic cell

Immunity

Imunidade

Imunologia celular

Monócitos (imunologia)

Monocytes (immunology)

RNA tumoral

Survivin

Survivina

Transfecção

Transfection

Tumor RNA

A combination of molecular and traditional chemotherapy: prospects of synergies against cancer

Singh, Preetinder Pal, Clinical School - Prince of Wales Hospital, Faculty of Medicine, UNSW

January 2009

In this study, we have explored the combination of a novel Purine Nucleoside Phosphorylase mediated Gene-Directed Enzyme Prodrug Therapy (PNP-GDEPT) with chemotherapeutics, Taxotere and/or Carboplatin to target prostate and ovarian cancer (PC & OC). PNP converts the prodrug (Fludarabine-phosphate) to a toxic purine, 2-fluoroadenine (2FA) that inhibits RNA/DNA synthesis. Taxotere is active against late stage PC whilst carboplatin is first line therapy for OC. Neither modality is adequately effective. We expect that a combination will target heterogeneity via cytotoxicity to diverse cancer cell populations leading to effective synergies, which may improve efficacy and quality of life. For PC, Synergy between Ad-PNP-GDEPT and Taxotere were assessed in vitro and in vivo. Cell killing effects of combination led to significant synergistic killing of human PC-3 & murine RM1 PC cells accompanied by enhanced apoptosis. A lower individual dose (by up to 8 fold) led to enhanced efficacy. In vivo, the combination regimen given at the suboptimal doses led to reduction in local tumour (PC-3 & RM1) growth in nude and in C57BL/6 mice, respectively. A significant reduction in lung RM1 colony numbers indicated enhanced systemic efficacy. Combination treated mice also displayed significantly improved survival (25 days vs 15 days for control mice). Importantly, the condition of combination treated mice (e.g. weight loss) was better than those given individual treatments. The possible involvement of the immune system in this enhanced effect is under investigation. For OC, three-way synergy between Ad-PNP-GDEPT, Taxotere and carboplatin was effectively demonstrated in SKOV-3 and OVCAR-3 cells. This was significantly greater than bimodal or individual treatments. A 10-50 fold dose reduction of individual treatments was effective when combined, accompanied by enhanced apoptosis. Western-blotting analyses revealed a shift in the expression of anti-apoptotic and proapoptotic proteins upon treatment with various combinations. This is the first demonstration of synergy between these modalities.

Prostate cancer

Combination therapy

Ovarian cancer

Gene therapy

Apoptosis

PNP-GDEPT

Adenovirus

Her-2 neu

Survivin

Chemotherapy

Docetaxel

Carboplatin

Διερεύνηση των μηχανισμών με τους οποίους χημικές ενώσεις με αντινεοπλασματικές ιδιότητες προκαλούν γενετικές ανωμαλίες / Investigation of the mechanisms by which antineoplasmatic compounds induce genetic instability

