Global ETD Search

161	Reação à infecção pelo vírus da tristeza dos citros (CTV) em plantas transgênicas de laranja \'Hamlin\' (Citrus sinensis (L.) Osbeck) expressando seqüências gênicas do CTV / Reaction to Citrus tristeza virus (CTV) infection of transgenic \'Hamlin\' sweet orange (Citrus sinensis (L.) Osbeck) plants transformed with CTV genetic sequences Amancio José de Souza 12 June 2008 (has links) O vírus da tristeza dos citros (CTV) é uma das maiores ameaças à citricultura mundial. No Brasil, mesmo com a pré-imunização e com a substituição de porta-enxertos, estirpes fortes de CTV ainda causam prejuízos consideráveis. Com o aparecimento da Morte Súbita dos Citros em 1999 e a possível relação desta doença com o CTV, este vírus voltou a figurar como patógeno de importância no cenário da citricultura brasileira. Uma das possíveis soluções para o controle de viroses em fruteiras é a obtenção de plantas transgênicas resistentes ou imunes. O objetivo deste trabalho foi avaliar a resistência ao CTV de plantas transgênicas de laranja \'Hamlin\' contendo três construções gênicas oriundas de seqüências do genoma do CTV. Estas construções gênicas visaram ativar rotas de RNAi (hairpin da capa protéica e seqüência conservada antisenso do CTV) e mecanismos de defesa relacionados à expressão da capa protéica do CTV. As plantas transgênicas foram desafiadas com uma estirpe fraca de CTV (CTV-IAC) por meio de borbulhas e pulgões pretos (Toxoptera citricida Kirkaldy) contendo o vírus. A avaliação da resistênica à replicação viral foi feita por análises de ELISA. As plantas transgênicas foram consideradas não resistentes à infecção e translocação viral quando inoculadas com borbulhas. Entretanto algumas plantas mostraram retardamento da infecção. Não foi possível determinar se houve resistência à transmissão de CTV por pulgões já que a técnica utilizada não foi capaz de infectar os controles de maneira uniforme. / The Citrus tristeza virus (CTV) is one of the greatest threats to the citrus industry worldwide. In Brazil, CTV continues to cause damage through strong strains despite the use of techniques like cross-protection and substitution of intolerant rootstocks. With the appearance and spread of the Citrus Sudden Death disease in 1999 and its possible relation to CTV, this virus was again among important pathogens within the Brazilian citrus industry. One of the possible solutions for controlling virus diseases in fruit crops is the development of immune or resistant transgenic plants. The objective of this work was to evaluate the resistance to CTV of transgenic \'Hamlin\' sweet orange plants containing three transgenic constructs obtained from CTV genomic sequences. The genetic constructs used aimed to activate RNAi defense routes (coat protein hairpin and a conserved sequence from CTV) and resistance mechanisms related to the coat protein expression. The transgenic plants were challenged with a weak strain of CTV, CTV-IAC, by bud and aphid (Toxoptera citricida Kirkaldy) inoculation. The evaluation of viral replication was done by ELISA analysis. The transgenic plants were considered susceptible to viral replication and translocation when bud inoculated. However, a few plants showed retardation of infection. It was not possible to determine resistance in the aphid transmission assay since the controls were not uniformly inoculated. Closterovirus Laranja Plantas transgênicas Tristeza cítrica. Citrus. CTV Gene silencing Genetic transformation RNAi
162	O movimento de (des)silenciamento em aula de Língua Portuguesa na rede estadual Amaral, Maria Feliciana da Silva 07 November 2013 (has links) Made available in DSpace on 2016-04-28T18:22:46Z (GMT). No. of bitstreams: 1 Maria Feliciana da Silva Amaral.pdf: 2487228 bytes, checksum: 145d487a1dbf459ffe5cbf76d5e939b9 (MD5) Previous issue date: 2013-11-07 / Secretaria da Educação do Estado de São Paulo / The objective of the research is to critically understand the existing modes of (un)silencing in a public school classroom in São Paulo. This research aims at answering the following question: How does the movement of (un)silencing occurs in a Portuguese language class with a group of students in the second and later the third high school years? In order to answer it, it was necessary to investigate which modes of managing the interaction within the participants facilitated the process of silencing and which enabled the process of unsilencing. This study takes place within the Applied Linguistic context and it is based on Social Cultural Historical Activity Theory, which reiterates the importance of language as a genetic source of human activity and consciousness, as stated by