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對當代新儒家的實踐問題之探討:勞思光的政治哲學孫善豪, Sun, Shan-Hao Unknown Date (has links)
本論文共乙冊,凡十萬字,分為八章,首章緒論,說明本論文研究之目的、方法與主
要論題;次章總論實踐之意義,及其與當代新儒家之關聯;三、四章討論唐君毅與牟
宗三理論中對實踐問題的態度;五、六、七章就勞思光的思想討論其所謂近百年來之
「中國苦難」的本質、苦難的解除,及解除行動之著手處等問題,而顯豁其實踐哲學
之內容。末章結論,則對勞思光思想針對唐君毅、牟宗三思想之可能補益進行討論,
並進而檢討此補益中之缺陷,期能對當代新儒家之實踐問題提供更為整全的解決。
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Caractérisation des transcrits antisens chez les rétrovirus HTLV et étude comparative des fonctions des protéines traduites à partir de ces transcrits antisensLarocque, Émilie 04 1900 (has links)
Le premier membre de la famille des rétrovirus humains HTLV (Virus T-lymphotropique Humain), HTLV-1, a été découvert en 1980 et l’on estime aujourd’hui à plus de 10 millions le nombre d’individus infectés à travers le monde. Après une période de latence d’environ 40 ans, 5% des individus infectés développent des leucémies, des lymphomes adultes de lymphocytes T (ATLL) ou encore une myélopathie associée à HTLV-1/ paraparésie spastique tropicale (HAM/TSP). L’apparition de la maladie serait en grande partie orchestrée par deux protéines virales, soit Tax et HTLV-1 bZIP factor (HBZ). L’expression du génome viral se fait à partir d’un transcrit sens de pleine longueur suite à un épissage alternatif, à l’exception du gène HBZ. HBZ est produite à partir d’un transcrit antisens initié dans la séquence terminale longue répétée (LTR)’3. Elle a été décrite comme étant capable de réguler négativement la transcription virale dépendante de Tax en se dimérisant avec des facteurs de transcription cellulaires tels que CREB-2 et certains membres de la famille Jun. HBZ a aussi un pouvoir prolifératif et bien que nous ne sachions toujours pas le mécanisme moléculaire menant à l’oncogenèse par HBZ, nous savons qu’elle module une multitude de voies de transduction de signaux, dont AP-1. Nous avons récemment mis en évidence un transcrit antisens nommé Antisense Protein of HTLV-2 (APH-2) chez HTLV-2 qui n’est associé qu’à une myélopathie apparentée au HAM/TSP. Ce n’est qu’en 2005 que HTLV-3 et HTLV-4 se sont rajoutés au groupe HTLV. Cependant, aucune corrélation avec le développement d’une quelconque maladie n’a été montrée jusqu’à ce jour. Le premier volet de ce projet de doctorat avait pour objectif de détecter et caractériser les transcrits antisens produits par HTLV-3 et HTLV-4 et d’étudier les protéines traduites à partir de ces transcrits pour ainsi évaluer leurs similitudes et/ou différences avec HBZ et APH-2. Nos études de localisation cellulaire réalisées par microscopie confocale ont montré que APH-3 et APH-4 sont des protéines nucléaires, se retrouvant sous la forme de granules et, dans le cas d’APH-3, partiellement cytoplasmique. Ces granules co-localisent en partie avec HBZ. Les analyses à l’aide d’un gène rapporteur luciférase contenant le LTR 5’ de HTLV-1 ont montré que APH-3 et APH-4 peuvent aussi inhiber la transactivation du LTR 5’ par Tax. Aussi, des études faisant appel au gène rapporteur précédé d’un promoteur de collagénase (site AP-1), ont montré que ces deux protéines, contrairement à HBZ, activent la transcription dépendante de tous les membres des facteurs de transcription de la famille Jun. De plus, les mutants ont montré que le motif fermeture éclair (LZ) atypique de ces protéines est impliqué dans cette régulation. En effet, APH-3 et APH-4 modulent la voie Jun-dépendante en se dimérisant via leur LZ atypique avec la famille Jun et semblent activer la voie par un mécanisme ne faisant pas par d’un domaine activateur autonome. Dans un deuxième volet, nous avions comme objectif d’approfondir nos connaissances sur la localisation nucléolaire de HBZ. Lors de nos analyses, nous avons identifié deux nouveaux partenaires d’interaction, B23 et la nucléoline, qui semblent être associés à sa localisation nucléolaire. En effet, ces interactions sont plus fortes suivant une délétion des domaines AD et bZIP de HBZ qui dans ce cas est localisée strictement au nucléole. De plus, bien que APH-3 et APH-4 puissent se localiser aux nucléoles, HBZ est la seule protéine traduite à partir d’un transcrit antisens pouvant interagir avec B23. Finalement, ces travaux ont clairement mis en évidence que HTLV-3 et HTLV-4 permettent la production de transcrits antisens comme chez d’autres rétrovirus. Les