Ευθυμίου, Μαρία

26 August 2010

Οι υπερίτες του αζώτου (nitrogen mustards) συνιστούν μία αποτελεσματική ομάδα φαρμάκων που χρησιμοποιούνται στη χημειοθεραπεία του καρκίνου. Πρόσφατα ευρήματα της ερευνητικής μας ομάδας έδειξαν ότι οι υπερίτες του αζώτου μελφαλάνη (MEL), χλωραμπουκίλη (CAB) και ο δραστικός της μεταβολίτης, το PHE, επιδεικνύουν ισχυρή θραυσματογόνο δράση, αλλά επιπρόσθετα, εμφανίζουν ανευπλοειδογόνο δράση, διαταράσσοντας το χρωμοσωματικό αποχωρισμό μέσω τροποποιήσεων της δομής και λειτουργίας της μιτωτικής συσκευής. Στην παρούσα διατριβή, διερευνήθηκε περαιτέρω ο μηχανισμός της ανευπλοειδογόνου δράσης των παραπάνω δραστικών ενώσεων και πραγματοποιήθηκε σύγκριση της γενετικής δράσης δύο νέων στεροειδών αναλόγων του PHE, τα ανάλογα ΕΑ-92 και ΕΑ-97 με αυτήν των MEL, CAB και PHE. Τα στεροειδή ανάλογα σχεδιάστηκαν με στόχο την αύξηση της εκλεκτικότητας της αντινεοπλασματικής δράσης. Η ικανότητα των MEL, CAB και PHE να προκαλούν φαινόμενα χρωμοσωματικής καθυστέρησης μελετήθηκε σε σύγκριση με τα στεροειδή ανάλογα ΕΑ-92 και ΕΑ-97. Η μελέτη πραγματοποιήθηκε σε ανθρώπινα λεμφοκύτταρα in vitro με τη μέθοδο αναστολής της κυτταροκίνησης (CBMN) σε συνδυασμό με τη μέθοδο FISH και τη χρήση πανκεντρομερικού ανιχνευτή. Επιβεβαιώθηκε η θραυσματογόνος και ανευπλοειδογόνος δράση των ενώσεων MEL, CAB και PHE, ενώ φάνηκε ότι τα στεροειδή ανάλογα ΕΑ-92 και ΕΑ-97 προκαλούν αποκλειστικά χρωμοσωματική θραύση. Το φαινόμενο της χρωμοσωματικής καθυστέρησης μελετήθηκε επίσης με τη μέθοδο CREST στην κυτταρική σειρά ποντικού C2C12. Με τη μέθοδο αυτή, επιβεβαιώθηκε η διπλή γενετική δράση των ενώσεων MEL, CAB και PHE. Τα στεροειδή ανάλογα ΕΑ-92 και ΕΑ-97 εμφανίστηκαν ως οι ηπιότεροι επαγωγείς ΜΝ και προκαλούν κυρίως χρωμοσωματική θραύση, ενώ ήπια ανευπλοειδογόνο δράση παρουσίασε μόνο το ανάλογο ΕΑ-92. Ακολούθως, εξετάσθηκε η ικανότητα των υπό εξέταση χημικών ενώσεων ΕΑ-92 και ΕΑ-97, να επηρεάζουν τη δομή και λειτουργία της μιτωτικής συσκευής σε σχέση με αυτήν των ενώσεων MEL, CAB, PHE, με διπλό ανοσοφθορισμό για τη β- και γ-τουμπουλίνη. Παρατηρήθηκε ότι όλες οι ενώσεις, εκτός από το στεροειδές ΕΑ-97 προκαλούν τη δημιουργία πολυπολικών μεταφάσεων, ενώ όλες οι ενώσεις επάγουν το σχηματισμό μεσοφασικών κυττάρων με ανώμαλο αριθμό κεντροσωμάτων. Όλες οι υπό εξέταση χημικές ενώσεις εμφανίζουν κυτταροτοξικότητα και καθυστέρηση του κυτταρικού κύκλου σε καλλιέργειες ανθρώπινων λεμφοκυττάρων και στα κύτταρα ποντικού C2C12. Στη συνέχεια διερευνήθηκε η ικανότητα των υπό εξέταση ενώσεων να επάγουν την απόπτωση και μελετήθηκε ο ρόλος της απόπτωσης στην εκδήλωση της γενετικής δράσης των ενώσεων MEL, CAB και PHE. Η μελέτη αυτή πραγματοποιήθηκε στα κύτταρα C2C12 με τη μέθοδο της διπλής χρώσης Αννεξίνης V/Ιωδιούχου προπιδίου και το διπλό ανοσοφθορισμό β- και