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Dimerization of human immunodeficiency virus type 1 genome : dimer maturation process and role of the 5' untranslated region in dimerizationSong, Rujun. January 2008 (has links)
Human Immunodeficiency Virus type I genome consists of two identical RNA molecules that are non-covalently linked to form a dimer. HIV-1 immature and mature genomic RNA (gRNA) dimers were found in protease defective (PR -) and wild type virions, respectively, and the 5'untranslated region (5' UTR) was shown to play key roles during the genome dimerization process; but the dimerization mechanism still remains to be clarified My research project is to characterize the dimerization process and the role of 5' UTR in genome dimerization in virions produced by tissue culture cells. I'll firstly show the dimer maturation processes of HIV-1 gRNA isolated from newly released to grown-up (≥10h old) wild type, PR-, and SL1 defective (DeltaIDS) virions respectively. The results showed that HIV-1 gRNA dimer maturation process was protease-dependent and involved multiple steps: from low to high dimerization level and dimer thermostability, and from low dimer mobility to intermediate and high mobility. PR- virions did not freeze gRNA conformation in the primordial nascent state and gRNA changed from monomeric in newly released virions to half dimeric in grown-up virions, which showed that genome was packaged in the form of monomeric RNA or fragile dimers, more thermolabile than immature dimers in grown-up PR- virions. DeltaDIS inhibited gRNA dimerization by about 50% in newly released virions, though grown-up DeltaDIS gRNA was fully dimeric, which indicated that the DIS played the initiation role in gRNA dimerization in HIV-1 virions. The gRNA dimerization rate in PR- or DeltaDIS virions was much slower than that in wild type virions. These results show for the first time the whole process of dimer maturation after virion release, the gRNA conformation rearrangement in PR- virions, and the initiation role of the DIS in HIV-1 virions. Next, I'll provide a rather systematic search for the contribution of different regions in 5' UTR to HIV-1 gRNA dimerization by studying selected mutations singly or together with defective SL1. The results showed that the 5'trans-activation response element (5'TAR) was directly involved in gRNA dimerization, and a long distance base-pairing interaction between a sequence in U5 region (nts105-1l5) and another around the initiation codon of the gag gene (nts334-344) was structurally contributive to gRNA dimerization. Deletions of sequences around the 3'end of Primer Binding Site (PBS) stem-loop moderately decreased gRNA dimerization level. Other sequences in 5' UTR except DIS/SL1, which was previously known to play important roles, didn't show any systematic role. Here the results suggested that the absence of inhibition on gRNA dimerization level with defective DIS might be the compensation of the direct role of 5'TAR; and wild type-like dimerization level of DeltaTAR must be the direct contribution of the DIS.
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Characterization of the internal ribosomal entry sites located in the 5' leader of the mouse TRKB MRNA /Timmerman, Stephanie Lynn. January 2006 (has links)
Thesis (Ph.D. in Biochemistry & Molecular Genetics) -- University of Colorado at Denver and Health Sciences Center, 2006. / Typescript. Includes bibliographical references (leaves 119-131). Free to UCDHSC affiliates. Online version available via ProQuest Digital Dissertations;
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Protein primers and a telomerase-like mechanism of poliovirus RNA replication maintain the 3' end of the RNA genome /Steil, Benjamin Peter. January 2008 (has links)
Thesis (Ph.D. in Microbiology) -- University of Colorado Denver, 2008. / Typescript. Includes bibliographical references (leaves 198-225). Online version available via ProQuest Digital Dissertations.
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Selective translation of influenza viral messenger RNAs mediated by trans-acting factor(s) through an interaction with the sequence element in the 5'-untranslated region /Park, Youngwoo. January 1999 (has links)
Thesis (Ph. D.)--University of Washington, 1999. / Vita. Includes bibliographical references (leaves 126-146).
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Dimerization of human immunodeficiency virus type 1 genome : dimer maturation process and role of the 5' untranslated region in dimerizationSong, Rujun. January 2008 (has links)
No description available.
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Characterizaton of human growth hormone receptor (hGHR) gene expression in human adipocytesWei, Yuhong, 1972- January 2007 (has links)
No description available.