protéines traduites à partir de ces transcrits antisens jouent d’importants rôles dans la réplication rétrovirale mais semblent avoir des fonctions différentes de celles de HBZ au niveau de la régulation de la transcription de la voie Jun. HBZ semble aussi jouer un rôle unique dans le nucléole en ciblant les protéines nucléolaires de la cellule. Ces études démontrent que les protéines produites à partir de transcrits antisens chez les rétrovirus HTLV partagent plusieurs ressemblances, mais démontrent aussi des différences. Ainsi, les APH pourraient, en tant qu’outil comparatif, aider à mieux cibler les mécanismes moléculaires importants utilisés par HBZ pour induire la pathogénèse associée à une infection par HTLV. / The first human T-cell lymphotropic virus (HTLV) family member was discovered in 1980 and it is estimated that approximately 10 million people are infected with HTLV-1 worldwide. After about 40 years, 5% of infected individuals will develop an adult T-cell leukemia/lymphoma (ATLL) while another 4% will develop HTLV-1-associated myelopathy/tropical spastic paraparesis (HAM/TSP). It is believed that two viral proteins, Tax and HBZ, together orchestrate the oncogenic process. The viral proteins are expressed from an alternatively spliced sense transcript except for the HBZ gene. HBZ is translated from an antisense transcript initiated in the long terminal repeat (LTR)’3. This viral protein is capable of inhibiting Tax transactivation of the LTR5’ by dimerizing with cellular transcription factors such as CREB-2 and c-Jun. HBZ also has proliferating capacities and while the molecular mechanisms leading to the disease still need to be elucidated, it is well known that HBZ can modulate a multitude of signal transduction pathways like AP-1. We have recently discovered an antisense transcript termed Antisense Protein of HTLV-2 (APH-2) produced in HTLV-2. HTLV-2 is only associated to myelopathies resembling HAM/TSP. HTLV-3 and HTLV-4 were discovered in 2005 and have not been associated with any type of disease thus far. The first goal of this PhD project was hence to detect and characterize the antisense transcripts produced in HTLV-3 and HTLV-4, to study the functions of these translated proteins and to evaluate their similarities and/or differences shared with HBZ and APH-2. Our localization studies using confocal microscopy demonstrated that APH-3 and APH-4 are found in the nucleus as speckles, and for APH-3, also partially cytoplasmic. These two proteins can also partially colocalize with HBZ. Using a luciferase reporter plasmid bearing the HTLV-1 LTR5’, we demonstrated that APH-3 and APH-4 could inhibit Tax transactivation of the LTR5’. We also used a luciferase reporter plasmid bearing the collagenase promoter, which bears an AP-1 site, and demonstrated that both viral proteins could activate transcription in the presence of any of the Jun family of transcription factors. We generated several mutants and the atypical leucine zipper (LZ) found in APH-3 and APH-4 is crucial for this regulation. In fact, APH-3 and APH-4 using their atypical LZ dimerize with Jun family members and activate this pathway using a mechanism other than an autonomous activation domain. Our next goal was to investigate the significance of the HBZ nucleolar localization. During this project, we identified two new interacting partners, B23 and nucleolin, which seem to be associated with its nucleolar localization. In fact, these interactions are stronger when HBZ is deleted of its AD and bZIP domains and hence when HBZ demonstrates a stronger nucleolar distribution. Moreover, while APH-3 and APH-4 are also found in the nucleolus, HBZ is the only antisense protein able to interact with B23. Finally, this work clearly demonstrates that HTLV-3 and HTLV-4 can produce an antisense transcript alike other retroviruses. The encoded proteins play an important role in retroviral replication and seem to regulate Jun-dependant transcription differently than HBZ. HBZ also seems to have a unique role in the nucleoli by targeting specific cellular nucleolar proteins. Similarities but also differences are shared between the antisense proteins. Thus, the APH proteins represent a good comparative tool in order to better understand the molecular mechanisms involved in HTLV induced diseases.