γ-τουμπουλίνης, ανεξάρτητα, σε κύτταρα ποντικού C2C12, παρουσία του γενικού αναστολέα της δράσης των κασπασών, Z-VAD-FMK, αλλά και αναστολέων της δράσης συγκεκριμένων κασπασών. Όλες οι υπό εξέταση ενώσεις επάγουν χαμηλά ποσοστά απόπτωσης. Οι κασπάσες-3, -6 και -8 συμμετέχουν στην επαγόμενη από τη MEL απόπτωση αλλά δεν συμμετέχουν στην απομάκρυνση των κυττάρων με μικροπυρήνες που επάγονται από τη δράση της ίδιας ένωσης. Η απόπτωση αποτελεί μηχανισμό απομάκρυνσης των κυττάρων με μικροπυρήνες και κανονικό κεντροσωματικό αριθμό που επάγονται από τις ενώσεις MEL, CAB και PHE. Αντίθετα, τα κύτταρα με υπεράριθμα κεντροσώματα, που προκύπτουν από τη δράση των παραπάνω ενώσεων δεν απομακρύνονται μέσω απόπτωσης. Για την περαιτέρω διερεύνηση του μηχανισμού με τον οποίο οι δραστικές ενώσεις MEL και CAB εκφράζουν τις ανευπλοειδογόνες ιδιότητες τους, μελετήθηκε η επίδραση τους στην έκφραση των πρωτεϊνών Aurora-B, survivin, Aurora-A και γ-τουμπουλίνη σε κύτταρα ποντικού C2C12, με τη μέθοδο της ανοσοαποτύπωσης των πρωτεϊνών. Παράλληλα μελετήθηκε η ένωση ΕΑ-97, η οποία σύμφωνα με τα ευρήματα μας, εμφάνισε αποκλειστικά θραυσματογόνο δράση. Οι ενώσεις MEL και CAB, εκδηλώνουν τις ανευπλοειδογόνες ιδιότητες τους προκαλώντας μείωση της έκφρασης των πρωτεϊνών Aurora-B και survivin και επάγοντας την αύξηση της έκφρασης της πρωτεΐνης Aurora-A. Επιπρόσθετα, η ένωση MEL, προκαλεί αύξηση της έκφρασης της γ-τουμπουλίνης. Τα ευρήματα αυτά υποδεικνύουν τη συμμετοχή των παραπάνω πρωτεϊνών στην εκδήλωση της ανευπλοειδογόνου δράσης των ενώσεων που μελετήθηκαν. Αντίθετα το στεροειδές ανάλογο ΕΑ-97 που εμφανίζει αποκλειστικά θραυσματογόνο δράση, δεν μεταβάλλει την έκφραση των παραπάνω πρωτεϊνών. / Nitrogen mustards represent an effective class of drugs that are used in chemotherapy. Recent findings of our group have shown that nitrogen mustard analogues, melphalan (MEL), chlorambucil (CAB) and PHE, in addition to their clastogenic activity, they exert their aneugenic potential by affecting chromosome segregation due to modifications of mitotic apparatus. In the present study, we investigated the mechanism by which the above compounds display their aneugenicity in comparison with two new steroidal analogues of PHE, EA-92 and EA-97, which were designed aiming at most effective antineoplasmatic activity. The ability of MEL, CAB and PHE to induce chromosome delay events was studied in comparison with the steroidal analogues EA-92 and EA-97. The mechanism of micronucleation was determined by Cytokinesis Block Micronucleus assay (CBMN assay) in combination with Fluorescence In Situ Hybridization (FISH) using pancentromeric DNA probe. It was confirmed that MEL, CAB and PHE generated MNi by two mechanisms, chromosome breakage and chromosome delay, while EA-92 and EA-97 induced the formation