Tesis sobre el tema "Promoter analysi"
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Kokulapalan, Wimalanathan. "Genome-wide Computational Analysis of Chlamydomonas reinhardtii Promoters". Miami University / OhioLINK, 2011. http://rave.ohiolink.edu/etdc/view?acc_num=miami1320638327.
Texto completoQi, Zhan [Verfasser] y Veit [Akademischer Betreuer] Hornung. "Large-scale analysis of Drosophila core promoter function using synthetic promoters / Zhan Qi ; Betreuer: Veit Hornung". München : Universitätsbibliothek der Ludwig-Maximilians-Universität, 2019. http://d-nb.info/1188200240/34.
Texto completoPhillips, Julian Peter. "Promoter analysis in transgenic sugar beet". Thesis, De Montfort University, 1995. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.391084.
Texto completoOliveira, Junior Silvio De. "Revalorisation des effluents thermiques industriels : analyse exergétique, entropique et économique". Vandoeuvre-les-Nancy, INPL, 1991. http://docnum.univ-lorraine.fr/public/INPL_T_1991_OLIVEIRA_JUNIOR_S_D.pdf.
Texto completoBohne, Alexandra-Viola. "Analyse von Komponenten der organellären Transkriptionsmaschinerien aus Arabidopsis thaliana und Nicotiana tabacum". Doctoral thesis, Humboldt-Universität zu Berlin, Mathematisch-Naturwissenschaftliche Fakultät I, 2009. http://dx.doi.org/10.18452/15965.
Texto completoAll mitochondrial and a subset of plastidial genes of photosynthetically active eukaryotes are transcribed by nuclear-encoded, phage-type RNA polymerases. In this study, a homologous in vitro transcription system was used to define the specific functions of Arabidopsis phage-type RNA polymerases RpoTm, RpoTp and RpoTmp in organellar transcription. RpoTmp displayed no significant promoter specificity, whereas RpoTm and RpoTp were able to accurately initiate transcription from overlapping subsets of mitochondrial and plastidial promoters of diverse architecture. RpoTm and RpoTp thereby demonstrated an intrinsic capability to recognize promoters on supercoiled DNA templates without the aid of protein cofactors. A selective promoter recognition by the phage-type RNAPs in vitro and the inability to recognize promoters on linear templates imply that auxiliary factors are required for efficient initiation of transcription and/or DNA melting in vivo. Crosswise recognition of organellar promoters by the phage-type RNA polymerases in vitro as well as other similarities of the mitochondrial and plastidial transcription machineries such as promoter structures and the phylogenetic origin inspired in planta studies to investigate specific transcription of a mitochondrial promoter in plastids. Therefore, the expression of an nptII reporter gene under control of the mitochondrial PatpA promoter from Oenothera was analyzed in transplastomic tobacco plants. The data presented here demonstrate the faithful recognition of the mitochondrial PatpA promoter by a plastid RNA polymerase both in in vitro transcription assays and in transplastomic tobacco plants. These findings disclose further unexpected similarities of the organellar gene expression systems which deliver interesting evolutionary insights and might facilitate improved applications for chloroplast genome engineering.
Featherstone, Mark S. "Structural analysis of the polyomavirus late promoter". Thesis, McGill University, 1986. http://digitool.Library.McGill.CA:80/R/?func=dbin-jump-full&object_id=72778.
Texto completoHe, Bing. "Systematic analysis of enhancer and promoter interactions". Diss., University of Iowa, 2015. https://ir.uiowa.edu/etd/1972.
Texto completoCollins, Malcolm Robert. "Characterisation of the human α2(I) procollagen promoter-binding proteins". Doctoral thesis, University of Cape Town, 1993. http://hdl.handle.net/11427/27139.
Texto completoDanevad, Margrete. "Functional analysis of the murine LI-Cadherin promoter". [S.l.] : [s.n.], 2004. http://www.diss.fu-berlin.de/2004/165/index.html.
Texto completoChaidir, Nadia. "Whole-genome comparative promoter sequence analysis in plants". Thesis, McGill University, 2014. http://digitool.Library.McGill.CA:80/R/?func=dbin-jump-full&object_id=123303.
