Rab-Proteine kontrollieren die Chlamydien-induzierte Fragmentierung des Golgi-Apparates

Lipinski, Anette Rejman

28 August 2009

Weltweit kommt es jährlich zu 90 Mio. Neuinfektionen mit dem sexuell übertragbaren Erreger Chlamydia trachomatis. Allerdings sind die Faktoren, die eine erfolgreiche bakterielle Vermehrung ermöglichen, weitgehend unbekannt. Während ihrer obligat intrazellulären Entwicklung sind Chlamydien auf die Errichtung und Erhaltung ihrer Nische, der Inklusion, angewiesen. Durch Interaktionen mit vesikulären Transportwegen der Wirtszelle, welche z.B. Sphingolipide transportieren, sichern die Bakterien ihr Überleben. In der vorliegenden Arbeit konnte gezeigt werden, dass Chlamydien während einer Infektion die Auflösung der Struktur des Golgi-Apparates induzieren. Mit Hilfe der RNA-Interferenz-Technik (RNAi) wurden die Auswirkungen des Verlustes von Golgi-Strukturproteinen auf die bakterielle Vermehrung untersucht. Der funktionelle Ausfall von Golginen, wie z.B. Golgin-84 führte zu einer Fragmentierung des Golgi-Apparates. Diese begünstigte die chlamydiale Produktion neuer infektiöser Partikel, was eine verbesserte Versorgung mit Nährstoffen nahelegt. Im vesikulären Transport von Nährstoffen übernehmen Rab-Proteine eine Schlüsselrolle. Interessanterweise konnte in dieser Arbeit gezeigt werden, dass der Verlust von Rab6 und Rab11 durch RNAi zu einer signifikanten Verringerung der Anzahl infektiöser Nachkommen führte. In diesen Zellen wurde der Golgi-Apparat nicht fragmentiert und der Transport von Sphingolipiden zu den Bakterien war stark vermindert. Untersuchungen nach simultaner Herunterregulation von Golgin-84 und Rab6 oder Rab11 demonstrierten abschließend, dass eine Kontrolle der Golgin-84-induzierten Golgi-Fragmentierung über Rab-Proteine möglich sein könnte. Die Ergebnisse dieser Arbeit offenbaren einen neuen Zusammenhang zwischen der Struktur des Golgi-Apparates und dessen Kontrolle über Rab-Proteine und ermöglichen einen tieferen Einblick in die Funktion des Golgi-Apparates während einer Chlamydien-Infektion. / Worldwide, approximately 90 mio. people are infected with the obligate intracellular bacterium Chlamydia trachomatis. However the factors involved in its successful infection and replication remain unknown. Chlamydia survive and replicate within a membrane bound niche inside host cells, termed the inclusion. To ensure survival, the chlamydial inclusion intercepts vesicular trafficking pathways of the host cell to acquire essential nutrients, such as sphingolipids. However, the exact mechanisms by which Chlamydia acquire these lipids have not been elucidated. The present work established that infection of host mammalian cells with C. trachomatis induced fragmentation of the Golgi-apparatus, but details of the mechanism to the bacterium’s pathogenesis are still required. Using RNA-Interference the role of specific Golgi-apparatus structural proteins in bacterial infectivity was investigated. Knockdown of Golgins in host cells resulted in a fragmented Golgi-apparatus and an associated increase in chlamydial replication, suggesting an enhanced acquisition of nutrients. Since Rab-proteins are known to co-ordinate the intracellular vesicular transport of nutrients, their importance in chlamydial infectivity was also investigated. Interestingly, knock down of Rab6 and Rab11 led to a significant reduction in infectious progeny. Surprisingly, upon knock down of Rab6 or Rab11 the Golgi-apparatus remained intact and sphingolipid transport into the inclusion was severely perturbed. Finally, analysis of cells simultaneously depleted of golgin-84 and Rab6 or Rab11 suggested a possible role of Rab-proteins in the control of golgin-84-induced Golgi fragmentation. These data demonstrate a yet unknown relationship between the structure of the Golgi-apparatus and its regulation and control by Rab-proteins. Furthermore, this work contributes to the existing knowledge regarding the function of the Golgi-apparatus during chlamydial infections.