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A Study on the Change of Chinese Oil Painting in Art MarketYeh, Wei-lih 10 September 2009 (has links)
The purposes of this thesis are probing into the change of Chinese Oil Painting in art market. By means of this study, we will able to understand the development processes of the art markets in China, on the other hand, to gather the data from the auction market of different age artists and analysis them. Furthermore, it¡¦s the way to clarify how strong the art market in China is, or just the strategy to sensationalize the whole market to get high attention. But, it¡¦s obvious to find out that the environment affects the artists¡¦ creation a lot, but the works in the art market will go by chance. Therefore, to conclude that the Chinese art market is immature because the position of Chinese oil paintings is not fixed by Chinese government, Chinese artists and Chinese art market, but the art market in the world. Consequently, the Chinese art market needs to connect with the international art market.
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Διερεύνηση μηχανισμών χημειοαντίστασης στην οξεία μυελογενή λευχαιμία με έμφαση στο ρόλο ενδοκυττάριων μονοπατιών μεταγωγής σήματοςΛαγκαδινού, Ελένη 26 October 2009 (has links)
Η θεραπεία της Οξείας Μυελογενούς Λευχαιμίας (ΟΜΛ) είναι συχνά ανεπιτυχής λόγω ανάπτυξης κυτταρικής αντίστασης στα αντιλευχαιμικά φάρμακα. Εκτός από την έκφραση Ρ-γλυκοπρωτείνης στα λευχαιμικά κύτταρα, άλλοι κυτταρικοί παράγοντες μπορούν επίσης να συμβάλλουν στην χημειοαντίσταση. Η c- Jun N-terminal Kinase (JNK) είναι μία πρωτεινική κινάση που ενεργοποιείται όταν τα κύτταρα εκτεθούν σε χημειοθεραπευτικά φάρμακα (ΧΜΘ). Πρόσφατες μελέτες σε συμπαγείς όγκους συσχετίζουν την χημειοαντίσταση με αδυναμία των καρκινικών κυττάρων να ενεργοποιήσουν τη JNK κατόπιν επίδρασης ΧΜΘ. Σκοπός της εργασίας είναι να διερευνήσει αν η χημειοαντίσταση στην ΟΜΛ οφείλεται σε ενδογενή αδυναμία των λευχαιμικών βλαστών να ενεργοποιήσουν τη JNK. Μεθοδολογία: Συγκρίναμε ευαίσθητες (U937) και ανθεκτικές (U937R) στις ανθρακυκλίνες κυτταρικές σειρές ΟΜΛ ως προς την δυνατότητα in vitro ενεργοποίησης της JNK κατόπιν επίδρασης ΧΜΘ (Western Blot). Επιπλέον, στις λευχαιμικές κυτταρικές σειρές ελέγξαμε απευθείας τη σημασία της JNK στην χημειοαντίσταση με πειράματα α) αποσιώπησης της JNK με JNK1–στοχεύον siRNA και β) ενεργοποίησης της JNK (διαμόλυνση με τον ΜΚΚ4/SEK1 άνωθεν ενεργοποιητή της JNK) Περαιτέρω, ελέγξαμε την in vitro δυνατότητα ενεργοποίησης της JNK σε 29 πρωτογενή μυελικά δείγματα ΟΜΛ κατόπιν βραχείας διάρκειας (30-60min) έκθεση στην daunorubicin (1μΜ) και συσχετίσαμε τα εργαστηριακά δεδομένα με κλινικά χαρακτηριστικά των ασθενών με ΟΜΛ. Αποτελέσματα: In vitro θεραπεία των U937 κυττάρων με ανθρακυκλίνες προκάλεσε ισχυρή και ταχεία ενεργοποίηση της JNK και