Transition of intrinsically unfolded α-synuclein into the fibrillar state characterized by NMR spectroscopy / Transition of intrinsically unfolded α-synuclein into the fibrillar state characterized by NMR spectroscopy

Cho, Min-Kyu

29 October 2008

No description available.

540 Chemie

Mathematics and Computer Science

NMR

α-synuclein

Amyloidfibrillen

Nativ entfaltete Proteine

NMR

α-synuclein

amyloid fibril

natively unfolded protein

35.99

SP 000: Strukturchemie

The identification of novel regulatory elements in the promoters of heat shock response genes

Ncube, Sifelani

January 2010

The main objective of this study was to investigate promoter sequences of putative HSR genes for the presence of unique regulatory elements and modules that might be involved in the regulation of HSR. In order to achieve this objective, an in silico promoter analysis strategy was devised, which focused on the identification of promoter sequences and regulatory elements, and modelling of promoter modules by using Genomatix software tools such as MatInspector and ModelInspector. Results showed that two modules (EGRF_SP1F_01 and SP1F_CEBP_01) were conserved in the promoter sequences of three well-known Hsp-genes (Hsp90, Hsp105β and αβ-crystallin). Screening the 60 target gene promoters for the presence of the two modules revealed that 12 genes (20 %) contained both modules. These included Moesin, Proline-4 hydroxylase, Poly(A) binding protein and Formin-binding protein. None of these genes had been previously associated with heat shock response.

Apoptosis

Cardiomyocytes

Cytoprotection

Heat shock proteins

Heat shock response

Inducible gene expression

Molecular chaperones

Real-time quantitative PCR

Regulatory elements

Unfolded protein response.

Effect of the unfolded protein response on MHC class I antigen presentation

Granados, Diana Paola

January 2008

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

CMH de classe I

Présentation antigénique

Antigène/peptide

Stress du RE

MHC class I

Antigen presentation

Peptide/antigen

ER stress

Unfolded protein response

Interface entre glicosilação pós-traducional e estresse de retículo em melanomas: alvo para sensibilização de células tumorais e agentes quimioterápicos? / Interface of post-translational glycosylation and ER stress in melanoma: target to cancer cell sensitization to chemotherapeutic agents?

Luiza Helena Madia Lourenço

26 July 2013

O melanoma é o tipo de câncer de pele mais letal, apesar de ser o menos incidente. Em virtude de sua alta letalidade e de sua crescente incidência, estudos sobre melanoma são de fundamental importância nos dias de hoje. Assim como células tumorais em geral, células de melanoma apresentam características metabólicas diferenciadas, como, por exemplo, altos níveis de espécies reativas de oxigênio e alta taxa de síntese proteica. Essas modificações no metabolismo dispararam vias de resposta a estresse, como a \"Unfolded Protein Response\" (UPR), contudo, essas células se adaptam a esse estresse constante, que não culmina com a morte das mesmas. Além disso, o padrão de glicosilação em células tumorais também é sabidamente alterado, entre outros motivos, pela expressão diferencial de enzimas da via de glicosilação, como a N-acetilglicosaminiltransferase 5 (MGAT5). Relacionando essas duas características de células de melanoma, propusemo-nos a avaliar se a alta expressão de MGAT5A ( e/ou MGAT5B) funcionaria como uma resposta adaptativa de células de melanoma ao estresse de retículo endoplasmático, e seria, portanto, responsável por manter o equilíbrio diferenciado nessas células. Durante o desenvolvimento desse estudo, foi possível comprovar que a indução de estresse de retículo por meio de tratamento com tunicamicina, um inibidor da N-glicosilação e indutor clássico de UPR, sensibilizou as células de melanoma ao posterior tratamento com cisplatina. Contudo, o tratamento com swainsonina, um inibidor do processamento dos N-glicanos que ocorre no complexo de Golgi, não foi capaz nem de disparar \"Unfolded Protein Response\" nem de induzir morte nessas células e, talvez por esse motivo, não apresentou efeito sensibilizador frente à cisplatina. Além disso, foi observado que as linhagens tumorigênicas apresentam maior expressão de MGAT5A em comparação à linhagem não-tumorigênica melan-a. As tentativas de realização de silenciamento de MGAT5A não foram exitosas. Informações relacionando estresse de retículo e N-glicosilação aberrante em células tumorais ainda serão foco de estudo em nosso grupo. Com os resultados apresentados, é possível concluir que o equilíbrio diferencial dos níveis de estresse de retículo em que se encontram as linhagens tumorigênicas do nosso modelo é importante para a sobrevivência das mesmas. Além disso, é de nosso interesse avaliar a dependência de células tumorais das vias ativadas pela superexpressão de MGAT5A, caso ela realmente exista / Melanoma is the most lethal skin cancer, despite being the least prevalent. Due to its lethality and resistance to a variety of known chemotherapeutic drugs, studies on melanoma are paramount. Tumor cells in general, and melanoma cells particularly, commonly present a disturbed metabolic rate, e.g., altered metabolism of reactive oxygen species and increased rates of protein synthesis. Altogether these perturbations trigger the Unfolded Protein Response (UPR); however, tumor cells are adapted to these conditions and are able to survive. Besides, glycosylation of tumor cells is commonly altered, due to differentiated expression rates of N-glycosylation enzymes, like N-acetylglucosaminyltransferase 5 (MGAT5). Considering these information together, we proposed that the sustained overexpression of MGAT5A (and/or MGAT5B) observed in Tm1 and Tm5 melanoma cells is part of an adaptive response to reticulum stress, maintaining an unstable equilibrium in tumor cells. In this work, we observed that the induction of endoplasmic reticulum stress caused by tunicamycin treatment, a N-glycosylation inhibitor and UPR inducer, sensitized melanoma cells to further cisplatin treatment. In contrast, swainsonine treatment, an inhibitor of Golgi N-glycan processing pathway, did not cause cell death nor UPR signaling, and this may be the reason why this treatment did not sensitize cells to cisplatin treatment. MGAT5A silencing was not successful yet. Altogether, the results above show that the unstable equilibrium under which Tm1 and Tm5 tumor cells are seems necessary for their survival. Therefore, it seems that upon malignant transformation, melanoma cells present dependence of MGAT5A expression. Its our interest exploit this melanoma model to understand the concept of oncogenic dependence for MGAT5A expression in the case of melanomas, if it exists