siRNA

Rab-Proteine

Chlamydia trachomatis

Golgi-Fragmentierung

siRNA

Rab proteins

Chlamydia trachomatis

Golgi fragmentation

570 Biowissenschaften, Biologie

32 Biologie

WE 3650

WL 2735

ddc:570

Global assessment of host cell functions involved in the intracellular survival and replication of Chlamydia using RNA interference in human cells

Gurumurthy, Rajendra Kumar

24 March 2010

Chlamydia trachomatis ist ein obligat intrazellulär lebendes Bakterium. Es wird mit einer Vielzahl von Krankheiten in Verbindung gebracht. Das Überleben von Chlamydia trachomatis hängt in nahezu allen Aspekten von der Wirtszelle ab, angefangen bei der Anheftung an die Wirtszelle, über die Invasion, bis zur intrazellulären Replikation. Für ein vollständiges Bild der Pathogenese sind sowohl das Verstehen der dazu beitragenden bakteriellen wie auch Wirtszellfaktoren essenziell. Die vorliegende Arbeit konzentriert sich dabei auf die an der Infektion beteiligten Wirtsfaktoren. Mit Hilfe eines RNA-Interferenz-vermittelten Funktionsverlustscreens wurden 59 Wirtszellgene identifiziert, die einen Einfluss auf die Infektion und Vermehrung von Chlamydia trachomatis hatten. Unter Zuhilfenahme von bioinformatischen Signaltransduktionsweganalyse-Programmen konnten einige der Hits bekannten zellulären Signalnetzwerken, unter anderem dem Ras/Raf/Mek/Erk-Signalweg, zugeordnet werden. Insbesondere der Funktionsverlust zweier validierter Targets, Ras und Raf1, erhöhte das Chlamydien-Wachstum und deren Vermehrung. Bisher wurde angenommen, dass die bei der Chlamydien-Infektion beobachtete Aktivierung der Kinase Erk, die mit der Aktivierung der Phospholipase cPLA2, der Induktion des Interleukins 8 sowie der Stabilisierung des antiapoptotischen Faktors Mcl-1 in Verbindung steht, über den Ras/Raf/Mek-Signalweg vermittelt wird. Ich konnte jedoch zeigen, dass die Chlamydien-induzierte Erk-Aktivierung unabhängig von Ras und Raf1 stattfindet. Vielmehr wird während der Chlamydien-Infektion, Raf1, abhängig von der Kinase Akt, durch Phosphorylierung an Serin259 inaktiviert. Zudem wird das inaktivierte Raf1 zur bakteriellen Inklusion rekrutiert. Dies lässt vermuten, dass das Überleben derChlamydien und deren Wachstum nicht nur von der Erk-Aktivierung und dessen Substrate, sondern auch von der Inaktivierung von Raf1 und dessen Rekrutierung zur Inklusion abhängt. / Chlamydia trachomatis is a Gram-negative obligate intracellular bacterial pathogen with a major impact on human health. As an obligate intracellular pathogen, Chlamydia rely on host cell for all aspects of their survival. Here we present RNAi screen that identified 59 host cell genes influencing C. trachomatis infection and infectivity. Network analysis of hits revealed several prominent signaling networks, including Ras-Raf-MEK-ERK pathway. Knockdown of Ras and Raf1 components of the aforesaid pathway led to increased Chlamydial growth and survival. In Chlamydia infections, ERK activation is believed to be activated through upstream kinases Ras-Raf-MEK and involved in activation of cPLA2, induction of IL8 and stabilization of the anti-apoptotic Mcl-1. However, I could show that ERK activation after Chlamydia infection is independent of Ras and Raf1. Moreover, I also showed that Raf1 is inactivated by phosphorylation at Ser259 in an Akt dependent manner. Consequently, the Ser259 phosphorylated Raf1 was recruited to the Chlamydia inclusion in an Akt and 14-3-3β dependent manner. This strongly suggests that Chlamydia survival and replication in the host cell depends not only on the activation of ERK and its downstream targets such as cPLA2, but also on the inactivation of Raf1 by phosphorylation and recruitment to the inclusion.

siRNA

Chlamydia trachomatis

RNAi-Technologie

MAPK Signaltransduktion

siRNA

Chlamydia trachomatis

RNAi-Technology

MAPK signaling

570 Biowissenschaften, Biologie

32 Biologie

WF 6000

ddc:570

Functional gene analysis in cultured vertebrate cells using siRNA mediated gene silencing / Funktionelle Genanalyse in kultivierten Vertebratenzellen durch siRNA bewirkte Gensupression

