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51	Subcellular localization and protein-protein interactions of two methyl recycling enzymes from Arabidopsis thaliana Lee, Sanghyun 08 December 2010 (has links) This thesis documents the subcellular localization and protein-protein interactions of two methyl recycling enzymes. These two enzymes, adenosine kinase (ADK) and S-adenosyl-L-homocysteine hydrolase (SAHH), are essential to sustain the hundreds of S-adenosyl-L-methionine (SAM)-dependent transmethylation reactions in plants. Both ADK and SAHH are involved in the removal of a competitive inhibitor of methyltransferases (MTs), S-adenosyl-L-homocysteine (SAH), that is generated as a by-product of the each transfer of a methyl group from SAM to a substrate. This research focused on understanding how SAH is metabolized in distinct cellular compartments to maintain MT activities required for plant growth and development. Localization studies using green fluorescent protein (GFP) fusions revealed that both ADK and SAHH localize to the cytoplasm and the nucleus, and possibly to the chloroplast, despite the fact that the primary amino acid sequence of neither protein contains detectable targeting signals. This suggested the possibility that these methyl-recycling enzymes may be targeted by specific protein-protein interactions. Moreover, deletion analysis of SAHH1 indicated that the insertion region (IR) of 41 amino acids (Gly150-Lys190), which is present only in plants and parasitic protozoan SAHHs among eukaryotes, is essential for nuclear targeting. This result suggested that the surface-exposed IR loop may serve as a binding domain for interactions with other proteins that may direct SAHH to the nucleus. To investigate protein-protein interactions, several methods were performed including co-immunoprecipitation, bimolecular fluorescence complementation, and pull-down assays. These results not only revealed that ADK and SAHH possibly interact through the IR loop of SAHH in planta, but also suggested that this interaction is either dynamic or indirect, requiring a cofactor/another protein(s) or post-translational modifications. Moreover, possible interactions of both ADK and SAHH with a putative Arabidopsis mRNA cap methyltransferase (CMT), which is localized predominantly in the nucleus, were also confirmed. These results support the hypothesis that the nuclear targeting of both SAHH and ADK can be mediated by the interaction with CMT. In addition, purification of Strep-tagged SAHH1 expressed in Arabidopsis identified a novel interaction between SAHH and aspartate-semialdehyde dehydrogenase (ASDH), an enzyme that catalyzes the second step of the aspartate-derived amino acid biosynthesis pathway. Analysis of ASDH-GFP fusions revealed that ASDH localizes to the chloroplast and the stromule-like structure that emanates from chloroplasts. Moreover the mutation in three amino acids (Pro164-Asp165-Pro166) located within the IR loop of SAHH disrupted its binding to ASDH which affected the plastid localization of SAHH, suggesting that the interaction between SAHH and ASDH is required for plastid-targeting of SAHH. Taken together, this thesis demonstrated that the localization of ADK and SAHH in or between compartments is possibly mediated by specific protein interactions, and that the surface-exposed IR loop of SAHH is crucial for these interactions. protein interaction transmethylation methyl recycling subcellular localization Adenosine kinase adenosylhomocysteine hydrolase Biology
52	Nephrin: cellular trafficking and intracellular interactions / Liu, Xiao Li, January 2004 (has links) Diss. (sammanfattning) Stockholm : Karol. inst., 2004. / Härtill 4 uppsatser.
53	Cultivo de Eucalyptus urograndis em atmosfera enriquecida com CO2: mudanças no proteoma cloroplastidial / Eucalyptus urograndis growth under CO2-enriched atmosphere: changes in the chloroplast proteome Santos, Bruna Marques dos [UNESP] 30 March 2016 (has links) Submitted by BRUNA MARQUES DOS SANTOS null (brunamarques.bio@gmail.com) on 2016-05-20T14:43:34Z No. of bitstreams: 1 Dissertação_Bruna_Marques_Santos.pdf: 2509707 bytes, checksum: d5b8e8138728f1d899f6f957bedf5425 (MD5) / Approved for entry into archive by Juliano Benedito Ferreira (julianoferreira@reitoria.unesp.br) on 2016-05-24T14:23:17Z (GMT) No. of bitstreams: 1 santos_bm_me_jabo.pdf: 2509707 bytes, checksum: d5b8e8138728f1d899f6f957bedf5425 (MD5) / Made available in DSpace on 2016-05-24T14:23:17Z (GMT). No. of bitstreams: 1 santos_bm_me_jabo.pdf: 2509707 bytes, checksum: d5b8e8138728f1d899f6f957bedf5425 (MD5) Previous issue date: 2016-03-30 / Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP) / A emissão de dióxido de carbono (CO2) pelas atividades humanas vem aumentando desde a revolução industrial. Previsões indicam que ocorrerá um aumento expressivo da concentração atmosférica deste gás nos próximos anos. Este fato deve resultar em alterações metabólicas nas plantas e, por consequência, impactar o setor florestal brasileiro. Os cloroplastos são as organelas-chave na fixação do CO2 e início do particionamento do carbono nas plantas. Alterações na disponibilidade de CO2 podem afetar o metabolismo dessas organelas. O objetivo do presente trabalho foi avaliar se o cultivo de plantas jovens de Eucalyptus urograndis em ambiente enriquecido com CO2 resulta em alterações no proteoma cloroplastidial. Para tanto, primeiramente foram avaliados diferentes métodos de isolamento de cloroplastos quanto aos seguintes parâmetros: morfologia dos cloroplastos observada em microscopia de luz (1); rendimento protéico após isolamento plastidial (2); grau de contaminação por proteínas não cloropastidiais (3); e abundância em número de proteínas identificadas e já descritas como plastidiais (4). Após a definição da melhor metodologia para obtenção do proteoma cloroplastidial, mudas de Eucalyptus