Estresse do retículo endoplasmático

Glicosilação

Melanoma

Resposta a proteínas não dobradas

Drug resistance neoplasm

Endoplasmatic reticulum stress

Glycosylation

Melanoma

Unfolded protein response

Indução de estresse de retículo endoplasmático como estratégia de quimiossensibilização de melanoma / Endoplasmic reticulum stress induction as a melanoma cell chemosensitization strategy

Renata de Freitas Saito

13 June 2014

de tumorigênese em melanomas, ainda não há tratamento eficaz para melanomas metastáticos. Esta ineficácia terapêutica pode estar relacionada com a adaptação e seleção de células de melanoma à indução de estresse de RE. Ultrapassar os níveis sustentados de estresse de RE, interferindo nas vias de adaptação a este estresse, foi o alvo deste estudo na tentativa de propor uma nova estratégia terapêutica para sensibilizar células de melanoma a morte induzida por cisplatina. Mostramos que GADD153, um dos componentes da via de UPR (Unfolded Protein Response) responsável por induzir apoptose em reposta ao estresse de RE, está excluída do núcleo em melanomas primários, metástases ganglionares e viscerais. Este dado sugere que a localização citoplasmática do fator de transcrição GADD153 possa estar envolvida na resposta adaptativa de melanomas ao estresse de RE, uma vez que se sabe que GADD153 se acumula no núcleo em resposta a este estresse. Investigamos se a indução de estresse de RE seria capaz de induzir a translocação de GADD153 para o núcleo e resultar na sensibilização de células de melanoma a morte induzida por cisplatina (CDDP). Realizamos o tratamento de células de melanoma (SbCl2, Mel85, SK-MEL- 29, SK-MEL-28 e SK-MEL-147) com tunicamicina (Tuni), indutor clássico de estresse de RE, previamente ao tratamento com CDDP. Demonstramos que em todas as linhagens exceto em SK-MEL-29, houve um aumento na porcentagem de células hipodiploides (>50%) no tratamento combinado (Tuni>CDDP) comparado ao tratamento com CDDP. As células SK-MEL-147 se mostraram mais sensíveis à indução de estresse de RE e as células SK-MEL-29 mais resistentes. Algumas diferenças entre estas linhagens como a expressão de GRP78 de superfície e presença de oligossacarídeos ?1-6 ligados de superfície podem estar relacionadas com esta resposta diferencial ao estresse de RE. Em todas as linhagens verificamos a acúmulo dos marcadores de UPR, GRP78 e GADD153, após o tratamento com tunicamicina. Além disso, GADD153 foi direcionada para o núcleo em reposta ao tratamento com tunicamicina. O acúmulo de vacúolos acídicos, da proteína autofágica LC3-II e de ROS após o tratamento com Tuni>CDDP, sugerem que tanto a autofagia quanto o estresse oxidativo parecem estar envolvidos na resposta de sensibilização. A inibição de autofagia com cloroquina aumentou a morte induzida por Tuni>CDDP, sugerindo que autofagia desempenha função protetora neste esquema terapêutico. Testamos um segundo agente genotóxico, temozolomida (TMZ), uma droga equivalente à dacarbazina, e a mesma capacidade de sensibilização foi observada pelo prévio tratamento com tunicamicina. A validação deste conceito in vivo foi dificultada pela acentuada toxicidade apresentada por tunicamicina. Avaliamos alguns candidatos a agentes estressores do RE que poderiam apresentar menor toxicidade celular, como swainsonina, atorvastatina, metformina e o composto de cobre [Cu2(apyhist)2(dpam)](ClO4)4. No entanto, não obtivemos resultados promissores com nenhum destes candidatos. Estes resultados mostram que as células tumorais podem ser pré-condicionadas à morte celular se expostas a um prévio estressor de RE, como Tuni, o