Gruber, Jens

10 February 2005

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

RNA interferenz

siRNA

Transfektion

funktionelle Genanalyse

RNA interference

siRNA

transfection

functional gene analysis

42.13 Molekularbiologie

WF 200: Molekularbiologie

Biochemical and cell biological analysis of the mechanism of RNA interference in human cells / Biochemische und zellbiologische Analyse des RNA Interferenz Mechanismus in menschlichen Zellen

Agnieszka, Patkaniowska

18 January 2006

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

RNAi

siRNA

miRNA

Argonaute

Ago

Piwi

RNAi

siRNA

miRNA

Argonaute

Ago

Piwi

35.7

WF 200: Molekularbiologie

Piwi and piRNAs act upstream of an endogenous siRNA pathway to suppress Tc3 transposon mobility in the Caenorhabditis elegans germline / Piwi und piRNAs reprimieren Tc3 Transposon Mobilität in der Caenorhabditis elegans Keimbahn durch Regulation endogener siRNAs

Das, Partha Pratim

31 October 2008

No description available.

500 Naturwissenschaften allgemein

Mathematics and Computer Science

Argonaute

Piwi

piRNA

siRNA

transposon

Argonaute

Piwi

piRNA

siRNA

transposon

42.13

WF 200: Molekularbiologie

MED 417: Hämatologie

MED 424: Onkologie

Investigation of SNARE function in the early endosomal compartment / Untersuchung der Funktion von SNARE Proteinen im frühendosomalen Kompartiment

Bethani, Ioanna

29 April 2009

No description available.

000 Allgemeines

Wissenschaft

SNARE Proteinen

Fusion

frühe Endosomen

siRNA

SNARE

membrane fusion

early endosomes

siRNA

42

WHC 500: Organellen

Zellorganellen {Cytologie}

Die Rolle der Transkriptionsfaktoren “runt-related transcriptionfactor-2“ (RUNX2) und Osterix in humanen Osteoblasten / The role of transcription factors runt-related transcription factor-2 (RUNX2) and Osterix in human osteoblasts

Giesen, Markus

24 January 2008

No description available.

610 Medizin, Gesundheit

MED 419

Medicine

primäre humane Osteoblasten

siRNA

Transfektion

RUNX2

Osterix

primary human osteoblasts

siRNA

transfection

RUNX2

Osterix

44.89

Small interfering RNA-vermittelte Hemmung der Apoptoseinhibitoren BCL2, BCL-XL, XIAP und Survivin in Zellkultur- und Mausmodellen des humanen Harnblasenkarzinoms