Vygotsky (1934/1999), Leontiev (1977-78) and Engeström (1999). This is a Critical Collaborative Research PCCol (MAGALHÃES, 2006), which aims at understanding, observing, transforming and contributing to the development of students and teachers in such way that all participants involved in this movement interact while searching for alternatives towards a critical, citizenship participation. This project has selected and analyzed the interactions within the participants during three Portuguese language classes recorded in audio and video. The data analysis was organized within an enunciative-discursive-linguistic perspective. The results show that the unsilencing process may be facilitated by more collaborative class managing proposals. Nevertheless, it is essential that the teacher intentionally engages and employs the necessary efforts towards the development of managing modes that involve the group in this direction / O objetivo deste trabalho é compreender de modo crítico as formas de (des)silenciamento existentes na sala de aula em uma escola estadual de São Paulo. A pergunta que direciona esta pesquisa é: como ocorre o movimento de (des)silenciamento em uma aula de LP com um mesmo grupo de ensino médio no 2º ano e, posteriormente, no 3º ano? Para respondê-la, foi preciso investigar que modos de gestão da interação entre os participantes propiciam o silenciamento e que modos propiciam o dessilenciamento. O estudo desenvolve-se no contexto da Linguística Aplicada e se insere na Teoria da Atividade Sócio-Histórico-Cultural, que reitera a importância da linguagem como fonte constituinte da atividade humana e da consciência, conforme Vygotsky (1934/1999), Leontiev (1977-78) e Engeström (1999). Trata-se de uma Pesquisa Crítica de Colaboração PCCol (MAGALHÃES, 2006), cujo foco é conhecer, observar, transformar e contribuir com alunos e professores, de forma que todos os participantes envolvidos nesse movimento se inter-relacionem, em busca de alternativas para um agir crítico e cidadão. Este projeto escolheu como corpus as interações entre os participantes durante três aulas de Língua Portuguesa, recuperadas por meio de gravações em áudio e vídeo. A análise de dados se organizou a partir da perspectiva enunciativo-discursivo-linguística. Os resultados mostram que o dessilenciamento pode ser propiciado a partir de propostas de gestão realizadas em sala de aula. No entanto, é preciso um engajamento intencional e um esforço do professor para o desenvolvimento de modos de gestão que mobilizem o grupo nessa direção Dessilenciamento Silenciamento Argumentação Colaboração Unsilencing Silencing Argumentation Collaboration
163	RNA interference (RNAi) for selective gene silencing in Astigmatid mites Marr, Edward John January 2016 (has links) Psoroptic mange, caused by the Astigmatid mite Psoroptes ovis, is an ectoparasitic disease of significant economic importance to agriculture on a global scale and poses a serious welfare concern. With the current chemotherapeutic controls considered unsustainable, there is pressing need for novel control strategies. RNA interference has been proposed as a potential high throughput approach for the identification of novel therapeutic targets with high specificity, speed and at a relatively low cost compared to the existing methods. The presence of the components of the RNA interference (RNAi) pathway in P. ovis was first confirmed through in silico analyses of the P. ovis transcriptome and, following development of a non-invasive immersion method of double stranded RNA (dsRNA) delivery, gene silencing by RNAi was demonstrated in P. ovis. Statistically-significant reduction of transcript level was measured for the three genes targeted: P. ovis mite group 2 allergen (Pso o 2), P. ovis mu class glutathione S-transferase (PoGST-mu1) and P. ovis beta tubulin (Poβtub). This is the first demonstration of gene silencing by RNAi in P. ovis and provides a key mechanism for mining transcriptomic and genomic datasets in the future for novel targets of intervention against P. ovis. The first assessment of gene silencing was also performed in two related Astigmatid mites of high medical importance; the European house dust mite Dermatophagoides pteronyssinus and the scabies mite Sarcoptes scabiei. A statistically-significant reduction in expression of a D. pteronyssinus mu class glutathione S-transferase (DpGST-mu1) transcript was observed. No significant reduction in expression of a S. scabiei mu class glutathione S-transferase (SsGST-mu1) transcript was observed. Additionally, microRNAs (miRNAs) from the related miRNA pathway were identified in a P. ovis small RNA sample and were sequenced and annotated.