que leva ao comprometimento da resposta adaptativa a indutores de morte celular como CDDP e TMZ. No entanto, ainda é necessário o estudo de agentes indutores de estresse de RE pouco tóxicos para que esta estratégia terapêutica possa ser utilizada em pacientes com melanoma / Melanoma is among the most aggressive malignancies with increasing worldwide incidence and there is no effective treatment for the metastatic disease. The absence of an effective therapy may be due to adaptation and selection of melanoma cells to endoplasmic reticulum (ER) stress. We showed that GADD153, one of the components of the ER stress-mediated apoptosis pathway, was mostly excluded from the nucleus of primary and metastatic melanoma cells compared to nevus cells. These data suggest that the unexpected GADD153 cellular localization could be involved in melanoma cell adaption to ER stress, since GADD153 accumulates in the nucleus during ER stress. Unfolded protein response (UPR) signaling induced in response to ER stress, is a dual process that induces a protective response to restore ER homeostasis or cell death if ER stress is severe or persistent. We investigated if induction of ER stress was a potential strategy to chemosensitize melanoma cells to a second insult by surpassing the adaptive levels to ER stress. We first treated human melanoma cells (SbCl2, SK-MEL-28, Mel85, SK-MEL-29 and SK-MEL-147) with tunicamycin (Tuni), an ER stress inducer, before cisplatin (CDDP) treatment. CDDP is a low cost chemotherapeutic drug currently used in Brazil as a second line for melanoma treatment, especially in youngsters. All cell lines, except SK-MEL-29, demonstrated an >50% increase in the percentage of hypodiploid cells with Tuni>CDDP treatment when compared to CDDP only. The same results were obtained with temozolomide (TMZ), equivalent drug to the active form of dacarbazine, the first line of cytotoxic treatment of melanomas. UPR markers, GRP78 and nuclear translocation of GADD153 were induced by Tuni. Differences between SK-MEL-29 and SK-MEL-147 as cell surface GRP78 and ?1-6 oligossacharides can be related with the differential ER stress sensitization observed in these cells. One of the cellular mechanisms that are regulated by ER stress is autophagy. Accordingly, we observed an increase in the acidic vesicular organelles and accumulation of LC3II in response to Tuni>CDDP treatment. Autophagy inhibition with chloroquine increased Tuni>CDDP induced-cell death, suggesting that autophagy plays a protective role in this response. Oxidative stress can be involved in this scenario since we demonstrated an accumulation of reactive oxygen species in response to Tuni>CDDP. Tunicamycin was cytotoxic in vivo and we investigated alternatives to this antibiotic as swainsonine, atorvastatin, metformin and [Cu2(apyhist)2(dpam)](ClO4)4 but we did not observed ER stress induction. These results indicate that tumor cells could be preconditioned to cell death if exposed to a first ER stressor, such as Tuni, which would compromise an effective adaptive response to a cell death inducer, as CDDP and TMZ. This combined approach may be a promising strategy for melanoma therapy but further studies are necessary to find noncytotoxic alternatives to tunicamycin

Autofagia

Cisplatino

Estresse de retículo endoplasmático

Fator de transcrição CHOP

Melanoma

Resposta a proteínas não dobradas

Autophagy

Cisplatin

Endoplasmic reticulum stress

Factor transcription CHOP

Melanoma

Unfolded protein response

The identification of novel regulatory elements in the promoters of heat shock response genes