απόπτωση. Αντίθετα, στα πολυανθεκτικά U937R κύτταρα δεν παρατηρήθηκε ενεργοποίηση της JNK, ακόμη και σε συνθήκες υψηλής ενδοκυττάριας συγκέντρωσης ανθρακυκλινών. Αποσιώπηση της JNK στα ευαίσθητα U937 κύτταρα τα έκανε ανθεκτικά στις ανθρακυκλίνες (JNK1-siRNA διαμολυσμένα U937 κύτταρα εμφάνισαν 50.4% και 61.3% ελαττωμένη daunorubicin- (DNR, 1μΜ 24hr) και doxorubicin- (DOX, 1.5μΜ 24hr) προκαλούμενη απόπτωση αντίστοιχα, συγκριτικά με U937 κύτταρα-μάρτυρες, P<0.001). Αντίστροφα, εκλεκτική ενεργοποίηση της ανενεργού JNK στα ανθεκτικά U937R κύτταρα τα έκανε 3.3 φορές πιο ευαίσθητα στη DNR και 3.1 φορά πιο ευαίσθητα στη DΟΧ, συγκριτικά με U937R κύτταρα-μάρτυρες. Επιπρόσθετα, παρατηρήσαμε ισχυρή συσχέτιση μεταξύ των in vitro φαρμακοδυναμικών αλλαγών των επιπέδων ενεργοποίησης της JNK στους λευχαιμικούς βλάστες και της ανταπόκρισης των ασθενών με ΟΜΛ στη χημειοθεραπευτική αγωγή (P=0.012). Η απουσία ενεργοποίησης της JNK στα βλαστικά κύτταρα συσχετίστηκε επίσης με αρνητικούς προγνωστικούς παράγοντες για την ΟΜΛ, όπως γηραιότερη ηλικία των ασθενών (P=0.046) και ΟΜΛ αναπτυσσόμενη επί εδάφους μυελοδυσπλασίας (P=0.017).
Συνοψίζοντας, τα in vitro και in vivo αποτελέσματα μας προτείνουν την ενδογενή αποτυχία ενεργοποίησης της πρωτεινικής κινάσης JNK στους λευχαιμικούς βλάστες σαν έναν εναλλακτικό μηχανισμό χημειοαντίστασης στην ΟΜΛ. Η διελεύκανση των μηχανισμών εκείνων που επιφέρουν καταστολή της JNK στην χημειοανθεκτική ΟΜΛ μπορεί να ωφελήσει θεραπευτικά. / Chemotherapy resistance is a major challenge in acute myeloid leukemia (AML). Besides the P-glycoprotein efflux, additional cellular factors may contribute to drug-resistance in AML. c- Jun N-terminal Kinase (JNK) is activated after exposure of cells to chemotherapeutics. We asked whether chemoresistance in AML is attributed to intrinsic failure of the AML blasts to activate JNK. In vitro treatment of U937 AML cell line with anthracyclines induced a rapid and robust JNK phosphorylation and apoptosis. In contrast, the anthracyline-resistant derivative cell lines U937R and URD40 showed no JNK activation after exposure to anthracyclines, also at doses that resulted in high accumulation of the drug within the cells. RNA interference-based depletion of JNK1 in drug-sensitive U937 cells made them chemoresistant, whereas selective restoration of the inactive JNK pathway in the resistant U937R cells sensitized them to anthracyclines. Short-term in vitro exposure of primary AML cells (n=29) to daunorubicin showed a strong correlation between the in vitro pharmacodymanic changes of phospho-JNK levels and the response of patients to standard induction chemotherapy (P=0.012). We conclude that JNK activation failure confers another mechanism of anthracycline resistance in AML. Elucidating the ultimate mechanisms leading to JNK suppression in chemoresistant AML may be of major therapeutic value.