Texto completoL'étude d'association pangénomique est maintenant rendue possible par le nombre de séquences génétiques de hautes qualités qui sont disponibles pour plusieurs espèces végétales. Pour comprendre les mécanismes de régulation de la transcription, un nombre d'outils d'analyses informatiques ont été développé pour identifier les éléments cis-régulatoires. Les bases de données utilisées comme saisie positive pour l'identification informatique des régions de régulation incluent communément les promoteurs des gènes co-régulés ainsi que des gènes orthologues (Wang et Stormo, 2003).Pour découvrir les motifs de novo, nous avons utilisé deux techniques; 1) une découverte basée sur la relation orthologue des gènes de 18 espèces végétales et, 2) une découverte basée sur les gènes co-régulés dans certains tissus végétales spécifiques provenant de données de séquençage d'ARN de soja. Dans la première approche nous avons utilisé une combinaison de plusieurs outils bioinformatiques pour prédire les motifs des promoteurs basés sur des groupes de gènes orthologues trouvés dans les bases de données des génomes entiers d'Arabidopsis lyrata, Arabidopsis thaliana, Brachypodium distachyon, Carica papaya, Chlamydomonas reinhardtii, Glycine max, Linus usitissimum, Malus domestica, Manihot esculenta, Medicago truncutula, Oryza sativa, Physcomitrella patens, Populus trichocarpa, Selaginella moellendorfii, Sorghum bicolor, Vitis vinivera, Volvox carteri et Zea mays. Les résultats ont démontré que, dans les plantes, plusieurs promoteurs de gènes orthologues contiennent des motifs cis-régulatoires similaires. En plus, en incluant des espèces évolutivement éloignées dans les analyses, nous avons été capable de démontrer que ces motifs sont conservés. Dans la deuxième partie, nous avons fait une analyse comparant les séquences des promoteurs co-régulés dans les méristèmes apicaux ainsi que dans l'épiderme de trois cultivars de soja; Clark sauvage, mutant a 5-feuilles et mutant glabre. Les résultats ont démontré que les promoteurs des gènes co-régulés en différents tissus contiennent des motifs cis-régulatoires similaires. Générer des données à l'échelle génomique demande une puissance informatique énorme qui n'est pas toujours disponible. En conséquence, nous avons créé une base de données pour 18 génomes de plantes composée de séquences de promoteurs, de motifs, d'annotations et des groupes de gènes orthologues ainsi que d'autres informations associées avec ceux-ci.
Burbridge, Stephen Anthony. "Analysis of the Xenopus N-cadherin promoter region". Thesis, University of Warwick, 1995. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.362548.
Texto completoMarden, Chloe Maria. "Functional analysis of the P47 PHOX gene promoter". Thesis, University College London (University of London), 1999. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.392359.
Texto completoLi, Xiaomeng. "Human Promoter Recognition Based on Principal Component Analysis". Thesis, The University of Sydney, 2008. http://hdl.handle.net/2123/3656.
Texto completoLi, Xiaomeng. "Human Promoter Recognition Based on Principal Component Analysis". University of Sydney, 2008. http://hdl.handle.net/2123/3656.
Texto completoThis thesis presents an innovative human promoter recognition model HPR-PCA. Principal component analysis (PCA) is applied on context feature selection DNA sequences and the prediction network is built with the artificial neural network (ANN). A thorough literature review of all the relevant topics in the promoter prediction field is also provided. As the main technique of HPR-PCA, the application of PCA on feature selection is firstly developed. In order to find informative and discriminative features for effective classification, PCA is applied on the different n-mer promoter and exon combined frequency matrices, and principal components (PCs) of each matrix are generated to construct the new feature space. ANN built classifiers are used to test the discriminability of each feature space. Finally, the 3 and 5-mer feature matrix is selected as the context feature in this model. Two proposed schemes of HPR-PCA model are discussed and the implementations of sub-modules in each scheme are introduced. The context features selected by PCA are III used to build three promoter and non-promoter classifiers. CpG-island modules are embedded into models in different ways. In the comparison, Scheme I obtains better prediction results on two test sets so it is adopted as the model for HPR-PCA for further evaluation. Three existing promoter prediction systems are used to compare to HPR-PCA on three test sets including the chromosome 22 sequence. The performance of HPR-PCA is outstanding compared to the other four systems.