Kunze, Doreen

03 January 2012

Das Harnblasenkarzinom (BCa) stellt in Deutschland die vierthäufigste Tumorneuerkrankung und die zehnthäufigste krebsbedingte Todesursache bei Männern dar. Nichtmuskelinvasive BCa werden organerhaltend aus der Blasenwand entfernt und zur Rezidiv- und Progressionsprophylaxe mittels intravesikaler Chemo- oder Immuntherapien behandelt. Trotz dieser adjuvanten Therapien, die mit starken Nebenwirkungen verbunden sein können, ist nur eine bedingte Minimierung des Rezidivrisikos möglich. Besonders im fortgeschrittenen Stadium weisen Harnblasenkarzinome eine schlechte Prognose auf. Obwohl das BCa eine chemosensitive Erkrankung darstellt, wird das Ansprechen auf lokale oder systemische Chemotherapien häufig durch auftretende Resistenzmechanismen limitiert. Daher stehen sowohl die Verbesserung konventioneller Chemotherapien als auch die Suche nach neuartigen Behandlungsstrategien im Fokus der experimentellen BCa-Forschung. Die Apoptose, eine Form des programmierten Zelltodes, ist ein essenzieller, streng regulierter biologischer Prozess, welcher der Aufrechterhaltung der Gewebshomöostase und der gezielten, entzündungsfreien Eliminierung geschädigter Zellen dient. Fehlregulationen in den Apoptosesignalwegen stellen ein zentrales Ereignis in der Tumorgenese dar und tragen außerdem zur Entstehung von Chemo- und Radiotherapieresistenzen bei. Eine wichtige Rolle in der Apoptoseregulation spielen die Mitglieder der BCL2- und der Inhibitor of Apoptosis Protein (IAP)-Familien, deren wichtigste antiapoptotische Vertreter BCL2, BCL-XL, XIAP und Survivin häufig in Tumoren, einschließlich des BCa, überexprimiert sind. Unter Verwendung von small interfering RNAs (siRNAs), synthetischen Nukleinsäurekonstrukten zur selektiven Geninhibition, wurde im Rahmen der Arbeit in vitro und in vivo untersucht, ob die Hemmung der Apoptoseinhibitoren BCL2, BCL-XL, XIAP und Survivin – allein und in Kombination mit Chemotherapie – eine Therapieoption zur Behandlung des BCa darstellen könnte. Da zur Tumorentstehung und -progression eine Vielzahl von genetischen Veränderungen beitragen, erscheint der Angriff eines einzelnen Zielgens unzureichend für eine effektive Tumortherapie. Aufgrund dessen wurde untersucht, ob durch simultane Reduktion der ausgewählten Apoptoseinhibitoren in BCa-Zellen stärkere wachstumsinhibitorische Effekte erzielt werden können. In der vorliegenden Arbeit wurde gezeigt, dass insbesondere die siRNA-vermittelte Hemmung von BCL-XL und Survivin in den BCa-Zelllinien EJ28 und J82 antiproliferative Effekte hervorruft und diese Tumorzellen gegenüber einer nachgeschalteten Chemotherapie mit Mitomycin C oder Cisplatin sensitiviert. Hingegen bewirkte sowohl die transiente als auch die stabile RNAi-induzierte Hemmung von BCL2 und XIAP in den untersuchten BCa-Monolayerzellkulturen, möglicherweise infolge kontinuierlicher Versorgung der Tumorzellen mit Sauerstoff und Nährstoffen, keine Reduktion des Tumorwachstums. Eine gegenüber den Einzelbehandlungen deutliche Verstärkung der antitumoralen und insbesondere der chemosensitivierenden Effekte in den BCa-Zelllinien wurde durch simultane Hemmung von BCL-XL und Survivin erzielt. Beispielsweise stieg der Anteil apoptotischer Zellen von 64 % nach Survivin-siRNA+Cisplatin-Behandlung auf 94 % nach gleichzeitiger BCL-XL+Survivin-Inhibition in Kombination mit Cisplatin. Folglich stellt die simultane Inhibition von BCL-XL und Survivin in Kombination mit Chemotherapeutika eine äußert viel versprechende BCa-Therapieoption dar. Tierexperimentelle Studien belegen die wachstumsinhibitorische Wirkung der Survivin-Reduktion und der kombinierten BCL-XL-siRNA+Chemotherapie-Behandlung, so wurde das Tumorendvolumen im Vergleich zur Kontrollbehandlung um 43 % bzw. um 48 % reduziert.

Harnblasenkarzinom

Apoptose

Chemotherapie

Chemosensitivierung

RNA-Interferenz

siRNA

small interfering RNA

bladder cancer

apoptosis

combination therapy

RNA interference

siRNA transfection

ddc:616

rvk:XH 7904

rvk:WG 7200

Análise da expressão e do silenciamento do receptor tipo 1 do fator de crescimento semelhante à insulina em tumores adrenocorticais humanos / Analysis of expression and silencing of insulin-like growth factor 1 receptor in human adrenocortical tumors