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TRAF6 stimulates TGFβ-induced oncogenic signal transduction in cancer cells / TRAF6 stimulerar TGFβ-inducerad onkogen signal transduction i cancerceller.Gudey, Shyam Kumar January 2014 (has links)
Prostate cancer is one of the leading causes of cancer-related deaths in men worldwide, with 10,000 new cases/year diagnosed in Sweden. In this context, there is an urgent need to identify new biomarkers to detect prostate cancer at an initial stage for earlier treatment intervention. Although how prostate cancer develops has not been fully established, the male sex hormone testosterone is a known prerequisite for prostate cancer development. High levels of transforming growth factor-β (TGFβ) are prognostically unfavorable in prostate cancer patients. TGFβ is a multifunctional cytokine that regulates a broad range of cellular responses. TGFβ signals through either the canonical Smad or the non-Smad signaling cascade. Cancerous cells develop different strategies to evade defense mechanisms and metastasize to different parts of the body. This thesis unveils one such novel mechanism related to TGFβ signaling. The first two articles provide evidence that TGFβ receptor type I (TβRI) is ubiquitinated by tumor necrosis factor receptor-associated factor 6 (TRAF6) and is cleaved at the ectodomain region by tumor necrosis factor alpha converting enzyme (TACE) in a protein kinase C zeta type-dependent manner. After TβRI is shed from the ectodomain, it undergoes a second cleavage by presenilin 1 (PS1), a γ-secretase catalytic subunit, which liberates the TβRI intracellular domain (TβRI-ICD) from the cell membrane. TRAF6 promotes TGFβ-dependent Lys63-linked polyubiquitination and recruitment of PS1 to the TβRI complex, and facilitates the cleavage of TβRI by PS1 to generate a TβRI-ICD. The TβRI-ICD then translocates to the nucleus, where it binds with the transcriptional co-activator p300 and regulates the transcription of pro-invasive target genes such as Snail1. Moreover, the nuclear translocated TβRI-ICD cooperates with the Notch intracellular domain (NICD), a core component in the Notch signaling pathway, to drive the expression of invasive genes. Interestingly, treatment with g-secretase inhibitors was able to inhibit cleavage of TβRI and inhibit the TGFβ-induced oncogenic pathway in an in vivo prostate cancer xenograft model. In the third article, we identified that Lysine 178 is the acceptor lysine in TβRI that is ubiquitinated by TRAF6. The TβRI K178R mutant was neither ubiquitinated nor translocated to the nucleus, and prevented transcriptional regulation of invasive genes in a dominant negative manner. In the fourth article, we show that TGFβ utilizes the E3-ligase TRAF6 and the p38 mitogen-activated protein kinase to phosphorylate c-Jun. In turn, the phosphorylated c-Jun activates p21 and Snail1 in a non-canonical Smad-independent pathway, and thereby promotes invasion in cancerous cells. In summary, we elucidate a new mechanism of TGFβ-induced oncogenic signal transduction in cancer cells in which TRAF6 plays a fundamental role. This opens a new avenue in the field of TGFβ signaling.
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The role of mitochondria in regulating MAPK signalling pathways during oxidative stressPang, Wei Wei January 2006 (has links)
[Truncated abstract] Reactive oxygen species (ROS) have been implicated to play a major role in many pathological conditions including heart attack and stroke. Their ability to modulate the extracellular signal-regulated protein kinase (ERK) and c-Jun Nterminal kinase (JNK) signalling pathways, thereby influencing cellular response has been well-documented. Recent studies implicate a central role for mitochondria in ERK and JNK activation by ROS although the mechanisms remained unresolved. Using Jurkat T-lymphocyte as a cell model, this study demonstrated increased mitochondrial ROS production as a result of decreased mitochondrial complex activities mediated by hydrogen peroxide treatment. This is the first study to show that mitochondria are not essential for activating ERKs, however damaged mitochondria producing ROS can be expected to cause sustained ERK activation . . . This study revealed that JNK and its upstream kinases MKK4, MKK7 and ASK1 are associated with the mitochondria. Furthermore, findings from this study imply that JNK resides in the mitochondrial matrix. This study is the first to demonstrate that mitochondrial JNK can be activated in a cell-free environment by signals originating from the mitochondria. Experimental work using isolated mitochondria demonstrated that mitochondrial JNK can be activated by ROS generated from the mitochondria themselves. Flavin-containing proteins appear to be the main sources of mitochondrial-ROS which signal through redoxsensitive proteins to activate mitochondrial JNK.