urograndis de aproximadamente três meses de idade foram cultivadas sob concentrações atmosféricas controladas de CO2 (400 e 1000 ppm) durante dez semanas. A avaliação do proteoma plastidial, por buscas restringentes contra um banco de dados de sequências protéicas de Eucalyptus grandis, resultou na identificação de 816 proteínas em E. urograndis, das quais 80% já haviam sido descritas como plastidiais. O mapeamento in silico de vias metabólicas resultou na identificação de todas as proteínas envolvidas no ciclo de Calvin-Benson, além da detecção de um aumento discreto, porém significativo na abundância de enzimas-chave: PGK, GAPDH, FBA, FBPase, SBPase e RPI. Embora a avaliação da eficiência quântica do fotossitema II tenha indicado ausência de alteração fotossintética, as plantas tratadas com 1000 ppm de CO2 apresentaram fechamento estomático em resposta à condição ambiental imposta, além da diminuição na área do tecido vascular foliar. Esta é a primeira caracterização do proteoma cloroplastidial do gênero Eucalyptus, cujos resultados indicam que a atmosfera enriquecida com CO2 causou respostas na espécie, incluindo um aumento na abundância de proteínas envolvidas na fixação de carbono. Os resultados apresentados aqui podem auxiliar na compreensão das respostas bioquímicas estimuladas por um aumento na concentração atmosférica de CO2 em plantas do tipo C3, além de contribuir para programas de melhoramento que visem obter plantas adaptadas às condições climáticas futuras. / Carbon dioxide (CO2) emissions from human activities have increased since the industrial revolution. Global projections indicate that there will be a significant increase in the atmospheric concentration of this gas in the coming years. This fact can result in metabolic changes in plants and, consequently, affect the Brazilian forest sector. Chloroplasts are key organelles in carbon fixation and early carbon partitioning in plants. Changes in the availability of CO2 may affect the metabolism of these organelles. The goal of the present study was to assess whether the cultivation of seedlings of Eucalyptus urograndis under a CO2 enriched environment could result in changes in the chloroplast proteome. For this purpose, different chloroplast isolation methods were evaluated to the following parameters: chloroplast morphology observed in bright-field microscopy (1); protein yield after plastid isolation (2); degree of contamination by non-plastidic proteins (3); and abundance in the number of identified proteins described as plastidic (4). After determining the best methodology for the isolation of the chloroplast proteome, E. urograndis seedlings about three months old were grown under CO2 controlled atmospheric concentrations (400 and 1000 ppm) for ten weeks. Evaluation of the plastid proteome, using stringent search against a protein sequence database from Eucalyptus grandis, resulted in the identification of 816 proteins in E. urograndis, from which 80% were already described as plastidic. In silico metabolic pathway mapping resulted in the identification of all proteins involved in the Calvin-Benson cycle and detection of a slight but significant increase in the abundance of key enzymes: PGK, GAPDH, FBA, FBPase, SBPase, and RPI. Although the assessment of the quantum efficiency of photosystem II suggested the absence of changes in the photosynthesis rate, plants treated with 1000 ppm of CO2 presented stomatal closure in response to the imposed environmental condition. A decreased area of the leaf vascular tissue was also detected in young leaves. This is the first characterization of chloroplast proteome of the genus Eucalyptus. Our results indicate that the CO2 enriched atmosphere stimulated metabolic responses, including an increase in the abundance of proteins involved in carbon fixation. Results showed here will assist on the understanding of the biochemical responses stimulated by an increase in the atmospheric CO2 concentration in C3-type plants, and contribute to breeding programs that aim to obtain plants adapted to future climate conditions. / FAPESP: 2014/07454-0 Assimilação de carbono Mudanças climáticas globais Proteômica subcelular Carbon assimilation Global climate change Subcellular proteomics
54	Localização subcelular de proteinas de cana-de-açucar (Sccharum spp.) : caracterização in silico e avaliação funcional / Subcellular localization of sugarcane (Sccharum spp.) proteins : in silico characterization and functional evaluation Vicentini, Renato, 1979- 06 March 2008 (has links) Orientador: Marcelo Menossi Teixeira / Tese (doutorado) - Universidade Estadual de Campinas, Instituto de Biologia / Made available in DSpace on 2018-08-11T15:42:58Z (GMT). No. of bitstreams: 1 Vicentini_Renato_D.pdf: 5901500 bytes, checksum: 7c8fe505e4c1675900f96c6643895d32 (MD5) Previous issue date: 2008 / Resumo: As células de plantas são altamente organizadas e muitos processos biológicos estão associados com estruturas subcelulares específicas. A localização subcelular é uma característica chave das proteínas, visto que está relacionada com a função biológica. A determinação da localização subcelular usando a predição é uma estratégia altamente desejável, principalmente porque as abordagens experimentais demandam um tempo considerável. Com o objetivo de desenvolver um método para melhorar a predição de localização subcelular, diversos algoritmos foram integrados visando à exploração ótima do potencial de cada um. O desempenho com 90% de exatidão deste novo método foi claramente superior a todos os métodos utilizados em sua criação. Usando esta estratégia foi realizada a primeira análise em larga escala da localização subcelular do proteoma de cana-de-açúcar (com 11.882 proteínas preditas), sendo encontrado que a maioria das proteínas estão localizadas em quatro compartimentos: núcleo (44%), citoplasma (19%), mitocôndria (12%), e