Khan, H. "Mutational analysis of the Klebsiella pneumoniae nifLA promoter". Thesis, University of Sussex, 1985. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.372054.
Texto completoChilds, Kevin. "Combinatorial motif analysis in yeast gene promoters: the benefits of a biological consideration of motifs". Thesis, Texas A&M University, 2004. http://hdl.handle.net/1969.1/1351.
Texto completoLorson, Christian. "An analysis of transcriptional regulation of the MVM capsid gene promoter". free to MU campus, to others for purchase, 1997. http://wwwlib.umi.com/cr/mo/fullcit?p9841319.
Texto completoSoanes, Darren Mark. "Regulation of the pathogenicity gene MPG1 in the rice blast fungus Magnaporthe grisea". Thesis, University of Exeter, 2001. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.368367.
Texto completoKirk, Jane A. E. "Region specific expression of a Dictyostelium discoideum prestalk marker". Thesis, Open University, 1995. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.262113.
Texto completoEristi, Can M. "Investigation of Transcriptional Regulation of 5'-Nucleotidase in Dictyostelium Discoideum". Diss., Virginia Tech, 2003. http://hdl.handle.net/10919/28822.
Texto completoPh. D.
Brown, Anthony Peter Colin. "A biomolecular analysis of the control of expression and function of a low temperature responsive barley gene". Thesis, University of Newcastle Upon Tyne, 1998. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.245079.
Texto completoMalik, Yousaf Amir. "Functional analysis of the human immunodeficiency virus type-1 long terminal repeat". Thesis, University of Reading, 2000. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.343172.
Texto completoedu, Kim Rice@mssm y Kim Lee Rice. "Functional Analysis of the HOX11 Target Genes ALDH1A1 and FHL1". Murdoch University, 2004. http://wwwlib.murdoch.edu.au/adt/browse/view/adt-MU20051012.93820.
Texto completoSawaya, Rana. "Promoter analysis of the porA gene of Neisseria meningitidis". Thesis, National Library of Canada = Bibliothèque nationale du Canada, 1998. http://www.collectionscanada.ca/obj/s4/f2/dsk1/tape10/PQDD_0025/MQ50871.pdf.
Texto completoRogers, David Howard. "Analysis of the rat Tal a-tubulin gene promoter". Thesis, McGill University, 2000. http://digitool.Library.McGill.CA:80/R/?func=dbin-jump-full&object_id=36831.
Texto completoThis thesis describes experiments that were designed to explore cell intrinsic mechanisms regulating the generation of neurons from neural precursor cells. Specifically, the regulatory region of the rat Talpha1 alpha-tubulin gene, which encodes an isoform of alpha-tubulin expressed in neurons throughout the nervous system immediately following cell cycle exit, was analyzed to identify DNA sequences directing early neuronal gene expression.
A novel 10-nucleotide regulatory sequence, named the neuronal restriction element (NRE), has been identified. In the context of the Talpha1 gene, the NRE inhibits precocious expression in neural precursor cells. Interestingly, the NRE is conserved in the alpha-1 alpha-tubulin gene and is found in a number of neural genes expressed widely and early in development. As such, the NRE may affect the onset time of a battery of neuronal genes and modulate the timing of neuronal differentiation. In vitro , the NRE binds Su(H), a highly conserved transcription factor involved in the repression of neuronal differentiation.
A second novel regulatory element has been identified, the forebrain response element (FRE), which acts to enhance gene expression specifically in the neocortex. The FRE overlaps the NRE and also contains a conserved 30-nucleotide sequence constituting a putative homeodomain recognition sequence. We speculate that the FRE consists of two subelements that act synergistically to promote gene expression in newborn and mature neocortical neurons.
Kim, S. "Structural analysis of the TRPI promoter in Saccharomyces cerevisiae". Thesis, University of Oxford, 1986. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.306685.
Texto completoAhmed, Nadeem M. "Transgenic analysis of the endodermin promoter in Xenopus laevis". Thesis, University of Warwick, 2002. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.269083.