of MN originated exclusively from chromosome breakage events. The ability of the tested compounds to induce chromosome delay was also investigated in C2C12 mouse cells by CREST analysis. The dual genetic activity of MEL, CAB, and PHE was confirmed in a different biological system. The analogues EA-92 and EA-97 appeared as weaker MN inducers and they induced mainly chromosome breakage, while a weak aneugenic activity was observed for EA-92. The ability of the nitrogen mustard analogues to affect the organization of mitotic apparatus was investigated in comparison with MEL, CAB and PHE by double immunofluorescence of β- and γ-tubulin in C2C12 mouse cells. It was observed that all compounds, except EA-97, induced mutlipolar metaphases, and also generated interphase cells with abnormal centrosome number. All compounds displayed increased cytotoxicity and they caused cell cycle delay in human lymphocyte cultures and in C2C12 mouse cells. The ability of the tested compounds to induce apoptosis was studied by Annexin V/PI assay. It was revealed that all compounds induced apoptosis. The effect of apoptosis on the genetic activity of MEL, CAB and PHE was investigated by inhibition of apoptosis in the presence of the inhibitor Z-VAD-FMK and the use of specific inhibitors for caspase -3, -6, -8 and -1. For this reason Annexin V/PI assay and double immunofluorescence of β- and γ-tubulin were performed, independently in C2C12 mouse cells. Caspases -3, -6 and -8 are involved in melphalan-induced apoptosis, but they are not involved in the elimination of cells in the presence of melphalan. Apoptosis is the responsible mechanism for the exclusion of cells with MNi and normal centrosome number that are induced by MEL, CAB and PHE. On the contrary, cells exerting supernumerary centrosomes are not eliminated by apoptosis in the presence of the above compounds. To further elucidate the mechanisms by which MEL and CAB exert their aneugenic potential, we examined the ability of the compounds to alter the expression of proteins having important role in chromosome segregation, such as the proteins Aurora-B, survivin, Aurora-A and γ-tubulin. The analysis was performed by Western blot method in C2C12 mouse cells. We also studied the steroid analogue EA-97, which according to our findings acts as a pure clastogen and do not exert aneugenic potential as opposed to MEL and CAB. MEL and CAB exert their aneugenic potential by the reduction of Aurora-B and survivin expression and by enhancing the expression of Aurora-A. γ-tubulin was upregulated in the presence of MEL. These findings show the implication of these proteins in chromosome delay events induced by MEL and CAB. On the other hand, the analogue EA-97 did not affect the expression of the above proteins.