164	Molecular characterization of the F-box protein FBW2 in the RNA silencing in Arabidopsis thaliana / Caractérisation moléculaire de la protéine F-box FBW2 dans l’ARN interférence chez Arabidopsis thaliana Hacquard, Thibaut 21 September 2018 (has links) L'ARN interférence est un mécanisme moléculaire conservé chez les Eucaryotes dont les principaux acteurs sont les protéines ARGONAUTE (AGO). Chez les plantes, AGO1 est une protéine essentielle à la croissance et la défense antivirale. Elle utilise des petits ARNs comme sondes pour reconnaître et réguler des ARN messagers. Les virus ont développé des suppresseurs de l'ARN interférence pour surmonter cette défense. L'un d'entre eux, P0 du virus de la mosaïque jaune du navet, est comme une protéine F-box qui détourne le complexe SCF, une ubiquitine ligase E3, et conduit AGO1 vers la protéolyse ubiquitine-dépendante. Cette dégradation utilise la vacuole au lieu du protéasome 26S, généralement associé à la dégradation ubiquitine-dépendante. Ce mécanisme de protéolyse n'est pas compris et est aussi apparent quand AGO1 est déstabilisé de manière endogène, suggérant que P0 utilise une voie déjà existante. Une protéine F-box d'Arabidopsis, FBW2, a été décrite comme impactant l'homéostasie d'AGO1 indépendamment du protéasome. Mon projet de thèse visait à caractériser l'activité F-box de FBW2 et à comprendre la relation entre AGO1 et FBW2 ainsi que ses conséquences sur l'ARN interférence. Les résultats obtenus dans ce manuscrit montrent que le complexe SCFFBW2 interagit avec AGO1 et déclenche sa dégradation via un processus indépendant de l'autophagie ou du protéasome, tout en n'affectant que faiblement l'ARN interférence. FBW2 ciblerait en fait un sous-ensemble de protéines AGO1 qui semble ne pas contenir de petits ARNs. Cette régulation jouerait un rôle de surveillance pour prévenir une activité délétère d'AGO1 en absence de petits ARNs. / RNA silencing is a conserved molecular mechanism in eukaryotes, of which the main effectors are the ARGONAUTE (AGO) proteins. In plants, AGO1 is a protein that is essential for growth and antiviral defence. It uses small RNAs as probe to recognize and regulate messenger RNAs. Viruses have developed suppressors of RNA silencing to overcome this defence. One of these, P0 from the Turnip Yellows Virus, acts as an F-box protein to hijack the SCF complex, an E3 ubiquitin ligase, and guide AGO1 to the ubiquitin-dependent proteolysis. This degradation uses the vacuole instead of the 26S proteasome, generally associated with ubiquitin-dependant proteolysis. This proteolysis mechanism is not understood and is also apparent when AGO1 is endogenously destabilized, suggesting that P0 uses an already existing pathway. An Arabidopsis F-box protein, FBW2, has been shown to impact AGO1 homeostasis independently from the proteasome. My PhD project aimed at characterizing FBW2 F-box activity and understanding the relationship between AGO1 and FBW2, as well as its consequences on the RNA silencing. The results obtained in this manuscript show that the SCFFBW2 interacts with AGO1 and triggers its degradation through an autophagy- and proteasome- independent process, while only weakly affecting the RNA silencing. FBW2 would actually target a subset of AGO1 proteins, which appears not to contain small RNAs. This regulation would play a surveillance role in order to prevent a deleterious activity of AGO1 in absence of small RNAs. Arabidopsis AGO1 Ubiquitine SCF FBW2 ARN interférence Arabidopsis RNA silencing AGO1 Ubiquitin SCF FBW2 572.8 581
165	The Experience of Loss of Voice in Adolescent Girls: An Existential-Phenomenological Study Cihonski, Deborah A 22 May 2003 (has links) The purpose of this study was to examine the meaning of the Loss of Voice experience in adolescent girls using an existential-phenomenological interview approach. An open-ended interview was conducted and participants were asked to "Please think of a specific time when you had something important to say, but did not say it. In as much detail as possible, describe that experience." Each interview was tape-recorded, transcribed by the investigator, and then independently thematized (Jones, 1984) by the author and a doctoral colleague trained in Jones' (1984) analysis method. Interrater reliability of the themes reached 96% agreement for the overall sample. Individual transcription reliabilities ranged between 85-98%. Thematic analysis revealed six superordinate