extracelular (11%). Adicionalmente foi observado que cerca de 19% das proteínas são localizadas em múltiplos compartimentos. Outros resultados foram capazes de identificar um conjunto de proteínas de cana-de-açúcar que podem apresentar duplo direcionamento pelo uso de variações na extremidade amino. Utilizando expressão transiente em células da epiderme de cebola, foi investigada a localização subcelular de 96 proteínas de cana com fusão a proteína GFP. As construções contendo fusão amino- e carboxi-terminal dos genes foram expressas, e a localização das proteínas de fusão foi detectada por microscopia de fluorescência. É relatado também a caracterização do gene ScBAK1, um receptor do tipo quinase com repetições ricas em leucina, que apresenta similaridade de seqüência com o gene brassinosteroid insensitive1-associated receptor kinase1. Foi mostrado que transcritos desse gene se acumulam em níveis muito mais altos nas células da bainha do feixe vascular do que nas células do mesófilo, e que a fusão ScBAK1-GFP é localizada na membrana plasmática. Essa distribuição espacial e esse padrão de expressão indicam que a ScBAK1 pode estar potencialmente envolvida em cascatas de sinalização celular intermediadas por altos níveis de açúcar na folha. Ainda considerando estudos de localização subcelular, é conhecido que seqüências de nucleotídeos que flanqueiam o códon de início da tradução afetam a eficiência traducional dos mRNA, e podem indicar a presença de sítios de inicio de tradução (TIS) alternativos. O multi-direcionamento pode ser um reflexo da variabilidade traducional destas outras formas da proteína. Neste estudo foi desenvolvido um método computacional para investigar o uso de TISs alternativos na síntese de novas variantes protéicas que podem apresentar localização subcelular diferente. Visando contribuir para o nosso entendimento da complexidade do genoma da cana-de-açúcar, foi empregada uma análise em larga escala dos TIS nesta espécie. Também é demonstrado que os transcritos com expressão induzida apresentam um forte TIS quando comparados com os reprimidos, e que os transcritos constitutivos possuem uma alta freqüência de TIS alternativos. O mesmo ocorre para os genes com altas taxas evolutivas, e transcritos específicos de folhas e entrenós, levantando a hipótese de que esses genes possam codificar diferentes polipeptídeos / Abstract: Plant cells are highly organized and many biological processes are associated with specialized subcellular structures. Subcellular localization is a key feature of proteins, since it is related to biological function. The determination of subcellular localization using computational prediction is a highly desirable strategy because experimental approaches are time-consuming. In order to develop a method for the enhanced prediction of subcellular localization, the outputs of some prediction tools were integrated so as to optimally exploit the potential of each one. The prediction performance (with 90%of accuracy) of this new method was clearly superior to all the methods used to create the predictor. Using this method, the first in silico genome-wide subcellular localization analysis was performed for sugarcane (with 11,882 predicted proteins). It was found that most of the proteins are localized to four compartments: nucleus (44%), cytosol (19%), mitochondria (12%), and secretory destination (11%). It is also shown that about 19%of the proteins are localized to multiple compartments, and that a potential set of sugarcane proteins can show dual targeting by use of N-truncated form of proteins. The subcellular localization of 96 sugarcane proteins fused with GFP were evaluated using transient expression in onion epidermal cells. Constructs containing the Nand C-terminal fusion of genes encoding both endogen and GFP proteins were transiently expressed, and the localization of the fusion proteins were detected by fluorescent microscopy. It was reported the characterization of ScBAK1, a sugarcane leucine-rich repeat receptor-like kinase, with sequence similarity to brassinosteroid insensitive1-associated receptor kinase1. We have found that ScBAK1 transcripts accumulated at higher levels in bundle-sheath than in mesophyll cells. ScBAK1-GFP fusions were localized to the plasma membrane. This spatial distribution and expression pattern indicates that ScBAK1 might be potentially involved in cellular signaling cascades mediated by high levels of sugar in this organ. The nucleotide sequence flanking the translation initiation codon affects the translational efficiency of eukaryotic mRNAs, and may indicate the presence of an alternative translation initiation site (TIS) to produce proteins with different properties. Multi-targeting may reflect the translational variability of these other protein forms. In this study it was also developed a computational method to investigate the usage of alternative TISs for the synthesis of new protein variants that might have different subcellular localization. To contribute to our understanding of the genome complexity of sugarcane, we undertook a genome wide TIS analysis in sugarcane data. It is demonstrated that up-regulated transcripts show a stronger TIS when compared with the down-regulated, and that ubiquitous transcripts have a high frequency of alternative TIS in the next downstream AUG codon. The same occurs for fast-evolving genes, and leaf and internodes specific transcripts, that may encode different polypeptides by N-terminal polymorphism / Doutorado / Genetica Vegetal e Melhoramento / Doutor em Genetica e Biologia Molecular Localização subcelular Proteinas - Tradução Cana-de-açúcar Subcellular localization Proteins - Translation Sugarcane