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Grafico misto de controle da media com amostragem em dois estagiosSampaio, Elvis dos Santos 20 July 2012 (has links)
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Previous issue date: 2012-07-20 / This paper proposes a new control chart to monitor a process mean employing a combined npx-X control chart. Basically the procedure consists of splitting the sample of size n into two sub-samples n1 and n2 determined by an optimization search. The sampling occur in two-stages. In the first stage the units of the sub-sample n1 are evaluated by attributes and plotted in npx control chart. If this chart signs then units of
second sub-sample are measured and the monitored statistic plotted in X control chart (second stage). If both control charts sign then the process is stopped for adjustment. The possibility of non-inspection in all n items may promote a reduction not only in the cost but also the time spent to examine the sampled items. Performances of the current proposal, individual X and npx control charts are compared. In this study the
proposed procedure presents many competitive options for the X control chart for a sample size n and a shift from the target mean. The average time to sign (ATS) of the current proposal lower than the values calculated from an individual X control chart points out that the combined control chart is an efficient tool in monitoring process mean. / Esta disserta??o prop?e um novo gr?fico (ou procedimento) de controle para monitorar a centralidade de um processo (m?dia) por meio da jun??o dos gr?ficos X e npx. Basicamente o procedimento consiste em dividir a amostra de tamanho n em duas (n1 e n2), definidas pelo processo de otimiza??o. Realiza-se a amostragem em dois est?gios. No primeiro est?gio conta-se o n?mero de itens n?o conformes amostra
de tamanho n1 por meio do gr?fico npx. Caso haja um n?mero excessivo de itens n?o conformes, segue-se para o segundo est?gio da amostragem, onde calcula-se a m?dia X
da amostra de tamanho n2. A possibilidade de n?o inspecionar todos os itens reduz tanto o custo quanto o tempo gasto para inspecionar os itens da amostra. Descreve-se a metodologia de constru??o, avalia??o e o funcionamento do gr?fico aqui proposto, e com o aux?lio do software estat?stico Rc e feito um estudo comparativo entre os gr?ficos individuais X e npx e o gr?fico misto. Neste estudo verificou-se que o procedimento
proposto fornece v?rias op??es concorrentes com o gr?fico X para um dado tamanho de amostra n e um desvio na m?dia . Os valores do tempo esperado at? o sinal (TES)
inferiores aos provenientes do gr?fico individual X evidenciaram que o gr?fico misto ? uma ferramenta eficaz no monitoramento de processos capaz de substituir o gr?fico da m?dia
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Mecanismos de jun??o em textos acad?micos: uma abordagem sist?mico-funcionalMendes, Wellington Vieira 22 August 2016 (has links)
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Previous issue date: 2016-08-22 / Coordena??o de Aperfei?oamento de Pessoal de N?vel Superior (CAPES) / A observa??o do modo como se organizam os textos acad?micos permite o entendimento dos mecanismos de constru??o dos sentidos nos diferentes estratos dos sistemas discursivos. Al?m das caracter?sticas lexicogramaticais que se configuram na superf?cie dos textos, o reconhecimento dos contextos em que s?o produzidos possibilita tamb?m compreend?-los como sendo resultantes de processos de constru??o de sentidos complexos e articulados nesses sistemas, tal como definido pela Lingu?stica Sist?mico-Funcional (LSF). Este estudo se filia aos modelos de sistemas discursivos propostos por Martin e Rose (2007), aos estudos de coes?o desenvolvidos em Halliday e Hasan (1976) e ? gram?tica sist?mico-funcional de Halliday e Matthiessen (2014). O foco e escopo do trabalho ? o fen?meno da jun??o com marcadores expl?citos ? aqui concebida como diferentes realiza??es da lexicogram?tica que, independentemente de seu estatuto ou extens?o, atuam na conflu?ncia de complexos oracionais. Neste caso espec?fico, o interesse se volta aos textos produzidos por graduandos e p?s-graduandos em Letras, a fim de: (i) identificar as rela??es de jun??o em textos acad?mico-cient?ficos produzidos por estudantes de gradua??o e de p?s-gradua??o; (ii) comparar os usos das rela??es de jun??o entre os textos produzidos por estudantes de gradua??o e p?s-gradua??o; (iii) apresentar contribui??es para as pr?ticas de escrita na academia a partir dos subs?dios te?ricos fornecidos