themes and four subthemes. The superordinate themes were Difficult Position, Feeling, Might Explode, Not Worth It, Who Am I?, and Nevermind. The subthemes So Much To Lose and Strong were part of superordinate theme Difficult Position. The subthemes Emotion and Physical were part of the superordinate theme Feeling. Analysis of these themes in their totality suggested a complex meaning structure of co-researchers Loss of Voice experiences. This research supports and expands the current literature on Loss of Voice by providing a more in-depth study of the meaning contained in a Loss of Voice experience. Directions for future research efforts, intervention, and prevention education are discussed. phenomenology authentic voice silencing silenced depression school American Studies Arts and Humanities
166	Identification et étude d'un nouveau mécanisme nucléaire de régulation post-transcriptionnelle par les micro-ARN / Nucleoplasmic post transcriptional gene silencing mediated by microRNAs is controlled by Sfpq Tekaya Hamouda, Nedra 31 March 2016 (has links) Les miARN sont de petits ARN non codant dont la taille varie entre 21-24 nucléotides. Ils jouent un rôle de régulateurs post-transcriptionnels en utilisant leur complémentarité de séquence avec l’ARN messager (ARNm) cible afin d’induire sa répression. Grâce à la protéine Argonaute 2 (Ago2) dans laquelle les miARN sont incorporés formant ainsi le complexe miRISC, des cofacteurs sont recrutés afin d’induire la dégradation ou le blocage de la traduction de l’ARNm cible. Initialement connus pour réguler leurs cibles dans le cytoplasme, les miARN sont de plus en plus décrits comme étant des régulateurs de l’expression génique au niveau nucléaire. Dans ce travail, nous avons démontré la présence, au sein du noyau, d’un nouveau mécanisme de régulation post-transcriptionel par les miARN dont les facteurs majeurs sont Sfpq et Pspc1 / Micro-RNA, nuclear regulation, gene silencing, SfpqThere is a growing body of evidence about the presence and the activity of the miRISC in the nucleus of mammalian cells. Here we show by quantitative proteomic analysis that Ago2 interacts with the complex formed by Sfpq, Pspc1 and NonO in a RNA-dependent fashion. Sfpq mediates the interaction between miRISC with Pspc1 and NonO in the nucleoplasm. By HITS-CLIP coupled with transcriptomic analysis, we demonstrated that Sfpq specifically controls the downregulation of a subset of crucial let-7a-target mRNAs in stem cells, including Lin28a, Prtg, and Igf2bp1. Sfpq directly binds to specific sequence in the 3'UTR to promote the recruitment of selected nucleoplasmic miRNAs and triggers the decay, as we show for Lin28a mRNA. These results extend the miRNA-mediated post-transcriptional gene silencing into the nucleus and indicate that a dual strategy Micro-ARN Régulation nucléaire Cellules souches Micro-RNA Nuclear regulation Gene silencing Sfpq
167	New mechanisms modulating S100A8 gene expression Endoh, Yasumi, Medical Sciences, Faculty of Medicine, UNSW January 2008 (has links) S100A8 is a highly-expressed calcium-binding protein in neutrophils and activated macrophages, and has proposed roles in myeloid cell differentiation and host defense. Functions of S100A8 are not fully understood, partly because of difficulties in generating S100A8 knockout mice. Attempts to silence S100A8 gene expression in activated macrophages and fibroblasts using RNA interference (RNAi) technology were unsuccessful. Despite establishing validated small interfering RNA (siRNA) systems, enzymaticallysynthesized siRNA targeted to S100A8 suppressed mRNA levels by only 40% in fibroblasts activated with FGF-2+heparin, whereas chemically-synthesized siRNAs suppressed S100A8 driven by an S100A8-expression vector by ~75% in fibroblasts. Suppression of the gene in activated macrophages/fibroblasts was low, and some enzymatically-synthesized siRNAs to S100A8, and unrelated siRNA to GAPDH, induced/enhanced S100A8 expression in macrophages. This indicated that S100A8 may be upregulated by type-1 interferon (IFN). IFN-β enhanced expression, but did not directly induce S100A8. Poly (I:C), a synthetic dsRNA, directly induced S100A8 through IL-10 and IFN-dependent pathways. Induction by dsRNA was dependent on RNA-dependent protein kinase (PKR), but not cyclooxygenase-2, suggesting divergent pathways in LPS- and dsRNA-induced responses. New mechanisms of S100A8 gene regulation are presented, that suggest functions