55	O papel da fosforilação de maspina em resíduos de tirosina / Rolle of maspin phosphorylation on tyrosine residues Mariana Tamazato Longhi 30 October 2012 (has links) Maspina (mammary serpin) foi identificada em 1994 como uma serpina (serine protease inhibitor) que apresenta atividade de supressão tumoral. Foi classificada como uma serpina devido à homologia na sequência de aminoácidos, porém, maspina não apresenta atividade de inibição de serina proteases. Entre os efeitos biológicos de maspina estão a modulação da adesão, a inibição do crescimento e a invasão tumoral, a inibição da angiogênese, o efeito pró-apoptótico e o controle da resposta ao stress oxidativo, propriedades que contribuem para supressão tumoral. Esta diversidade de funções se reflete nos inúmeros ligantes de maspina e na sua localização subcelular, já que é encontrada na membrana plasmática, no citoplasma, núcleo e mitocôndrias. A localização subcelular de maspina guarda importante relação com sua função, já que foi demonstrado que sua localização nuclear está correlacionada com bom prognóstico em diversos tumores e seu efeito supressor de tumor foi observado somente quando maspina está localizada no núcleo. Entre os ligantes de maspina estão a HDAC1, IRF6, GST, HSP90 e HSP70, β1 integrina, uPAR e colágeno tipo I e III. O mecanismo molecular envolvido na regulação dessas atividades não foi elucidado, e até o momento, somente um gene e uma proteína de maspina foram descritos, desta forma alterações pós-traducionais devem estar envolvidas na regulação dessas atividades. Com objetivo de verificar se há modificações pós-traducionais em maspina, utilizamos células MCF10A, que expressam grande quantidade dessa proteína, e submetemos seu extrato proteico à separação por gel bidimensional seguido de western blot. Identificamos quatro formas de maspina com a mesma massa molecular (42kDa), mas pontos isoelétricos distintos. Três destas formas são sensíveis ao tratamento com fosfatase ácida, o que sugere que estas sejam fosforiladas. Utilizamos ainda peroxidovanadato de sódio, um potente inibidor de tirosina fosfatase para investigar o papel da fosforilação de maspina em resíduos de tirosina. Através de western blot e imunofluorescência, observamos que o tratamento das células com o inibidor resultou no aumento dos níveis celulares de maspina assim como no seu acúmulo no citoplasma. Deste modo, concluímos que existem três diferentes fosfoformas de maspina em células MCF10A e ainda a inibição de tirosinas fosfatases aumentam os níveis de maspina e resultam no acúmulo da proteína no citoplasma. Esses resultados sugerem que a fosforilação pode estar envolvida na localização subcelular de maspina e na regulação dos seus níveis proteicos na célula. / Maspin (mammary serpin) was identified in 1994 as a serpin (serine protease inhibitor) which presents tumor suppressor activity. It was classified as a serpin due to its homology in amino acids sequence; however, maspin doesn\'t exhibit serine protease inhibition activity. Among maspin biological effects are modulation of cell adhesion, inhibition of tumor growth, invasion and angiogenesis, a pro-apoptotic effect and control of oxidative stress response, properties which contribute to tumor suppression. This functional diversity reflects maspin numerous ligands and its subcellular localization, since it is found on the plasma membrane, in the cytoplasm, nucleus and in mitochondria. Maspin subcellular localization is closely related to its function, as its nuclear localization correlates with good prognostic in several tumors and maspin tumor suppressor activity is only observed when it is located in the nucleus. Among maspin ligands are histone H1 deacetylase, IRF6, GST, HSP90 e HSP70, β1 integrin, uPAR and type I and III collagen. The molecular mechanisms involved in the regulation of maspin biological activities are poorly understood. So far, only one gene and one protein have been assigned to maspin, so posttranslational modification should be involved. In order to verify posttranslational modification in maspin, we utilized MCF10A cells, which express great amount of this protein, and we submitted its proteic extract to 2D-SDS-PAGE followed by western blot. We identified four maspin forms with the same molecular mass (42kDa), but different isoelectric point. Three of these forms are sensitive to acidic phosphatase treatment, suggesting that they are phosphorylated maspin forms. We also utilized sodium peroxovanadate, a potent tyrosine phosphatase inhibitor to investigate the role of maspin tyrosine phosphorylation. Through western blot and immunofluorescence analyses, we observed that cell treatment resulted in increase in maspin cellular levels as well as its cytoplasmic accumulation. Thus, we concluded that there are three diferente maspin phosphoforms in MCF10A cells and yet tyrosine phosphatase inhibition increases maspin levels and results in accumulation of the protein in the cytoplasm. These data suggest that phosphorylation may be involved in maspin subcellular localization and regulation of its protein levels in the cell. Células MCF10A Fosforilação Localização subcelular Maspina Tirosina Maspin MCF10A cells Phosphorylation Subcellular localization Tyrosine