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Parâmetros bioinformáticos do contexto genômico como preditores do efeito funcional de substituições pontuais na sequência 5' UTR em genes humanos / Bioinformatic parameters of genomic context as predictors of functional impact in point substitutions of human gene 5' UTRUrioste, Eduardo Arcanjo, 1989- 22 August 2018 (has links)
Orientador: Sérgio Roberto Peres Line / Dissertação (mestrado) - Universidade Estadual de Campinas, Faculdade de Odontologia de Piracicaba / Made available in DSpace on 2018-08-22T18:59:49Z (GMT). No. of bitstreams: 1
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Previous issue date: 2013 / Resumo: Estima-se que cada indivíduo carregue cerca de 120 a 430 variantes raras em regiões UTRs (Abecasis et al, 2012). Apesar da tolerância a variação na região 5' UTR, a patofisiologia de várias doenças está ligada a mutações na mesma (Cazzola & Skoda, 2000; Reynolds, 2002; Chatterjee & Pal, 2009; Wethmar et al 2010), sendo necessário o entendimento a determinação dos mecanismos regulatórios. O objetivo deste trabalho é descobrir assinaturas genéticas encontradas no contexto genômico de mutações pontuais de região 5' UTR que permitam prever o impacto funcional de outras variações pontuais na mesma região. As mutações, causadora de doença, foram selecionadas do banco de dados do Human Gene Mutation Database (HGMD) (Stenson et al, 2008); e os polimorfismos, de impacto funcional desconhecido, foram obtidos no banco de dados NHLBI Grand Opportunity Exome Sequencing Project (ESP), sendo originados do trabalho de Tenessen et al (2012). No total foram utilizadas 235 mutações e 21.542 polimorfismos. Para as variações foram calculados parâmetros de variação da estabilidade da estrutura secundária do contexto das variações (??Gfolding), presença de sítios de ligação de fatores de transcrição (JASPAR), tipo de variação (transição/transversão, tipoV), distância do início da sequência codificante (DiSC), distância do início de transcrição (DiTr) e conservação filogenética por distância de Levenshtein do contexto (Lev). A estatística foi calculada pelos testes de Wilcoxon e Binomial. A partir destes foram gerados modelos de regressão logísticos analisados através de curva ROC. Os parâmetros ??Gfolding máximo, tipoV, DiSC, e Lev permitiram a distinção significativa (? = 0,05) entres os polimorfismos e as mutações permitindo modelos explicativos, mas incompletos (área da Curva ROC 0, 772). ??Gfolding max. indicou uma relação entre as mutações e entre estruturas secundárias mais estáveis geradas pelas mesmas. Os parâmetros Lev e tipoV sugerem a origem das mutações como resultantes de hotspots. O parâmetro DiSC indicou regiões com provável funcionalidade. Apesar de não ter sido possível estabelecer relação causal entre os parâmetros e o impacto funcional das variações, encontrou-se correlações importantes / Abstract: It is estimated that each individual carries about 120 to 430 rare variante in the UTR regions (Abecasis et al, 2012). Despite the increased tolerance towards variations in 5' UTR region, the patho-phisiology of several diseases is linked to its mutations (Cazzola & Skoda, 2000; Reynolds, 2002; Chatterjee & Pal, 2009; Wethmar et al 2010). Therefore it is necessary the understanding and the determination of the regulatory elements. The objective of this study is the discovery of genetic signatures found in the genomic context of disease causing point mutations in 5' UTR, thus allowing the prediction of the functional impact of other point variations in the same region. The disease causing mutations were selected from Human Gene Mutation Database (HGMD) (Stenson et al, 2008). The polymorphisms of unknown functional impact were obtained from the NHLBI Grand Opportunity Exome Sequencing Project (ESP), originated from the work of Tenessen et al (2012). A total of 235 mutations and 21,542 polymorphisms were used. For each variation, parameters related with the differences of the variation's context folding stability (??Gfolding), presence of transcription factor binding sites (JASPAR), type of variation (transition/transversion, tipoV), distance from coding sequence start (DiSC), distance from transcription start site (DiTr) and phylogenetic conservations by distance of Levenshtein from wild type to variant context (Lev). The statistical test was done by Wilcoxon and Binomial. Logistical regressions models were generated from the parameters and its performance was evaluated by a ROC curve. The parameters maximal ??Gfolding, tipoV, logarithm of DiSC and Lev allowed a significant distinction (? = 0,05) between the groups, generating models of reasonable explanation but incomplete (area under the ROC curve 0,772). Maximal ??Gfolding showed a relationship between mutations and stable secondary structures generated by them. Lev and tipoV suggested the origin of the mutation from hotspots. The DiSC parameter identified regions with possible functionality. While it was not possible to establish any clear causal relationship between the parameters and the functional impact of the variations, important correlations were found / Mestrado / Histologia e Embriologia / Mestre em Biologia Buco-Dental
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