Υπερίτες του αζώτου

Ανευπλοειδία

Μικροπυρήνες

Aurora κινάσες

Απόπτωση

γ-τουμπουλίνη

616.994 061 072 4

Nitrogen mustards

Aneuploidy

Supernumerary centrosomes

Micronucleus

Aurora kinases

Apoptosis

Survivin

γ-tubulin

Differentiation and malignant transformation of epithelial cells:3D cell culture models

Capra, J. (Janne)

06 March 2018

Abstract The epithelial cells form barriers that compartmentalize the organs. Carcinomas are cancers stemming from epithelial cells and are the most common cancer type. The aim of this study was to understand the differentiation and malignant transformation of epithelial Madin-Darby canine kidney (MDCK) cells and to analyse the electrophysiological parameters which regulate their transport capacity. Emphasis was placed on comparing different culture environments, both in 2D and 3D. First, the effects of drugs or basal extracellular fluid composition on MDCK cell, cyst and lumen volumes were analysed using time-lapse microscopy. The results showed that MDCK cells were capable of both water secretion and reabsorption. The cells were able to perform these functions in a hyperpolarizing or depolarizing environment; change in osmolality of basal fluid was not required. Taken together, these results validate MDCK cells as a good basic model for studying kidney function. Next, the aim was to analyse the effect of 2D and 3D culture environments on the gene expression of untransformed MDCK and temperature sensitive ts-Src -transformed MDCK cells and the changes a single oncogene can induce. Microarray analysis revealed a decrease in the expression of survivin, an inhibitor of apoptosis protein, when switching the untransformed cells from 2D environment to 3D. This downregulation of survivin occurs in adult tissues as well, indicating that the cells grown in 3D are closer to the in vivo state than 2D cells. Src oncogene induced disintegration of cell junctions, but did not downregulate E-cadherin expression. The last part was to study further the factors controlling survivin expression and its significance to cell survival. MDCK cells grown in 3D did not suffer apoptosis if the cells remained in contact with the extracellular matrix. If MDCK cells were denied of ECM contacts they were more susceptible to apoptosis than survivin-expressing ts-Src MDCK cells. Finally, if cells were denied of cell-cell junctions, cells lacking survivin suffered apoptosis even though they had proper cell-matrix contacts. Taken together, these results highlighted the importance of cellular contacts to the cells: MDCK cells needed ECM contacts to differentiate and cell-cell contacts to avoid apoptosis. / Tiivistelmä Epiteelisolut ovat erikoistuneet toimimaan rajapintana elimen ja ympäristön välillä. Ihmisten yleisin syöpä on epiteelisoluista alkunsa saanut karsinooma. Tämän tutkimuksen tarkoituksena oli ymmärtää Madin-Darby-koiran munuaisen solujen (MDCK) erilaistumista ja pahanlaatuistumista sekä analysoida sähköfysiologisia tekijöitä, jotka säätelevät näiden solujen kuljetustoimintaa. Erityisenä kiinnostuksen kohteena oli erilaisten kasvuympäristöjen vertailu. Farmakologisten aineiden tai basaalisen, solunulkopuolisen nesteen koostumuksen vaikutusta MDCK-solujen, -kystan sekä luumenin kokoon tutkittiin valomikroskooppisten aikasarjojen avulla. Tulokset osoittivat MDCK-solujen olevan kykeneviä sekä veden eritykseen että absorptioon, niin hyperpolarisoivassa kuin depolarisoivassakin ympäristössä. Basaalisen nesteen osmolaliteetin muutosta ei tarvittu. Nämä tulokset osoittavat MDCK-solujen olevan hyvä munuaisen tutkimuksen perusmalli. Seuraavaksi analysoitiin kaksi- ja kolmiulotteisten (2D ja 3D) viljely-ympäristöjen vaikutusta ei-transformoitujen MDCK-solujen ja lämpötilaherkkien ts-Src-transformoitujen MDCK-solujen geenien ilmentymiseen sekä yhden onkogeenin aktivoimisen aikaansaamia muutoksia. Microarray-analyysi osoitti apoptoosin estäjän, surviviinin, ilmentymisen vähenemisen, kun kasvuympäristö vaihdettiin 2D-ympäristöstä 3D-ympäristöön. Koska surviviinin väheneminen on normaali tapahtuma aikuisissa kudoksissa, voitiin todeta, että 3D-ympäristössä kasvatetut solut ovat lähempänä luonnonmukaista olotilaa kuin 2D-ympäristössä kasvaneet. Src-onkogeeni sai aikaan soluliitosten hajoamisen, mutta ei vähentänyt E-kadheriinin ilmentymistä. Tutkimuksen viimeinen osa keskittyi surviviinin ilmentymistä säätelevien tekijöiden analysoimiseen ja surviviinin merkitykseen solujen eloonjäämiselle. 3D-ympäristössä kasvaneet MDCK-solut eivät kärsineet apoptoosista edellyttäen, että solut pysyivät kosketuksissa soluväliaineeseen. Jos solut irtautuivat soluväliaineesta, ne päätyivät herkemmin apoptoosiin kuin surviviinia ilmentävät ts-Src MDCK-solut. Mikäli solujen väliset liitokset pakotettiin avautumaan, solut joutuivat apoptoosiin, vaikka ne olivat kosketuksissa soluväliaineeseen. Yhteenvetona nämä tulokset korostavat solujen kontaktien merkitystä: MDCK-solut tarvitsevat soluväliainekontakteja erilaistumiseen ja solujen välisiä kontakteja välttyäkseen apoptoosilta.

MDCK cells

Src kinase

apoptosis

live cell microscopy

polarity

survivin

transepithelial transport

MDCK-solut

Src-kinaasi

apoptoosi

elävien solujen mikroskopointi

polariteetti

surviviini

transepiteelinen kuljetus

Avaliação da transfecção de células dendríticas com RNA tumoral como estratégia para indução de imunidade específica em pacientes com leucemia linfóide crônica. / Evaluation of dendritic cell transfection with tumor RNA as a strategy to induce specific immunity in chronic lymphoid leukemia patients.