in anti-viral defense. S100A8 expression was confirmed in lungs from influenza virus-infected mice and from a patient with severe acute respiratory syndrome (SARS). Multiple pathways via mitochondria mediated S100A8 induction in LPS-activated macrophages; Generation of reactive oxygen species via the mitochondrial electron transport chain and de novo synthesis of ATP may be involved. This pathway also regulated IL-10 production, possibly via PKR. Extracellular ATP and its metabolites enhanced S100A8 induction. Results support involvement of cell stress, such as transfection, in S100A8 expression. A breast tumor cell line (MCF-7) in which the S100A8 gene was silenced, was established using micro RNA technology; S100A8 induction by oncostatin M was reduced by >90% in stably-transfected cells. This did not alter MCF-7 growth. The new approach to investigate the role of S100A8 in a human tumor cell line may assist in exploring its functions and lead to new studies concerning its role in cancer. S100A8 Gene silencing Macrophage activation Interleukin 10 TLR- 3 Mitochondrial reactive oxygen species
168	Characterization of AtSUVR3 functions in Arabidopsis thaliana using RNA interference Wang, Tao 15 May 2009 (has links) Variability of transgene expression levels resulting from gene silencing is considered as ahindrance to the successful application of plant genetic engineering. Towards alleviatinggene silencing, I decided to screen for novel genes involved in transgene silencing and toinvestigate how these genes regulate plant development. Genes encoding putative chromatinremodeling factors, especially those including a SET domain, were selected as candidatetargets. A bioinformatic analysis of the Arabidopsis SET genes (AtSET) was performed andthese genes were classified into 6 groups based on the domain architecture. RNA interference (RNAi) vectors were constructed for ~ 20 AtSET genes and wereintroduced into both wild type lines and transgenic lines silenced for a GFP reporter gene.Surprisingly, altered developmental phenotypes were only observed for three constructs,raising questions as to the effectiveness of the RNAi approach for the chosen Arabidopsissystem. To assess this situation, I targeted a phytoene desaturase (PDS) gene using the sameRNAi approach. Inactivation of PDS renders plant a readily identifiable phenotype. Whereasthe RNAi penetrance in Arabidopsis can be very high, the expressivity of RNAi in varioustissues and among different plants can vary dramatically. Contradictory to previous reports,I found that there is correlation between transcript level and silencing phenotype. Possiblereasons for this discrepancy are discussed. No apparent correlation between transgene copynumber and RNAi phenotypes was observed. Among the three RNAi constructs that caused an abnormal development inArabidopsis, K-23 which targets SuvR3 has the highest expressivity and could reactivate asilenced GFP locus. SuvR3 RNAi lines were selfed for six generations and were screenedfor morphological phenotypes. Abnormal number of flower organs, loss of viability of malegametophytes, and decreased seedling germination percentage were found in SuvR3 RNAilines. A progressive increase in both severity and frequency of abnormal phenotypes wereseen in subsequent generations, suggesting an epigenetic regulatory mechanism involvedwith SuvR3. Alternative splicing of SuvR3 was also observed in most of Arabidopsis tissues.One of the protein isoforms, SuvR3, lacks 16 amino acids within the highly conserved SETdomain. Possible effects of isoform interaction are proposed. RNA interference RNAi penetrance RNAi expressivity gene silencing SET domain alternative splicing
169	Molecular Insights into Kcnq1ot1 Noncoding Antisense RNA Mediated Long Range Transcriptional Gene Silencing Pandey, Radha Raman January 2008 (has links) Non-coding antisense RNAs have been implicated in the epigenetic silencing of individual gene as well as chromosomal domains. While silencing of the overlapping gene by antisense RNAs has been well investigated, their functional role in silencing of chromosomal domains remains enigmatic. To elucidate mechanisms underlying the non-coding RNA mediated epigenetic silencing of chromosomal domains, we have chosen an antisense non-coding RNA, Kcnq1ot1, as a model system. Previously, a functional role of Kcnq1ot1 RNA and/or its transcriptional process has been implicated in silencing of multiple genes in the