Texto completoHellen, Elizabeth H. B. "Identification of co-regulated candidate genes by promoter analysis". Thesis, University of Brighton, 2010. https://research.brighton.ac.uk/en/studentTheses/68e2d36a-1d90-4e21-b407-2e67df1e351c.
Texto completoGosemärker, Anna Teresa. "Charakterisierung der humanen und murinen I-kappa-B-Kinase-beta--Promotoren zur Analyse der gewebsspezifischen Variationen in der Zusammensetzng des I-kappa-B-Kinase-Komplexes". [S.l. : s.n.], 2008. http://nbn-resolving.de/urn:nbn:de:bsz:289-vts-64393.
Texto completoGuillocheau, Gabriel. "Etude des polymorphismes altérant la régulation de l'expression des gènes chez le bovin". Thesis, Université Paris-Saclay (ComUE), 2018. http://www.theses.fr/2018SACLA045.
Texto completoAn increasing number of genes and genomic loci have been associated with diseases or phenotypes of interest, by either linkage or association studies. Identifying causative genetic variants is crucial. The regulators with the strongest effect tend to be cis-acting regulatory polymorphisms, close to genes for which altered mRNA expression was detected. The overall objective of this PhD project is to develop a large-scale approach to identify regulatory polymorphisms that potentially alter the regulation of gene expression and impact phenotypes of interest, in cattle.We have developed an approach to ascertain causative SNPs (Single Nucleotide Polymorphisms) of gene expression regulation. To this end, we analysed genome and muscle transcriptome from 19 Limousine bull calves and genome and transcriptome of eight tissues (including ovary and uterus) transcriptome from 6 Holstein cows. For the Limousine breed, we identified 5,658 SNPs showing an allele-specific expression (ASE-SNPs) in 13% of genes with detectable expression in muscle; we linked some of them to SNPs in a regulatory region. Interestingly, we found genes involved in meat quality traits (AOX1, PALLD and CAST) with an allelic imbalance. For the Holstein breed, we identified 33, 527 ASE-SNPs across 8 tissues including 3,369 ASE-SNPs from muscle data, 5,771 from ovary data and 5,499 from uterus data. By analysing these two data records, we discovered genes impacted by ASE. This study is the first done for the Limousine breed and the second for thr Holstein breed.The results of these studies provide a best understanding of gene expression regulation in cattle, in particular by identifying candidate causal polymorphisms and by proposing new methods to detect them
Kühn, Kristina. "Analysis of components of the mitochondrial transcription machinery in Arabidopsis thaliana". Doctoral thesis, Humboldt-Universität zu Berlin, Mathematisch-Naturwissenschaftliche Fakultät I, 2006. http://dx.doi.org/10.18452/15453.
Texto completoMitochondria depend on a nucleus-encoded transcription machinery to express their genome. The present study examined the transcription of mitochondrial genes by two nucleus-encoded phage-type RNA polymerases, RpoTm and RpoTmp, in the plant Arabidopsis. For selected mitochondrial genes in Arabidopsis, transcription initiation sites were determined. Most genes were found to possess multiple promoters. The identified promoters displayed diverse sequence elements and mostly deviated from a nonanucleotide consensus derived previously for dicot mitochondrial promoters. Several promoters were detected that activate transcription of presumably non-functional sequences. Promoter architecture, distribution and utilization suggest a non-stringent control of transcription initiation in Arabidopsis mitochondria. An in vitro transcription system was set up to elucidate the roles of RpoTm and RpoTmp. Since RpoT enzymes possibly require auxiliary factors, the Arabidopsis genome was screened for potential cofactors of phage-type RNA polymerases. A mitochondrial protein (MetA) with similarity to mtTFB, an essential transcription factor in yeast mitochondria, was identified. In in vitro transcription studies, RpoTm recognized various promoters whereas RpoTmp displayed no significant promoter specificity. Promoter recognition by RpoTm depended on supercoiled DNA templates. Transcription initiation by RpoTm or RpoTmp was not affected by MetA, indicating that MetA is not functionally equivalent to mtTFB. Besides, MetA was found to be more closely related to non-mitochondrial rRNA dimethylases than to mtTFB. The present study establishes RpoTm to transcribe mitochondrial genes; RpoTmp may have a non-overlapping transcriptional role in mitochondria. The cofactor-independent promoter specificity of RpoTm and the apparently non-stringent control of transcription initiation in vivo imply that mitochondrial genes in Arabidopsis may not be regulated individually at the transcriptional level.