Tamaya Castro Ribeiro

12 January 2015

Introdução O sistema dos fatores de crescimento semelhantes à insulina (IGF) desempenha importante papel no crescimento e desenvolvimento celular normal. Hiperexpressão do gene IGF1R tem sido demonstrada em diversos tumores, sugerindo que a expressão deste receptor represente um pré-requisito fundamental para transformação celular. Nosso grupo de pesquisa demonstrou o aumento de expressão de IGF1R em tumores adrenocorticais pediátricos. Objetivos: Induzir o silenciamento do gene IGF1R por siRNA na linhagem de tumor adrenocortical humano NCI H295R, bem como avaliar os efeitos in vitro por meio da análise de proliferação celular e apoptose desta linhagem celular. Adicionalmente, avaliar a expressão de IGF-1R e de microRNAs relacionados a sua transcrição em tumores adrenocorticais humanos. Pacientes e métodos: A linhagem celular de carcinoma adrenocortical humano NCI H295R foi cultivada e submetida ao tratamento com 2 siRNAs específicos para IGF-1R. Todos os experimentos foram realizados em quatro grupos: (1) células não tratadas com siRNA, (2) células tratadas com siRNA # 1, (3) células tratadas com siRNA # 2 e (4) células tratadas com o siRNA controle negativo. A expressão gênica e proteica de IGF-1R foram determinadas por meio das técnicas de PCR em tempo real e Western Blot, respectivamente. Os efeitos do silenciamento de IGF-1R in vitro foram avaliados por ensaios de proliferação celular e análise de atividade de caspases. Além disso, 202 pacientes com tumor adrenocortical foram selecionados para o estudo de expressão proteica de IGF-1R por imunohistoquímica. Para avaliação de expressão de microRNAs relacionados à expressão de IGF-1R (miR-100, 375, 145 e 126) por PCR em tempo real foram selecionados 32 pacientes dos 202 disponíveis. Resultados: A expressão de IGF-1R foi significantemente diminuída nas células tratadas com siRNA # 1 e siRNA # 2. Os valores relativos de RNA mensageiro de IGF1R diminuíram aproximadamente 50% e as análises de Western Blot revelaram uma redução de 30% na proteína de IGF-1R. A diminuição de expressão foi acompanhada por uma redução de 40% na taxa de crescimento celular in vitro e um aumento de 45% das taxas de apoptose. A análise de expressão dos microRNAs 100, 375, 145 e 126 demostrou que a expressão de IGF-1R não se correlaciona com a expressão destes RNAs pequenos. Adicionalmente, a análise de expressão proteica de IGF-1R em tumores adrenocorticais humanos revelou que expressão forte (20%) de IGF-1R foi mais comum em carcinomas de adultos. Além disso, a imunolocalização do IGF-1R nos carcinomas (19%) foi mais frequentemente nuclear em relação aos adenomas de adultos. Conclusões: Os dados obtidos reforçam a importância de IGF-1R nas vias tumorigênicas das neoplasias malignas do córtex da glândula suprarrenal. A inibição deste receptor foi capaz de inibir o crescimento tumoral in vitro por meio da redução das taxas de proliferação celular e aumento da apoptose em linhagem celular de carcinoma adrenocortical humano. Além disso, a expressão proteica nuclear de IGF-1R foi mais comum entre os carcinomas, sugerindo representar um marcador biológico desta neoplasia / Introduction: The insulin-like growth factor (IGF) system plays a key role in normal cell growth and development. IGF1R overexpression has been demonstrated in several tumors suggesting that its expression is a prerequisite for cell transformation. We demonstrated IGF1R overexpression in pediatric adrenocortical tumors. Objectives: To induce IGF1R silencing by siRNA in a human adrenocortical cell line NCI H295R and evaluate its effects on cell proliferation and apoptosis. Additionally, evaluate the expression of IGF-1R protein and microRNAs related to its transcription in human adrenocortical tumors. Patients and methods: The human adrenocortical tumor cell line NCI H295R was cultured and treated with 2 specific IGF1R siRNA. All experiments were carried out in four groups: (1) untreated NCI H295R cells, (2) NCI H295R cells transfected with specific IGF1R siRNA # 1, (3) NCI H295R cells transfected with specific IGF1R siRNA # 2 and (4) NCI H295R cells transfected with a negative control. IGF-1R gene and protein expression was determined by the techniques of real-time PCR and Western blot, respectively. We assessed the effects of IGF-1R silencing on cell proliferation and apoptosis. Moreover, 202 patients with adrenocortical tumors were selected for the study of IGF-1R protein expression by immunohistochemistry. In the analysis of microRNAs that are related to IGF1R (miR-100, 375, 145 e 126) by real time PCR, 32 out 202 patients were selected. Results: IGF-1R levels were significantly decreased in cells that were treated with IGF-1R siRNA # 1 and siRNA # 2. The relative values of IGF1R mRNA decreased approximately 50% and Western blot analysis revealed a 30% of reduction in IGF-1R protein. Downregulation of this gene was accompanied by a reduction in 40% of cell growth in vitro and an increase in 45% of apoptosis. The analysis of microRNAs demonstrated that IGF1R expression is not correlated with the expression of these small RNAs. Additionally, the analysis of IGF-1R protein expression in human adrenocortical tumors revealed that strong expression (20%) of IGF-1R was more common in adult carcinomas. Moreover, the nuclear IGF-1R was more frequent in carcinomas diagnosed in adults (19%) when compared to adenomas. Conclusions: These data demonstrate the importance of IGF-1R in tumorigenic pathways of malignant neoplasms of the adrenocortical gland. IGF-1R silencing could inhibit tumor growth in vitro by reducing cell proliferation and increasing apoptosis in a cell line of human adrenocortical carcinoma. Furthermore, nuclear IGF-1R expression was more frequent in carcinomas diagnosed in adults, suggesting that IGF-1R may be a biological marker of this neoplasia