Patrícia Argenta Toniolo

07 December 2010

O desenvolvimento da imunoterapia do câncer baseada em células dendríticas (DCs) é alvo de vários estudos. Para tumores sólidos, a abordagem baseada no uso de DCs alogenêicas fundidas com células tumorais tem se mostrado relativamente eficaz. Por outro lado, esta estratégia necessita uma massa tumoral considerável de cada paciente para a geração das células híbridas. Para contornar este problema o uso de DCs transfectadas com mRNA tumoral, o qual pode ser amplificado in vitro a partir de uma pequena amostra inicial do tumor, tem sido investigado. Para isto, uma transfecção eficiente e tradução correta do mRNA tumoral nas DCs são etapas críticas. Sabendo-se que as DCs de pacientes com câncer possuem atividade aloestimuladora defeituosa, DCs derivadas de doadores saudáveis poderiam ser uma alternativa para induzir uma resposta imune mais eficiente. Assim, este trabalho pretendeu aprimorar a metodologia de transfecção de DCs alogenêicas, derivadas de monócitos de doadores saudáveis, com mRNA de antígenos tumorais (survivina e RPSA) super-expressos na leucemia linfóide crônica (LLC) e avaliar sua capacidade em estimular a resposta linfocitária. Ao mesmo tempo, foram estabelecidas as metodologias para amplificação e síntese do RNA destes antígenos tumorais específicos, assim como do RNA mensageiro total, contidos nas células tumorais de pacientes com LLC. Os resultados mostraram ser possível a amplificação do mRNA total extraído das células leucêmicas com manutenção da expressão dos antígenos tumorais. Ainda, várias condições de transfecção com mRNA da survivina, transcrito in vitro, foram testadas, encontrando-se na lipofecção, a melhor maneira de transfectar as DCs. A lipofecção mostrou-se com baixa toxicidade quando comparada à técnica de eletroporação. Observou-se uma eficiência em torno de 40% de células transfectadas num intervalo de tempo entre 12 e 48 horas. Estas células foram usadas como estimuladoras em ensaios de proliferação usando-se linfócitos T alogenêicos como células respondedoras. As células transfectadas com mRNA da survivina foram capazes de estimular resposta linfoproliferativa com maior produção de IFN-gama, avaliado por ELISA. Além disso, a transfecção não alterou o padrão de expressão dos marcadores de superfície característicos das DCs. Estes dados mostram que a transfecção das DCs com mRNA pode afetar a resposta imune induzida por estas APCs. Nossos resultados suportam o uso de DCs transfectadas com mRNA para produção de vacinas anti-tumorais e mostram a survivina como um potente antígeno indutor da resposta linfocitária. / The development of dendritic cell (DC)-based cancer immunotherapy has been the target of many studies. For solid tumors, a promising approach based in allogeneic DCs fused to tumor cells has been relatively effective. On the other hand, this approach needs large tumor samples to generate enough DC-tumor cell hybrids. To overcome this problem, tumor mRNA-transfected DCs can be used, since mRNA can be amplified in vitro and allow unlimited vaccine production. For this, efficient transfection and optimal translation of tumor mRNA in DCs are critical. Moreover, DC derived from cancer patients has defective alostimulatory activity. In this case, DC derived from healthy donors may be an alternative to induce immune response more efficiently. Here, we established the methodology of allogeneic DC transfection with mRNA for tumor antigens (survivin and RPSA) overexpressed in chronic lymphocytic leukemia (CLL), and evaluated their ability for T cell stimulation. At the same time, we established mRNA amplification and mRNA in vitro transcription methodology for specific tumor antigens and total messenger RNA, present in CLL tumor cells. Our results showed it to be possible to amplify total mRNA derived from leukemic cells maintaining tumor antigen expression. Moreover, several transfection conditions using survivin mRNA obtained from in vitro transcript reactions were evaluated, defining lipofection as the better way to transfect DC. We obtained nearly 40% of transfected DCs between 12 and 48 hours. Transfected DCs were used as stimulator cells in proliferation assays using allogeneic T cells as responder cells. Survivin mRNA transfected DCs were able to stimulate T cell proliferation with increased IFN-gama production, measured by ELISA. Furthermore, the transfection did not change the pattern of surface molecules expression characteristic of DC. These data show that mRNA DC transfection can affect immune responses induced by these APCs. These findings support the use of tumor mRNA transfected DCs for anti-cancer vaccine production and show survivin as a potent antigen to induce T cell responses.

Células cultivadas de tumor

Células dendríticas

Imunidade

Imunologia celular

Monócitos (imunologia)

RNA tumoral

Survivina

Transfecção

Cellular immunology

Cultured tumor cells

Dendritic cell

Immunity

Monocytes (immunology)

Survivin

Transfection

Tumor RNA

Development of 3-D Microbioreactor Systems for Cell-Based High Throughput Screening

Zang, Ru

26 June 2012

No description available.

Chemical Engineering

microbioreactor

dissolved oxygen

cell proliferation

three-dimensional

cytotoxicity

embryotoxicity

developmental toxicity

survivin

green fluorescence protein

carbon nanotubes

embryonic stem cells