Wiles, Natasha Shawn. "Identification of Regulatory Binding Sites and Corresponding Transcription Factors Involved in the Developmental Control of 5'-nucleotidase Expression in Dictyostelium discoideum". Diss., Virginia Tech, 2005. http://hdl.handle.net/10919/27810.
Texto completoPh. D.
Joyce, Bradley Ryan. "The Regulation of Alkaline Phosphatase during the Development of Dictyostelium". Diss., Virginia Tech, 2006. http://hdl.handle.net/10919/27646.
Texto completoPh. D.
Vickers, Claudia Estelle. "Functional analysis of the endosperm - specific AsGlo1 promoter in barley /". St. Lucia, Qld, 2003. http://www.library.uq.edu.au/pdfserve.php?image=thesisabs/absthe17515.pdf.
Texto completoWang, Fang. "DNA methylation and promoter sequence analysis of colon cancer genes". Connect to this title online, 2008. http://etd.lib.clemson.edu/documents/1211398606/.
Texto completoTitle from first page of PDF file. Document formatted into pages; contains ix, 68 p. ; also includes graphics (some col.). Contains additional supplemental files.
Klan, Niko [Verfasser]. "Functional analysis of the human 5-LO promoter / Niko Klan". Aachen : Shaker, 2003. http://d-nb.info/1179024540/34.
Texto completoMcDonald, Bernadette Catherine. "Characterisation and analysis of the prostate-specific membrane antigen promoter". Thesis, University of York, 2000. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.369325.
Texto completoGardella, Thomas James. "A Genetic Analysis of RNA Polymerase-Promoter Interactions: A Thesis". eScholarship@UMMS, 1988. http://escholarship.umassmed.edu/gsbs_diss/200.
Texto completoJain, Nishant Rajkumar. "Characterization and functional analysis of the P2Y₂R gene promoter". Diss., Columbia, Mo. : University of Missouri-Columbia, 2006. http://hdl.handle.net/10355/4629.
Texto completoThe entire dissertation/thesis text is included in the research.pdf file; the official abstract appears in the short.pdf file (which also appears in the research.pdf); a non-technical general description, or public abstract, appears in the public.pdf file. Title from title screen of research.pdf file (viewed on April 21, 2009) Includes bibliographical references.
Karanam, Suresh Kumar. "Automation of comparative genomic promoter analysis of DNA microarray datasets". Thesis, Available online, Georgia Institute of Technology, 2004:, 2003. http://etd.gatech.edu/theses/available/etd-04062004-164658/unrestricted/karanam%5Fsuresh%5Fk%5F200312%5Fms.pdf.
Texto completoCrespo, Marion. "Analyse multi-omique des acylations de lysines d'histones pendant la gamétogénèse". Thesis, Université Grenoble Alpes (ComUE), 2019. http://www.theses.fr/2019GREAV066.