Imunohistoquímica

MicroRNAs

Neoplasias do córtex suprarrenal

Proteínas

Receptor IGF tipo 1

siRNA

Adrenal cortex neoplasms

Immunohistochemestry

MicroRNAs

Proteins

Receptor IGF type 1

siRNA

Influência do Gene APE1/REF-1 nas Respostas Celulares das Linhagens de Glioblastoma ao Quimioterápico Temozolomida / Influence of APE1/REF-1 Gene on Cellular Responses of Glioblastoma Cells to Chemotherapeutic Temozolomide

Ana Paula de Lima Montaldi

05 September 2013

A proteína APE1 (do inglêsApurinic/Apyrimidinicendonuclease 1/ Redox Factor-1 - APE1/REF-1) é uma enzima multifuncional, cuja expressão encontra-se frequentemente aumentada em gliomas. Além de apresentar atividade no reparo por excisão de base (BER), o gene APE1 também atua como fator de redução, mantendo fatores de transcrição (FTs) em um estado reduzido ativo. A via BER de reparo do DNA tem sido apontada como um possível fator de resistência a terapias baseadas no uso de agentes alquilantes, tais como temozolomida (TMZ). No presente trabalho, utilizou-se a estratégia de inibição da transcrição do gene APE1 pelo método de RNA interferente(siRNA) e tratamento com a droga TMZ nas células de glioblastoma (GBM), T98G (resistente à TMZ) e U87MG (sensível à TMZ), a fim de verificar a influência do silenciamento do gene APE1 sobre as respostas celulares à droga avaliadas por vários ensaios, bem como os efeitos sobre a expressão transcricional dos genes alvos dos FTs regulados por APE1. O silenciamento de APE1 e o tratamento das células T98G com a TMZ foram eficazes no sentido de reduzir a proliferação e a capacidade clonogênica, além de intervir na progressão do ciclo celular com bloqueio na fase S. Tais efeitos foram acompanhados pelo aumento da indução de danos no DNA e da expressão de H2AX fosforilada (H2AX), o que justifica a queda na sobrevivência celular. O mesmo efeito não foi observado nas células U87MG silenciadas para APE1 e tratadas com a TMZ, havendo o predomínio dos efeitos causados pela TMZ, exceto por uma leve indução de danos no DNA e de H2AX. Adicionalmente, nas células T98G silenciadas e tratadas, verificou-se uma moderada indução de apoptose, que foi observada ao longo dos tempos avaliados (1 a 10 dias), com uma leve indução de caspase-3 (5 dias); nessas células, observou-se também a indução (3,8 vezes) de morte celular autofágica (5 dias). Entretanto, nas células U87MG,a indução de apoptose foi baixa e não houve indução de morte por autofagia, sugerindo outros mecanismos de morte envolvidos na eliminação dessas células em resposta ao tratamento com a TMZ. O silenciamento de APE1 causou uma redução acentuada na invasão das células T98G, de forma similar à observada nas células somente tratadas com a TMZ, sendo que a combinação (silenciamento de APE1 e tratamento com a droga) resultou em um efeito aditivo, enquanto que nas células U87MG a combinação foi eficaz no sentido de reduzir a proporção de células invasivas, fato não observado nas condições isoladas. Os genes COX2 e VEGF, alvos dos FT NFB e HIF-1 (regulados por APE1) foram reprimidos nas células T98G enquanto que o gene VEGF foi induzido nas células U87MG, entretanto, tais alterações no padrão de expressão transcricional foram observadas somente em resposta ao tratamento com a TMZ, independentemente do silenciamento de APE1, indicando nenhuma mudança na atividade redox de APE1, possivelmente pela existência de proteínas APE1 remanescentes na célula. Além disso, a expressão proteica de NFBp65(ser563) foi aumentada em ambas as linhagens silenciadas e tratadas com a TMZ, provavelmente devido à inibição da proliferação celular. Em geral, os resultados do presente trabalho demonstraram que a estratégia de inibição do gene APE1 (participante da via BER) mostrou-se potencialmente viável, suportando a contribuição do BER na resistência à TMZ, visto que nas condições testadas, observou-se uma sensibilização das células de GBM, com efeito restrito às células de GBM resistentes (linhagem