Ncube, Sifelani

January 2010

Masters of Science / The main objective of this study was to investigate promoter sequences of putative HSR genes for the presence of unique regulatory elements and modules that might be involved in the regulation of HSR. In order to achieve this objective, an in silico promoter analysis strategy was devised, which focused on the identification of promoter sequences and regulatory elements, and modelling of promoter modules by using Genomatix software tools such as MatInspector and ModelInspector. Results showed that two modules (EGRF_SP1F_01 and SP1F_CEBP_01) were conserved in the promoter sequences of three well-known Hsp-genes (Hsp90, Hsp105β and αβ-crystallin). Screening the 60 target gene promoters for the presence of the two modules revealed that 12 genes (20 %) contained both modules. These included Moesin, Proline-4 hydroxylase, Poly(A) binding protein and Formin-binding protein. None of these genes had been previously associated with heat shock response. / South Africa

Apoptosis

Cardiomyocytes

Cytoprotection

Heat shock proteins

Heat shock response

Inducible gene expression

Molecular chaperones

Real-time quantitative PCR

Regulatory elements

Unfolded protein response

Contribution à la validation fonctionnelle du gène majeur contrôlant la dureté / tendreté de l'albumen du grain de blé par l'étude de lignées quasi-isogéniques / Contribution to functional validation of the major gene controlling hardness / softness trait in bread wheat endosperm of near-isogenic lines

Lesage, Véronique

15 December 2011

La dureté du grain de blé est un des paramètres fondamentaux de la texture de l’albumen. Ce caractère, essentiel pour la valeur d’utilisation des farines, est fortement lié à l’absence ou à la modification des puroindolines. Afin de mieux comprendre la fonction biologique de ces protéines dans le grain de blé (Triticum aestivum L.), nous avons étudié à quatre stades de développement du grain la localisation subcellulaire des puroindolines par immunocytochimie et les protéomes dans deux lignées de blé quasi-isogéniques pour la dureté. Dès la fin de la cellularisation de l’albumen, les puroindolines sont localisées sur la face interne des membranes vésiculaires et dans les corps protéiques en formation, structures dans lesquelles s’accumulent les protéines de réserve du grain. L’analyse par AFFFF (Asymmetrical Flow Field-Flow Fractionation) des deux lignées Hard et Soft, qui diffèrent essentiellement par l’absence du gène Pina dans la lignée Hard, a montré une corrélation entre la dureté et la taille des polymères de protéines de réserve. L’analyse protéomique des fractions albumines/globulines et amphiphiles des grains en développement a révélé une augmentation des protéines de la machinerie de repliement et de réponse au stress dans la lignée Hard, par rapport à la lignée Soft. Les deux approches méthodologiques utilisées semblent également mettre en évidence une cinétique de développement du grain raccourcie dans la lignée Hard. Ces observations suggèrent que les puroindolines interagissent avec les protéines de réserve du grain et suivent le même routage cellulaire. Elles pourraient être impliquées dans les mécanismes de repliement et d’assemblage des prolamines. / Wheat grain hardness, a major trait for endosperm texture and flour end-use properties, is strongly associated to absence or modification of puroindolines. To gain insight into biological function of those proteins in bread wheat kernel (Triticum aestivum L.), puroindolines’ subcellular localization was sought by immunocytochemistry and proteomes were analyzed at four stages of developing kernels in two near-isogenic lines for hardness, differing mainly in the absence of Pina in the Hardline. As early as the end of endosperm cellularisation, puroindolines were localized onto vesicular membranes and into protein bodies, where storage proteins accumulate. Using AFFFF (Asymmetrical Flow Field-Flow Fractionation), we observed a correlation between hardness and storage protein polymer size. Proteomic analyses of the albumin/globulin and amphiphilic fractions revealed an increase in folding and stress-related proteins in the Hard line, as compared to the Soft one. Both ultrastructural and proteomic studies suggested also that the Hard/Soft genotype affects the kinetics of kernel development. These lines of evidence imply that puroindolines interact with storage proteins and display the same routage. Puroindolines could therefore be involved in prolamines folding and assembly mechanisms.

Albumen

Blé

Développement du grain

Dureté

Protéines de réserve

Puroindolines

UPR

Stress oxydant

Endosperm

Hardness

Kernel development

Oxidative stress

Puroindolines

Storage proteins

Unfolded Protein Response

Wheat

Respons på oveckade proteiner : kan plasmid pEGFP-XBPdeldDBD-STOP-tagRFPt användas för detektion av celler vars endoplasmatiska retikulum är stressat? / Unfolded Protein Response : can plasmid pEGFP-XBPdeldDBD-STOP-tagRFPt be used for detection of cells whose endoplasmatic reticulum is stressed?