Kcnq1 imprinted cluster. However, these studies could not rule out the mechanisms involving other than Kcnq1ot1 RNA. Furthermore, it was also unclear how the Kcnq1ot1 promoter escapes silencing when its encoded RNA is capable of silencing flanking genes in cis. We have shown that NF-Y transcription factor plays a central role in the Kcnq1ot1 promoter activity, and that mutation of the NF-Y binding sites not only resulted in loss of silencing of flanking genes but also the ability of the Kcnq1ot1 promoter to protect against repressive chromatin marks, indicating that NF-Y maintains transcription-competent chromatin at the promoter through resisting the strong silencing effects of Kcnq1ot1 RNA. The Kcnq1ot1 RNA is an RNA Polymerase II encoded 91 kb long moderately stable nuclear transcript. We have demonstrated that it is the RNA not the act of transcription responsible for silencing and that the degree of silencing was proportional to the length of Kcnq1ot1 RNA. The kinetics of heterochromatin formation in relation to Kcnq1ot1 transcription revealed that overlapping gene was silenced initially by occlusion of basal transcription machinery and heterochromatin formation, whereas nonoverlapping gene was silenced subsequently by Kcnq1ot1-mediated heterochromatin spreading. This transcriptional silencing by Kcnq1ot1 RNA is mediated by an 890 bp region through promoting its interaction with the chromatin. Interestingly, we show that Kcnq1ot1 RNA establishes heterochromatin structures in a lineage-specific fashion by interacting with chromatin and chromatin remodelling complexes such as G9a and PRC2 complexes. More importantly, one of the parental chromosomes comprising Kcnq1 domain always found in the vicinity of perinucleolar region. Based on these data we proposed a mechanism whereby Kcnq1ot1 RNA establishes transcriptional silencing through recruitment of chromatin remodelling machinery and the maintenance of silencing achieved via targeting to the perinucleolar region. epigenetics gene silencing noncoding RNA genomic imprinting Kcnq1ot1 Medical genetics Medicinsk genetik
170	Mating type switching and transcriptional silencing in Kluyveromyces lactis Barsoum, Emad January 2010 (has links) To explore the similarities and differences of regulatory circuits among budding yeasts, we characterized the role of unscheduled meiotic gene expression 6 (UME6) and a novel mating type switching pathway in Kluyveromyces lactis. We found that Ume6 was required for transcriptional silencing of the cryptic mating-type loci HMLα and HMRa. Ume6 acted directly at these loci by binding to the cis-regulatory silencers. Ume6 also served as a block to polyploidy and was required for repression of three meiotic genes, independently of the Rpd3 and Sin3 corepressors. Mating type switching from MATα to MATa required the α3 protein. The α3 protein was similar to transposases of the mutator like elements (MULEs). Mutational analysis showed that the DDE-motif in α3, which is conserved in MULEs was necessary for switching. During switching α3 mobilizes from the genome in the form of a DNA circle. The sequences encompassing the α3 gene circle junctions in the MATα locus were essential for switching from MATα to MATa. Switching also required a DNA binding protein, Mating type switch 1 (Mts1), whose binding sites in MATα were important. Expression of Mts1 was repressed in MATa/MATα diploids and by nutrients, limiting switching to haploids in low nutrient conditions. In a genetic selection for strains with increased switching rates we found a mutation in the RAS1 gene. By measuring the levels of the MTS1 mRNA and switching rates in ras1, pde2 and msn2 mutant strains we show that mating type switching in K. lactis was regulated by the RAS/cAMP pathway and the transcription factor Msn2. ras1 mutants contained 20-fold higher levels of MTS1 mRNA compared to wild type whereas pde2 and msn2 expressed less MTS1 mRNA and had decreased switching rates. Furthermore we found that MTS1 contained several potential Msn2 binding sites upstream of its ORF. We suggest that these observations explain the nutrient regulation of switching. / At the time of the doctoral defense, the following papers were unpublished and had a status as follows: Paper 3: Manuscript. Mating type switch transcriptional silencing alpha3 transposase Ume6 Mts1 Ras cAMP K. lactis Developmental biology Utvecklingsbiologi

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