T98G), sendo pouco eficaz no sentido de sensibilizar as células sensíveis (linhagem U87MG) a esse agente. Assim, há que considerar as características genéticas de cada linhagem de GBM, visto que estas são cruciais para as respostas apresentadas pelas células aos tratamentos empregados. / APE1 (Apurinic/Apyrimidinic endonuclease 1/ Redox Factor-1 - APE1/REF-1) protein is a multifunctional enzyme whose expression is often increased in gliomas. Besides presenting activity in base excision repair (BER), APE1 also acts as a reduction factor, maintaining transcription factors (TFs) in an active reduced state. The BER pathway has been implicated as a possible factor of resistance to therapies based on the use of alkylating agents such as temozolomide (TMZ). In the present study, we have been using a strategy of small interference RNA (siRNA) to down-regulate the APE1 gene under conditions of treatment with TMZ in T98G (resistant to TMZ) and U87MG (sensitive to TMZ), glioblastoma (GBM), in order to determine the effects of APE1 gene silencing on cellular responses to this drug, evaluated by several assays, as well as the effects on the transcriptional expression of target genes of TFs regulated by APE1. APE1 silencing and TMZ treatment was effective to reduce the cell proliferation and clonogenic capacity of T98G cells, in addition to interfering in the cell cycle progression (S-phase arrest). These effects were accompanied by induction of DNA damage and phosphorylation of H2AX (H2AX), which may explain the decrease in cell survival. The same effect was not observed in silenced U87MG and TMZ-treated cells, being observed a predominance of the effects caused by TMZ itself, except for a slight induction of DNA damage and H2AX. Additionally, in silenced T98G and TMZ-treated cells, there was a moderate induction of apoptosis, as observed over time (1 to 10 days), with a slight induction of caspase-3 (on day 5); for those cells, we also observed autophagic induction (3.8 fold) at day 5. However, the induction of apoptosis and autophagy in U87MG cells was very low, suggesting that other mechanisms of cell death might be involved in the elimination of GBM cells under TMZ treatment. APE1 silencing caused a marked reduction on the invasiveness of T98G cells, similarly to that observed in TMZ treated cells, while the combination (APE1 silencing and drug treatment) led to an additive effect. For U87MG, the treatment combination was effective in reducing the proportion of invasive cells, in spite of an absence of any effect produced by each isolated condition tested. Regarding to the expression profile of target genes of TFs regulated by the APE1 redox activity, it was observed that COX2 and VEGF genes, targets of FTs NFB and HIF-1, were down-regulated in T98G while VEGF gene showed induced in U87MG cells; however, such alterations in the transcriptional expression pattern were observed only in response to TMZ treatment, independently of APE1 gene silencing, indicating no change in the APE1 redox activity, possibly due to the presence of APE1 remaining proteins inside cells. In addition, NFBp65(ser563) protein expression was increased in both cell lines (silenced and treated with TMZ), probably due to the reduced cell proliferation rates. In general, the present results show that the strategy of APE1 gene knockdown was potentially viable, supporting the BER contribution of the mechanism of TMZ resistance, since under the conditions tested, there was a sensitization of GBM cells. However, this effect was restricted to the resistant cell line (T98G cells). Thus, it should be considered the genetic characteristics of each GBM cell line, since these are crucial to the cellular responses to the conditions tested in the present work.

Gene APE1/REF-1.2

Glioblastoma

Reparo por excisão de base

Respostas a danos no DNA

siRNA

Temozolomida

APE1/REF-1 gene

Base excision repair

DNA damage responses

Glioblastoma

siRNA

Temozolomide