56	Análise molecular de genes relacionados à síndrome de Pendred em indivíduos com surdez e estudo funcional da proteína pendrina = Molecular analysis of genes related to Pendred syndrome in individuals with deafness and functional study of pendrin protein / Molecular analysis of genes related to Pendred syndrome in individuals with deafness and functional study of pendrin protein De Moraes, Vanessa Cristine Sousa, 1984- 23 August 2018 (has links) Orientador: Edi Lúcia Sartorato / Tese (doutorado) - Universidade Estadual de Campinas, Instituto de Biologia / Made available in DSpace on 2018-08-23T15:12:43Z (GMT). No. of bitstreams: 1 DeMoraes_VanessaCristineSousa_D.pdf: 4935241 bytes, checksum: ce8c385da6e3872d30f08426c629d34d (MD5) Previous issue date: 2013 / Resumo: O alargamento do aqueduto vestibular (EVA) é uma malformação da orelha interna que pode ser identificado por tomografia computadorizada ou ressonância magnética. O EVA é um dos principais sinais clínicos da Síndrome de Pendred (PDS), uma doença genética com padrão de herança autossômico recessivo causada na maioria dos casos por mutações no gene SLC26A4. Além de EVA, o bócio e defeito na organificação do iodeto na tireóide são achados clínicos típicos da PDS. Por sua vez, mutações no gene SLC26A4 têm também sido observadas em indivíduos com surdez não sindrômica associada ao EVA. Recentemente os genes FOXI1 e KCNJ10 também foram implicados na PDS. O gene FOXI1 é um fator de transcrição do gene SLC26A4. Medições electrofisiológicas mostraram que a alteração da pendrina, proteína codificada pelo gene SLC26A4, em modelos animais levava indivíduos à surdez pela falta do potencial endococlear devido à perda de expressão de canais potássio. Sendo atribuído ao gene KCNJ10 a função de manutenção do potencial endococlear. Desta maneira, o presente estudo teve como objetivo avaliar a ocorrência de mutações nos genes SLC26A4, FOXI1 e KCNJ10 em 60 indivíduos brasileiros portadores de perda auditiva sensorioneural, associada ou não a alterações no aqueduto vestibular. Foram encontradas 14 diferentes alterações no gene SLC26A4, das quais 3 ainda não haviam sido descritas na literatura (P142L, G149R e C282Y) e 4 já haviam sido descritas, porém ainda não haviam sido caracterizadas funcionalmente (T193I, Q413R, L445W e R776C). Dessa forma, foi realizada a análise funcional e a co-localização celular da proteína Pendrina com estas 7 variações alélicas. Não foi encontrada nenhuma evidência de contribuição digênica relacionada ao gene FOXI1 e/ou KCNJ10, uma vez que nenhum paciente desta casuística com alteração no gene SLC26A4 apresentou mutações nesses genes. Além disso, no grupo composto por 30 indivíduos surdos que não apresentam EVA, ficou evidente que o rastreamento do gene SLC26A4 não foi suficiente para explicar a perda auditiva nesses pacientes, uma vez que foram encontradas apenas alterações em um alelo do gene. Por outro lado, no grupo formado por 30 indivíduos surdos que apresentam EVA, o rastreamento do gene SLC26A4 possibilitou o esclarecimento do diagnóstico etiológico da perda auditiva em 5 pacientes que apresentaram mutações nos dois alelos do gene SLC26A4 / Abstract: Enlargement of the vestibular aqueduct (EVA) is a malformation of the inner ear that can be identified by computed tomography or magnetic resonance imaging. EVA is the main feature of Pendred syndrome (PDS), a genetic disease with autosomal recessive inheritance pattern, in most cases caused by mutations in the SLC26A4 gene. Besides EVA, goiter and defective organification of iodide in the thyroid are other typical clinical signs of PDS. In turn, SLC26A4 gene mutations have been also observed in patients with non-syndromic deafness associated with EVA. Recently the genes FOXI1 and KCNJ10 were also implicated in the PDS. The FOXI1 gene is a transcription factor of SLC26A4 gene. Electrophysiological measurements in animal models showed that the mutated pendrin, the protein encoded by the SLC26A4 gene, led individuals to deafness by the lack of endocochlear potential due to loss of expression of potassium channels. Being assigned to the KCNJ10 gene the maintenance of endocochlear potential. Thus, the present study aimed to evaluate the occurrence of mutations in SLC26A4, and KCNJ10 FOXI1 genes in 60 Brazilian patients with sensorineural hearing loss, with or without changes in the vestibular aqueduct. We found 14 different mutations in SLC26A4 gene, of which 3 had not yet been described in the literature (P142L, G149R and C282Y) and 4 had already been described, but had not been characterized functionally yet (T193I, Q413R, L445W and R776C). Thus, we performed the functional analysis and cellular co-localization of Pendrin protein with these 7 allelic variants. We found no evidence of digenic contribution related to FOXI1 and/or KCNJ10 genes, since no patient in with mutations in SLC26A4 gene showed mutations in these genes. In addition, the screening of SLC26A4 gene in 30 deaf individuals with no EVA was not sufficient to explain the hearing loss in these patients, since mutations were found only in one allele of the gene. On the other hand, the screening of SLC26A4 gene in 30 deaf individuals with EVA allowed the elucidation of the etiology of hearing loss in 5 patients with mutations in both alleles of this gene / Doutorado / Genetica Animal e Evolução / Doutora em Genética e Biologia Molecular Síndrome de Pendred Surdez Análise funcional Localização subcelular Mutação Pendred syndrome Deafness Functional analysis Subcellular localization Mutation
57	A computational investigation of solubility, functionality and the adaptation in subcellular compartments of proteins Chan, Pedro January 2011 (has links) A cell is considered to be the smallest unit of life. It carries out a variety of biochemical reactions through the activities of proteins and protein enzymes. In order to perform functions, proteins must be in their native folded state together with the correct environmental conditions. A slight change in pH or temperature could cause disruption to the electrostatic interactions within the protein, thus leading to conformational change and the loss of activity. Studies have shown that solubility could be enhanced by increasing the number of charges on the protein surface. And from the studies of extremophiles, we learned that the presence of non-polar aromatic residues could be a key for thermostable proteins. Thus, charges are important to determine the function and adaptation of proteins.Over the decades, large amount of protein sequence and structure information relating to molecular biology has been produced. By employing algorithms, computational and statistical