Texto completoThe innovative aspect of this project lies in the study of acylations at lysine 27 from histone H3 (H3K27), conventionally studied in a methylated or an acetylated form. We performed this work on meiotic and post-meiotic mouse germ cells. Spermiogenesis, which involves a specific expression program as well as a fine regulation of transcription, is a process that is particularly well suited to understanding the roles of new histone modifications. This work combines the use of four different omics approaches, namely proteomics, metabolomics, transcriptomics and ChIP- sequencing to decipher the regulation of acylations on H3K27.In the first part of this project, we explored the dynamics of acetylation and crotonylation on histone lysines during the processes of yeast sporulation and mouse spermatogenesis, which allowed us to highlight in particular crotonylated H3K27. Its accumulation on the histone variant H3.3 and its important stoichiometry compared to the acetylated form H3K27ac in mouse post-meiotic germ cells led us to study the genomic distribution of this mark by ChIP-seq analysis. The comparative analysis of H3K27ac and H3K27cr revealed a synergy between the presence of these acylations at both promoters and distal enhancers, suggesting a possible alternation of the two marks to regulate transcription. At the promoter level, we observed an increase of these modifications between the meiotic and post-meiotic stages upstream of the genes characteristic of spermiogenesis. In addition, the simultaneous presence of the two marks coincides with the co-localization of several transcriptional regulators specific for this process (SLY, SOX30) and of chromatin-binding proteins (BRD4, BORIS and CTCF), whereas a binding selectivity is observed when H3K27ac and H3K27cr are identified alone at promoters. Interestingly, we observe similar results at enhancers as well as super-enhancers, confirming that the regulation of transcription is modulated by the alternative presence of these two acylations.The second part of my thesis focused on the study of the possible propionylation and butyrylation of H3K27 during yeast sporulation and mouse spermatogenesis. However, this part proved to be full of surprises because the MS/MS analyses and the comparison with the corresponding synthetic peptides did not make it possible to validate a propionylation and a butyrylation on H3K27. It turned out that the modifications observed on H3K27 from mouse histones were strictly isobaric with these known modifications, but of a different nature, since they are more hydrophilic. Several hypotheses were tested in order to determine the structure of these modifications, but at the time of finalizing this manuscript, we have not found out what it is all about.My PhD work contributes further to the idea of a dynamics between acetylation and acylations on lysine residues at the origin of the differential binding of chromatin-binding proteins responsible for regulating transcription. It also highlighted an important role of H3K27crat enhancers which are not classically considered in studies aiming at understanding the roles of new acylations
Srinivasan, Venkataraghavan. "A Biclustering Approach to Combinatorial Transcription Control". Thesis, Virginia Tech, 2005. http://hdl.handle.net/10919/43915.
Texto completoMaster of Science
Barrera, Leah Ortiz-Luis. "Genome-wide mapping and analysis of mammalian promoters". Connect to a 24 p. preview or request complete full text in PDF format. Access restricted to UC campuses, 2007. http://wwwlib.umi.com/cr/ucsd/fullcit?p3258393.
Texto completoTitle from first page of PDF file (viewed June 1, 2007). Available via ProQuest Digital Dissertations. Vita. Includes bibliographical references (p. 151-169).
Boulay, Thomas M. "Analysis of the downstream promoter element in Drosophila melanogaster and humans /". Diss., Connect to a 24 p. preview or request complete full text in PDF formate. Access restricted to UC campuses, 2005. http://wwwlib.umi.com/cr/ucsd/fullcit?p3191995.
Texto completoStaudt, Michelle Ruth. "Analysis of the principle latent promoter of Kaposi's sarcoma-associated herpesvirus". Oklahoma City : [s.n.], 2006.
Buscar texto completoMacleod, Donald T. "A molecular analysis of a promoter trap in embryonic stem systems". Thesis, University of Edinburgh, 1991. http://ethos.bl.uk/OrderDetails.do?uin=uk.bl.ethos.280628.
Texto completoFasani, Elisa. "Identification of regulatory elements responsible for metal hyperaccumulation in the Brassicaceae family. Functional analysis of the Arabidopsis thaliana MYB48 and MYB59 transcription factors". Doctoral thesis, 2014. http://hdl.handle.net/11562/671558.