pela LSF sobre articula??o textual. Para atendimento destes objetivos, a pesquisa analisa um corpus de 9,8 milh?es de palavras composto por artigos, monografias, disserta??es e teses da ?rea de Lingu?stica. Os dados foram recenseados com apoio de ferramentas dispon?veis nas aplica??es do WordSmith Tools (SCOTT, 2012), especificamente no tratamento quantitativo de amostras. ? guisa de resultados, ? poss?vel indicar que a jun??o com marcador expl?cito se situa com maior recorr?ncia nos textos de graduandos, mas colabora, indistintamente nos trabalhos de gradua??o e p?s-gradua??o, para a constru??o de sentidos no discurso porque configuram rela??es e atividades dentro do pr?prio texto e para al?m dele, tanto pelas passagens argumentativas de um t?pico a outro, como pelo emprego de recursos como met?frase, transposi??o e/ou amplia??o de sentidos quando esses componentes funcionais apontam para a experi?ncia ou idea??o e, noutros casos, para a organiza??o sequencial do texto. / The observation of how academic texts are organized provides the understanding of the meaning construction mechanisms in the different strata of the discursive systems. Besides the lexicogrammatical characteristics which configure on the surface of the texts, the contexts recognition in which they are produced also make it possible to understand them as a result of a complex process of meaning construction and articulated in these systems according to Systemic Functional Linguistics (SFL). The theoretical frameworks of this study are the discursive system model suggested by Martin and Rose (2007), the cohesion studies carried out by Halliday and Hasan (1976) and the Systemic-Functional Grammar by Halliday and Matthiessen (2014). The focus and objective of this research is the junction phenomenon with overt markers - here conceived as different lexicogrammatical realizations which, regardless their status or length, act in the confluence of clause complexes. In this specific case, the focus is shifted towards texts written by Letras undergraduate and graduate students. It aims at: (i) Identifying the relations of junction in academic texts written by undergraduate and graduate students; (ii) comparing the usages of relation of junctions within the texts written by undergraduate and graduate students; (iii) provide input to writing practices in the gym from the theoretical basis provided by LSF on textual articulation. To reach these objectives, the research analyzes a corpus of 9,8 million words composed of research articles, monographs, master?s dissertations and doctoral theses in Linguistics. The data were compiled with the support of the tools available for use on WordSmith Tools (SCOTT, 2012), specifically on the quantitative treatment of the samples. By way of results, it is possible to state that junction with overt marker shows a higher recurrence in the undergraduates? texts, but cooperate, indistinctly, with the undergraduates? and graduates? works, for the meaning construction in discourse because they configure relations and activities in the text itself and beyond, as much for the argumentative passages of a given topic or another, as for the usage of resources such as metaphrase, transposition and/or amplification of meanings when these functional components point out towards the experience or ideation and, in other cases, for the sequential organization of the text.
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Role of the JNK Signal Transduction Pathway in Cell Survival: a DissertationLamb, Jennifer A. 15 December 2004 (has links)
The c-Jun NH2-terminal kinases (JNK) are evolutionarily conserved serine/threonine protein kinases that are activated by proinflammatory cytokines, environmental stress, and genotoxic agents. These kinases play key regulatory roles within a cell by coordinating signals from the cell surface to nuclear transcription factors. JNK phosphorylates the amino terminal domain of all three Jun transcription factors (JunB, c-Jun and JunD) all members of the AP-1 family. The activated transcription factors modulate gene expression to generate appropriate biological responses, including cell migration, proliferation, differentiation and cell death.
The role of the JNK signaling pathway in cell death/apoptosis is controversial, both pro-apoptotic and pro-survival roles have been attributed to JNK. The mechanism that enables the JNK signaling pathway to mediate both apoptosis and survival is unclear. The aim of this study is to examine the role of TNF-stimulated JNK activation on cell survival.