techniques, it is possible to analyse these data to solve biological problems. Often these investigations are based mainly on sequences since their numbers outstrip the number of available structures. However, adding structures would allow us to investigate problems such as the relationship between charges, sequence, structure and functions, which is the aim of this study.In this thesis, the relationships between proteins and function were examined by various electrostatic features derived from charges and also geometric properties from structures. One interesting finding is that the averaged value of pH of maximum stability of proteins within a subcellular location was highly correlated to the pH of that subcellular compartment, which was due to pKas (of histidines), and their locations on the proteins. We also found that the size of the largest non-charged patch on the protein surface correlates with solubility and provides a predictor with a maximum accuracy of 76%. The use of novel charge-based methods shows little improvement in distinguishing between enzymes and non-enzymes. However, the method of using real charges with grid size of 1 angstrom has paved a way into the idea of using charges and dipoles pattern from enzyme active site to distinguish different enzymes. Finally, a web-tool for displaying conserved residues on 3D protein structure is made available to the public for identifying residues that may be of functional importance. 572
58	Conjugated Polymer Nanoparticles for Biological Labeling and Delivery Mendez, Eladio A 18 March 2015 (has links) Cancer remains one of the world’s most devastating diseases, with more than 10 million new cases every year. However, traditional treatments have proven insufficient for successful medical management of cancer due to the chemotherapeutics’ difficulty in achieving therapeutic concentrations at the target site, non-specific cytotoxicity to normal tissues, and limited systemic circulation lifetime. Although, a concerted effort has been placed in developing and successfully employing nanoparticle(NP)-based drug delivery vehicles successfully mitigate the physiochemical and pharmacological limitations of chemotherapeutics, work towards controlling the subcellular fate of the carrier, and ultimately its payload, has been limited. Because efficient therapeutic action requires drug delivery to specific organelles, the subcellular barrier remains critical obstacle to maximize the full potential of NP-based delivery vehicles. The aim of my dissertation work is to better understand how NP-delivery vehicles’ structural, chemical, and physical properties affect the internalization method and subcellular localization of the nanocarrier. In this work we explored how side-chain and backbone modifications affect the conjugated polymer nanoparticle (CPN) toxicity and subcellular localization. We discovered how subtle chemical modifications had profound consequences on the polymer’s accumulation inside the cell and cellular retention. We also examined how complexation of CPN with polysaccharides affects uptake efficiency and subcellular localization. This work also presents how changes to CPN backbone biodegradability can significantly affect the subcellular localization of the material. A series of triphenyl phosphonium-containing CPNs were synthesized and the effect of backbone modifications have on the cellular toxicity and intracellular fate of the material. A mitochondrial-specific polymer exhibiting time-dependent release is reported. Finally, we present a novel polymerization technique which allows for the controlled incorporation of electron-accepting benzothiadiazole units onto the polymer chain. This facilitates tuning CPN emission towards red emission. The work presented here, specifically, the effect that side-chain and structure, polysaccharide formulation and CPN degradability have on material’s uptake behavior, can help maximize the full potential of NP-based delivery vehicles for improved chemotherapeutic drug delivery. Conjugated Polymers Nanoparticles Drug Delivery Cellular Labeling Subcellular localization Cytotoxicity Materials Chemistry Nanotechnology Organic Chemistry
59	Caracterização da fosforilação de maspina no desenvolvimento da glândula mamária murina e a correlação com sua localização subcelular. / Characterization of maspin phosphorylation in the development of the murine mammary gland and the correlation with subcellular localization. Magna Magalhães Silva 10 September 2015 (has links) Maspina é uma proteína supressora de tumor e metástase e sua localização subcelular está relacionada ao prognóstico do câncer de mama. Nosso grupo mostrou em MCF-10A que quando fosforilada maspina se acumula no citoplasma. Porém, esta correlação ainda não foi relatada in vivo. Aqui investigamos a expressão, fosforilação e localização subcelular de maspina ao longo do desenvolvimento da glândula mamária murina. Maspina foi detectada no estágio mais tardio da gestação, na lactação e na involução. Os níveis de fosforilação de maspina são maiores no período de lactação do que na involução. Interessantemente, a porcentagem de células que apresenta maspina no núcleo é maior na fase de involução do que na fase de lactação Estes dados mostram que a correlação entre níveis de fosforilação de maspina e localização subcelular também é observada in vivo e que esses processos são reguladas ao longo do desenvolvimento na glândula mamária murina. / Maspin is a protein with tumor and metastasis suppressing activity and its subcellular localization is related to breast cancer prognosis. Using MCF-10A cells as a model system, our group demonstrated a correlation between maspin phosphorylation and cytoplasmic accumulation. Here we investigated maspin expression, phosphorylation levels and subcellular localization in vivo during the murine mammary gland development. Maspin was detected in late pregnancy, during lactation and involution. Maspin phosphorylation levels is higher during lactation than during involution. Interestingly, the percentage of cells which present nuclear maspin is higher in the involution than in lactation. These data show that the correlation between maspin phosphorylation and subcellular localization is also observed in vivo and these processes are regulated during murine mammary gland development. Fosforilação Glândula mamária Localização subcelular Maspina Núcleo Mammary gland Maspin Nucleus Phosphorylation Subcellular localization