Texto completoChapter 1: Identification of regulatory elements responsible for metal hyperaccumulation in the Brassicaceae family. The role of the metal transporter MTP1 in metal tolerance and accumulation has been extensively studied, due also to its great importance in the hypertolerance trait. MTP1 is known to have undergone copy number expansion in hyperaccumulator Arabidopsis halleri; moreover, possible differences in cis-regulation between hyperaccumulators and non-accumulators have been proposed. This work focuses on the analysis of the MTP1 promoter. The expression pattern and levels driven by the Arabidopsis thaliana and A. halleri promoter sequences are markedly different, coherently with the different accumulation ability and metal storage tissues displayed by the two species. MTP1 expression in roots was found in both species and is associated with the presence of root-specific cis elements in both promoters. Similarly, guard cell-specific expression was observed for both A. thaliana and A. halleri sequences and is associated with the presence of Dof-binding sites. In addition, the MTP1 promoter of A. halleri drives expression in trichomes. This interesting localization is likely associated to a couple of MYB-binding sites in the 5’UTR of the gene. Metal accumulation in trichomes is an intriguing feature in A. halleri and is possibly involved in short-term tolerance to metals. Chapter 2: Functional analysis of the Arabidopsis thaliana MYB48 and MYB59 transcription factors. MYB transcription factors are involved in many events of plant life, as cell differentiation and metabolism, plant development, response to hormones and to environmental stimuli. Among the others, MYB48 and MYB59 have been proposed to participate in secondary development, cell cycle regulation and response to abiotic stress in Arabidopsis thaliana. In this work, a myb48myb59 double mutant was used due to probable functional redundancy of the two transcription factors. myb48myb59 plants show smaller rosette leaves, likely due to reduced cell distension, delayed flowering and longer roots in comparison to wt; early senescence was also considered and confirmed by the higher SAG12 expression levels. The phenotype is consistent with a reduced cytokinin content: this observation was confirmed by the increased sensitivity to exogenous cytokinins and by the modulated genes resulting from the microarray experiment.
Francis, Zachary T. "ANALYSIS OF THE CRYPTIC PROMOTER IN THE 5’-UTR OF P27". Thesis, 2012. http://hdl.handle.net/1805/2760.
Texto completoCyclin Dependent Kinase regulation is often manipulated by cancer cells to promote unlimited proliferation. P27 is an important regulator of Cyclin E/CDK 2, which has been found in low amounts in many types of malignant cancers. Lovastatin has been shown to cause cell cycle arrest in the G1 phase of the cell cycle by increasing the P27 protein. There has been some question, however, if lovastatin regulates P27 at the transcriptional or translational level. Although it has been claimed that P27 expression regulation is due to an IRES located in its 5’UTR, other studies suggested that P27 expression is regulated at the level of transcription. To further investigate the regulation mechanism of P27 expression, the 5’-UTR of P27 and its deletion mutants were examined using a luciferase reporter gene in HeLa cells following exposure to lovastatin. It was found that lovastatin stimulated a significant 1.4 fold increase in its promoter activity of the full length 5’UTR (575). Deletion of 35 nucleotides from the 5’ end of the UTR eliminated the lovastatin-induced increase in promoter activity. Further mapping analyses of the first 35 bases showed that two regions, M1 (575-559) and M3 (543-527), were less sensitive to lovastatin than the other mutated constructs. Since M1 and M3 still showed some activity, a construct was created with deletions in both the M1 and M3 regions. This showed no increase in luciferase activity when exposed to lovastatin. Looking at RNA levels, there was a 1.5 fold increase in RNA when the full length 5’UTR was inserted into HeLa cells and exposed to 81 µM of lovastatin. In contrast, there was no increase in RNA when M1/M3 (575-559; 543-527) was inserted into HeLa cells and exposed to 81 µM of lovastatin. In addition, there was a 1.6 fold increase in endogenous P27 RNA levels after HeLa cells were exposed to 81 µM of lovastatin. In all of these experiments, there seems to be two promoters that work cooperatively: M1 (575-559) and M3 (543-527).
Huang, Yi-Chien y 黃怡倩. "Promoter analysis of rice embryogenesis". Thesis, 2002. http://ndltd.ncl.edu.tw/handle/42245248845701782564.