Wiklund, Magdalena

January 2016

Bakgrund: Endoplasmatiskt retikulum upprätthåller proteinhomeostasen genom syntes och degradering av proteiner. Tre signalvägar reglerar processen via ”unfolded protein response” på olika sätt. Inositol-requiring enzyme 1 alpha är en signalväg aktiverad av en störd proteinhomeostas. Stressen uppstår om cellen utsätts för kemiska substanser t.ex. i samband med djurförsök vid framtagning av läkemedel. Den aktiverade signalvägens respons leder bl.a. till splicing av X-box-binding Protein 1 mRNA. Syfte: Projektets syfte är att minska behovet av djurförsök genom att möjliggöra ökad implementering av 3R-principen. Frågeställningen är om den fluorescerande plasmiden pEGFP-XBP1∆dDBD-STOP-tagRFPt som binder till X-box binding protein 1 mRNA kan användas för detektion av celler vars endoplasmatiska retikulum är stressat. Metod: Plasmid pEGFP-XBP1∆dDBD-STOP-tagRFPt renades ur DH5-Alpha Escherichia coli med JETstar 2.0 Plasmid Purification Midiprep Kit. Humana epiteliala njurceller 293 transfekterades med plasmiden varpå de doserades med tunicamycin. Kontrollen utgjordes av dimetylsulfoxid. Mikroskopering skedde i fluorescensmikroskopet Zeiss Axiovert 200. Mjukvaran AxioVision Ver. 4.8.1.0. Carl Zeiss Imaging Solutions framställde cellerna på dataskärm. Resultat: Hypotestestets signifians bestämdes till p < 0,05. Resultatet antyder att antalet ER- stressade celler ökar med ökande inkubationstid (p = 0,001 – 0,966). En mindre antydan finns också mot en ökande koncentration av tunicamycin (p = 0,096 – 0,690). Slutsats: En rimlig slutsats kan inte dras då antalet utförda analyser är för få. / Background: Endoplasmic reticulum maintains protein homeostasis by protein synthesis and degradation. Three signal paths regulates the process by ”unfolded protein response” in different ways. Inositol-requiring enzyme 1 alpha is one path activated by a disturbed protein homeostasis. Stress starts if the cell is exposed to chemical substances as in connection with scientific animal experiments when pharmaceuticals are developed. The response of the activated signal path leads e.g. to splicing of X-box-binding protein 1 mRNA. Object: The object of the project is to reduce the need of scientific animal experiments by enabling increased implementation of the 3R principle. The question is if the fluorescent plasmid pEGFP-XBP1∆dDBD-STOP-tagRFPt binding to X-box binding protein 1 mRNA can be used for detection of cells whose endoplasmatic reticulum is stressed. Method: Plasmid pEGFP-XBP1 ∆ dDBD-STOP-tagRFPt was purified from DH5-Alpha Escherichia coli with JETstar 2.0 Plasmid Purification Midiprep Kit. Human epithelial kidney cells 293 were transfected with the plasmid whereupon they were dosed with tunicamycin. The control was made off dimethylsulfoxide. Microscopy was done in the fluorescence microscope Zeiss Axiovert 200. The software AxioVision Ver. 4.8.1.0. Carl Zeiss Imaging Solutions imaged cells on the computer screen. Result: The significans of the hypothesis test was set to p < 0,05. The result suggests that the number of ER-stressed cells increase with increasing incubation time (p = 0,001 – 0,966). A smaller hint is also pointing toward increasing concentrations of tunicamycin (p = 0,096 – 0,690). Conclusion: A reasonable conclusion cannot be made because of too few tests.

unfolded protein response

plasmid

fluorescence

microscopy

3R

respons på oveckade proteiner

plasmid

fluorescens

mikroskopi

3R

Biomedical Laboratory Science/Technology

Characterization of a novel regulator of the unfolded protein response in Ustilago maydis and mammals

Martorana, Domenica

05 June 2019

No description available.

570

UPR

IRE1a

XBP1s

XBP1u

Ustilago maydis

cell culture

clonogenic survival

transcriptional activity

luciferase assay

Cib1u

unfolded protein response

Cib1s

bZIP transcription factor

Ustilago maydis

Biologie (PPN619462639)

Interplay of Verticillium signaling genes favoring beneficial or detrimental outcomes in interactions with plant hosts

Starke, Jessica

22 July 2019

No description available.

570

Biologie (PPN619462639)