60	Metabolic engineering of plants using a disarmed potyvirus vector Majer, Eszter 01 September 2016 (has links) [EN] Plant viruses are obligate intracellular parasites which were used to develop recombinant plant virus vectors to express heterologous proteins and to modify endogenous metabolic pathways of natural products in plants. The main limitation of many plant virus-based systems is the difficulty to co-express various heterologous proteins in the same cell with proper subcellular localization, which is a crucial question in metabolic engineering. This work provides a solution to overcome this problem by using a potyvirus-based vector system. Potyviruses (genus Potyvirus, family Potyviridae) are plus-strand single-stranded RNA viruses, which have a genome expression strategy that allows the equimolar production of most viral proteins. On the basis of an infectious clone of Tobacco etch virus (TEV), Bedoya et al. (2010) developed an expression system in which the RNA-dependent RNA polymerase (NIb) gene was replaced by an expression cassette, harboring several heterologous proteins. This viral vector was able to express three fluorescent proteins with nucleocytoplasmic localization in equimolar amounts in transgenic tobacco plants in which NIb was supplemented in trans. Despite of the apparent simplicity of potyvirus genome expression strategy, foreign cDNA insertion is a complicated task. Thus, our first goal was to analyze the effect of gene insertion on TEV genome stability. As a result of this work, a novel insertion position was discovered at the amino-terminal end of the potyvirus polyprotein, which opened the possibility to explore new questions of recombinant protein expression. Since metabolic pathways are highly compartmentalized, proper subcellular targeting of enzymes is an essential task. Thus, our second objective centralized on the subcellular targeting of expressed proteins from the TEV-based viral vector. cDNAs coding for the green fluorescent protein (GFP) fused to chloroplast, nucleus and mitochondria targeting signal sequences were inserted into the newly described amino-terminal insertion position or into an internal site, replacing the NIb cistron. Our results showed that for protein delivery to chloroplasts and mitochondria, foreign genes have to be inserted at the amino-terminal site of the viral vector, but for nuclear delivery, both insertion positions are suitable. The last objective of this work was to investigate whether the potyvirus-based vector was able to express an entire heterologous multistep biosynthetic pathway in plant cells. For this aim we purposed to produce lycopene, a plant pigment with health promoting properties. To do so, we inserted cDNAs coding for the enzymes of a three-step metabolic pathway of bacterial origin into the potyvirus-based vector. Infected tobacco plants developed orange symptoms indicating lycopene accumulation, which was confirmed by high-performance liquid chromatography analysis and microscopy observations. Our results also illustrated that the sole expression of Pantoea ananatis phytoene synthase, crtB, is enough to induce carotenoid accumulation, conferring yellow coloration to the infected tissue and serves as reporter system to visually track viral infection in several plant species. / [ES] Los virus de plantas son parásitos intracelulares obligados que han sido utilizados para desarrollar vectores virales y expresar proteínas heterólogas y modificar rutas metabólicas endógenas de productos naturales. La principal limitación de muchos sistemas basados en virus de plantas es la dificultad de coexpresar diversas proteínas heterólogas en la misma célula con la localización subcelular apropiada, lo cual es una cuestión crucial en ingeniería metabólica. Este trabajo presenta una solución para superar este problema mediante el uso de un vector viral basado en un potyvirus. Los potyvirus (género Potyvirus, familia Potyviridae) son virus de RNA de cadena positiva simple que tienen una estrategia de expresión génica que permite la producción de la mayoría de las proteínas virales en cantidades equimolares. Basado en un clon infeccioso del virus del grabado del tabaco (Tobacco etch virus, TEV) Bedoya et al. (2010) desarrollaron un sistema de expresión en el que el gen de la RNA polimerasa dependiente de RNA (NIb) fue sustituido por un casete de expresión, que albergaba varias proteínas heterólogas. Este vector viral fue capaz de expresar tres proteínas fluorescentes con localización nucleocitoplásmica en cantidades equimolares en plantas de tabaco transgénicas que complementaban el cistron NIb en trans. A pesar de la aparente simplicidad de la estrategia de expresión génica de los potyvirus, la inserción de un cDNA foráneo es una tarea complicada. Por lo tanto, nuestro primer objetivo fue analizar el efecto de la inserción en la estabilidad del genoma de TEV. Como resultado de este trabajo, descubrimos una nueva posición de inserción en el extremo amino-terminal de la poliproteína viral que nos permitió explorar otras cuestiones sobre la expresión de proteínas recombinantes. Dado que las vías metabólicas son muy compartimentalizadas, la adecuada localización subcelular de enzimas es una tarea esencial en ingeniería metabólica. Por eso, nuestro