Texto completo國立中興大學
分子生物學研究所
90
The purpose of this study is to set up a transient assay system to analyze the important DNA sequences involved in promoter activity of rice embryo-specific genes. Two rice embryo-specific genes, Ose705 and Ose730, were used in this study. Neither the function nor the sequence of Ose705 gene has been reported in GenBank. The Ose730 gene has been identified tentatively to be a Late Embryogenesis Abundant (LEA) protein, but how these genes being regulated were still unknown. In order to understand their regulation, the upstream DNA sequences of Ose705 and Ose730 genes were deleted serially with exonuclease III to get various lengths of promoter. These promoters were then fused to a reporter GUS gene for activity assay. Rice coleoptiles and embryo-derived calli were used as materials in this transient assay. In addition to the transient assay, some deletion constructs were selected for stable transformation to further investigate their tissue-specific expression in transgenic plants. All the tested Ose705 deletion constructs including promoter length ranged from -1659 to -119 bp showed GUS activities in transient assay. The highest GUS activity was observed in the -497 bp construct suggesting the existence of a negative regulation region between -1297 and -497 bp, and possibly some positive sequence domains between -497 and -218 bp. The preliminary observations for Ose705 gene in transgenic study suggested that the sequences between -1659 and -1585 bp might contain an embryo-specific element. Another transient assay for Ose730 gene showed that the -907 bp construct had a much higher GUS activity than -2315 and all other tested constructs --- an observation consistent with the previous result obtained in transgenic assay. On the contrary, the observation that -1248 had a better GUS activity than that of -989 was not consistent with the result obtained in transgenic study. This inconsistency required further verification. However, the transient assay set-up using embryo-derived calli is reproducible and this study represents one step further in studying the regulation of embryo-specific gene in terms of the DNA sequence elements involved in regulation.
Chen, Feng-Wei y 陳逢維. "Promoter analysis of Interleukin 19". Thesis, 2002. http://ndltd.ncl.edu.tw/handle/y6v75h.
Texto completo國立成功大學
生物化學研究所
90
Cytokines are important molecules of hormones. Most of the cytokines are small to medium sized proteins which mediate potent biological effects on most cell types. Originally they are identified as being important in inflammatory processes, the development and maintenance of immune respones and haematopoiesis. A family of interleukin-10 (IL-10)-related cytokines has been emerged which include IL-19, IL-20, IL-22 [IL-10-related T-cell-derived inducible factor (IL-TIF)], IL-24 [melanoma differentiation-associated antigen 7 (MDA-7)] and IL-26 (AK155). Whereas IL-10 is a well-studied pleiotropic immunosuppressive and immun-stimulatory cytokine. It inhibits the production of IL-1, IL-6 and TNF-α. IL-22/IL-TIF can mediate acute-phase response signals in hepatocytes and IL-20 induces the hyperproliferation of keratinocytes. IL-24 is related to the suppression of tumor cell growth. But the function of IL-19 and IL-26 are still unclear. The genes for IL-10, IL-19, IL-20 and IL-24 are found within a 200kb region of chromosome 1 and the two other family members IL-22 and IL-26 are found on chromosome 12. IL-19 was first discoveried in year 2000. It shares 21% amino acid identity with the amino acid sequence of IL-10. In the previous study, it was reported that IL-10 functions as an inhibitor in immune system especial on monocyte、T cell and B cell and the production of cytokines ,such as IFN-γ. The expression of IL-19 mRNA could be induced by LPS and GM-CSF treatment in monocytes. The exon/intron structure of IL-19 is similar to that of the human IL-10 gene, comprising five exons and four introns within the coding region of the IL-19 cDNA. There are at least two distinct IL-19 mRNA species that differ in their 5'-sequences. By 5’RACE experiment, we identified the transcription start site and constructed 5 potential promoter fragments of different length upstream of exon1. We termed these five constructs to PSA、PSB、PSC、PSD、PSE and transfected these plasmid into MDCK and 293 cell lines. The results of luciferase activity showed that the PSE region expressed highest promoter activity in both MDCK and 293 cells. To find the binding protein and binding region of IL-19 promoter, we used EMSA experiment to define the binding sequence between promoter region and transcription factor. The EMSA data proved that a specific region of PSE can bind to some transcription factors contained in the nuclear extract and control the luciferase activity. In the region of nt.-141~-146 and nt.-42~-51, the HNF-5 and TFIID-MBP may bind to the DNA sequence. Furthermore, we mutated the six nucleotide of -141~-146 region in reporter vector. We found the luciferase activity of this mutant decreased 70% activity compared to the wild type control. When we treated cells with several reagents:LPS、TGF-β、IFN-γ、IL-6、GM-CSF. We found that GM-CSF could enhance the IL-19 promoter activity in 293 cell line.