The proinflammatory cytokine TNF, is known to activate JNK and induce apoptosis. To test whether the JNK signaling pathway contributes to TNF-induced apoptosis, the response of wild type and Jnk1-/- Jnk2-/- (JNK deficient fibroblasts) fibroblasts to TNF was examined. JNK deficient fibroblasts are more sensitive to TNF-induced apoptosis than wild-type fibroblasts. The TNF-sensitivity cannot be attributed to altered expression of TNF receptors or defects in the NF-кB or AKT pathways, known anti-apoptotic signal transduction pathways. (In fact, TNF stimulated NF-кB activation provides a major mechanism to account for survival in both wild-type and JNK deficient cells.) However this increased TNF-sensitivity can be attributed to JNK deficiency. Apoptosis is suppressed in JNK deficient cells when transduced with JNK1 retrovirus. These data implicate the JNK signaling pathway in cell survival.
The AP-1 family of transcription factors is a target of the JNK signal transduction pathway. In addition JNK is required for the normal expression of the AP-1 family member, JunD. Previous studies have indicated that JunD can mediate survival. Interestingly, JNK deficient and JunD null cells display similar phenotypes: premature senescence and increased sensitivity to TNF induced apoptosis. In fact, the TNF-sensitivity is also suppressed in JNK deficient fibroblasts transduced with JunD retrovirus. Although JunD can replace the survival signaling role of JNK, phosphorylation of JunD is essential to inhibit TNF induced apoptosis. JNK deficient cells transduced with phosphomutant JunD retrovirus maintain TNF-sensitivity.
Activated transcription factors modulate gene expression. It is most likely that JunD functions by regulating the expression of key molecules that act to inhibit TNF-stimulated apoptosis. Microarray analysis comparing wild-type with JNK deficient fibroblasts revealed that the expression of the survival gene, cIAP-2, was induced by TNF in only wild-type fibroblasts. Furthermore, protein expression of cIAP-2 was induced by TNF in only wild-type fibroblasts. Analysis of the cIAP-2 promoter revealed two critical NF-кB binding sites and one AP-1 binding site. Luciferase reporter assays indicated key roles for both NF-кB and the AP-1 component, JunD in TNF-induced cIAP-2 gene expression. These experiments establish that the JNK/JunD pathway collaborates with NF-кB pathway to increase the expression of the anti-apoptotic protein cIAP-2 in TNF treated cells. Without this collaboration, the JNK pathway mediates apoptosis.
The integration of JNK signaling with other signaling pathways represents a mechanism to account for the dual ability of the JNK pathway to mediate either survival or apoptosis. The dynamic coordination of signals within and between pathways is critical. The future challenge will be to fit the details of individual signaling pathways into the context of signaling networks.
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The c-Jun NH₂-Terminal Kinase Regulates Jun <em>in vitro</em> and <em>in vivo</em> during the Process of Dorsal Closure: A DissertationSluss, Hayla Karen 12 December 1997 (has links)
Tyrosine phosphorylation of proteins by protein tyrosine kinases is an important step in initiating mitogenic signal transduction pathways. The receptor tyrosine kinases represent a class of protein kinases that employ phosphorylation cascades to transmit a signal generated at the cell surface. The AP-1 transcription factor is a common target of receptor tyrosine kinase activation, transformation by Ras-like proteins and activation of the MAP kinase pathway. The AP-1 complex contains a dimer of Jun proteins or a heterodimer of Jun and Fos or other bZip proteins. The transcriptional activation of Jun is enhanced by phosphorylation on residues Ser-63 and Ser-73. Therefore, identifying the regulatory proteins kinases of Jun would be an important link in signaling from the upstream cell surface events to downstream events, such as gene expression. The JNK1 protein kinase was identified and phosphorylates c-Jun at these sites. The JNK1 protein is a member of the JNK group of protein kinases, which are activated in response to UV treatment. JNK1 is the 46 kDa isoform, and the isolation of the 55 kDa isoform is described in this thesis. Furthermore, a role for JNK was established in Drosophila. Drosphila JNK (DJNK) is essential for the process of dorsal closure. The JNK protein kinases are involved in cytokine signaling, response to environmental stress and development.
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