segundo objetivo se centró en la distribución de las proteínas heterológas expresadas con el vector viral a diferentes orgánulos subcelulares. cDNAs que codificaban la proteína fluorescente verde (green fluorescent protein, GFP) fusionada a péptidos señal se insertaron en la nueva posición amino-terminal y en un sitio interno, sustituyendo el cistrón NIb, para enviarla al cloroplasto, núcleo y a la mitocondria. Nuestros resultados mostraron que para la distribución de proteínas al cloroplasto y mitocondria, los genes foráneos deben ser insertados en el sitio amino-terminal del vector viral, pero para la distribución nuclear, ambas posiciones son adecuadas. El último objetivo de este trabajo fue estudiar si el vector viral basado en potyvirus es capaz de expresar una ruta biosíntética de múltiples pasos en células vegetales. Para ello nos propusimos producir licopeno, un pigmento vegetal con propiedades beneficiosas para la salud humana. Para ello, insertamos un cDNA que codificaba las enzimas de una ruta metabólica de tres pasos de origen bacteriano en el vector viral. Las plantas de tabaco infectadas con el vector viral desarrollaron síntomas de color naranja indicando la acumulación de licopeno, que fue confirmado por análisis de cromatografía líquida de alta eficacia y observaciones de microscopía. Nuestros resultados también ilustraron que la sola expresión de la fitoeno sintasa de Pantonea ananatis, crtB, es suficiente para inducir la acumulación de carotenoides que confieren una coloración amarilla al tejido infectado y sirve como sistema reportero visual en varias especies de plantas. / [CAT] Els virus de plantes són paràsits intracel·lulars obligats que han estat utilitzats per a desenvolupar vectors virals i expressar proteïnes heteròlogues y modificar rutes metabòliques endògenes de productes naturals silenciant certs gens o expressant factors de transcripció i enzims metabòlics. La principal limitació de molts sistemes basats en virus de plantes és la dificultat de coexpressar diverses proteïnes heteròlogues en la mateixa cèl·lula amb la localització subcel·lular apropiada, cosa que és una qüestió crucial en enginyeria metabòlica. Aquest treball presenta una solució per a superar aquest problema mitjançant l'ús d'un vector viral basat en un potyvirus. Els potyvirus (gènere Potyvirus, família Potyviridae) són virus d'RNA de cadena positiva simple que tenen una estratègia d'expressió gènica que permet la producció de la majoria de les proteïnes virals en quantitats equimolars. Basat en un clon infecciós del virus del gravat del tabac (Tobacco etch virus, TEV) Bedoya et al. (2010) van desenvolupar un sistema d'expressió en el qual el gen de l'RNA polimerasa depenent d'RNA (NIb) va ser substituït per un casset d'expressió, que albergava diverses proteïnes heteròlogues. Aquest vector viral va ser capaç d'expressar tres proteïnes fluorescents amb localització nucleocitoplàsmica en quantitats equimolars en plantes de tabac transgèniques que complementaven el cistró NIb en trans. Malgrat l'aparent simplicitat de l'estratègia d'expressió gènica dels potyvirus, la inserció d'un cDNA forà és una tasca complicada. Per tant, el nostre primer objectiu va ser analitzar l'efecte de la inserció en l'estabilitat del genoma de TEV. Com a resultat d'aquest treball, hem descobert una nova posició d'inserció en l'extrem amino terminal de la poliproteïna viral que ens va permetre explorar altres qüestions sobre l'expressió de proteïnes recombinants. Atès que les vies metabòliques són molt compartimentalitzades, l'adequada localització subcel·lular d'enzims és una tasca essencial en enginyeria metabòlica. Per açò, el nostre segon objectiu es va centrar en la distribució de les proteïnes heteròlogues expressades amb el vector viral a diferents orgànuls subcelul·lars. cDNAs que codificaven la proteïna fluorescent verda (green fluorescent protein, GFP) fusionada a pèptids senyal es van inserir en la nova posició amino terminal i en un lloc intern, substituint el cistró NIb, per a enviar-la al cloroplast, nucli i al mitocondri. Els nostres resultats van mostrar que per a la distribució de proteïnes al cloroplast i mitocondri, els gens forans han de ser inserits en el lloc amino terminal del vector viral, però per a la distribució nuclear, ambdues posicions són adequades. El lloc amino terminal va resultar ser més adequat per a produir quantitats més grans de proteïnes recombinants, però el lloc d'inserció intern va demostrar ser més estable. Sobre la base d'aquests resultats, hem sigut capaços de distribuir dues proteïnes fluorescents diferents als cloroplasts i nuclis des d'un únic vector viral. L'últim objectiu d'aquest treball va ser estudiar si el vector viral basat en potyvirus és capaç d'expressar una ruta biosintètica de múltiples passos en cèl·lules vegetals. Per açò ens vam proposar produir licopè, un pigment vegetal amb propietats beneficioses per a la salut humana. Per això inserírem un cDNA que codificaba els tres enzims de una ruta metabòlica de tres passos d'origen bacterià en el vector viral. Les plantes de tabac infectades amb el vector viral van desenvolupar símptomes de color taronja indicant l'acumulació de licopè, que va ser confirmat per anàlisi de cromatografia líquida d'alta eficàcia i observacions de microscòpia. Els nostres resultats també van il·lustrar que la sola expressió de fitoè sintasa de Pantonea ananatis, crtB, és suficient per a induir l'acumulació de carotenoides que confereixen una colora / Majer, E. (2016). Metabolic engineering of plants using a disarmed potyvirus vector [Tesis doctoral no publicada]. Universitat Politècnica de València. https://doi.org/10.4995/Thesis/10251/68477 / TESIS Tobacco etch virus Potyvirus genome organization Chimeric plant virus Subcellular targeting Metabolic engineering Secondary metabolite

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