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  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
141

Možnosti ovlivnění vývoje motoriky laboratorního potkana opakovaným podáváním specifického antagonisty NMDA receptoru / Possible influencing the motor performance of developing rats by repeated administration of the NMDA receptor antagonist specific for NR2 subunit

Kozlová, Lucie January 2016 (has links)
Nonspecific NMDA receptor antagonists induce hyperlocomotion in rats. The aim of this work is to determine whether the NMDA receptor antagonist specific for NR2 subunit exhibit similar negative effect as nonspecific antagonists. This subunit is predominant in the brain in the early postnatal period. The introduction summarizes the data on NMDA receptors and the development of rat. The experimental part deals with the action of a specific NMDA receptor antagonist Ro 25-6981 on motor performance of developing rats. Substance was repeatedly administered to rats at postnatal days 7 to 11. Spontaneous locomotion and motor performance of the animals were repeatedly tested up to adulthood by battery of tests appropriate for individual ages. Our research demonstrated that this substance does not have significant effect on motor system of laboratory rat and that it might be further tested as a possible age-bound antiepileptic drug.
142

Úloha N-terminální domény a/TIF32 podjednotky iniciačního faktoru eIF3 ve vazbě mRNA na 43S pre-iniciační komplexy. / The role of the N-terminal domain of the a/TIF32 subunit of eIF3 in mRNA recruitment to the 43S pre-initiation complexes.

Vlčková, Vladislava January 2013 (has links)
Translation initiation is a complex process which results in the assembly of the elongation competent 80S ribosome from the 40S and 60S ribosomal subunits, the initiator tRNA and mRNA, and is orchestrated by numerous eukaryotic initiation factors (eIFs). Although it represents one of the most regulated processes of gene expression, the exact mechanism of one of the key steps of translation initiation - mRNA recruitment to the 43S pre-initiation complex (PIC) - is still only poorly understood. Recent studies indicated that besides eIF4F and poly(A)-binding protein, also eIF3 might play an important, if not crucial, role in this step. In our laboratory, we recently identified a 10 Ala substitution (Box37) in the a/TIF32 subunit of Saccharomyces cerevisiae eIF3, which interfered with translation initiation rates. Detailed analysis showed that this mutation significantly reduces the amounts of model mRNA in the gradient fractions containing 48S PICs as the only detectable effect in vivo. Moreover, a recently solved crystal structure of the N-terminal part of a/TIF32 pointed to two Box37 residues, Arg363 and Lys364, both proposed to contribute to one of the positive, potentially RNA-binding areas on the a/TIF32 surface. The fact that also their substitutions with alanines severely impaired the mRNA recruitment...
143

Hledání potenciálního vazebného partnera glutamátkarboxypeptidasy II pomocí hmotnostní spektrometrie / Mass Spectrometry-Based Identification of a Potential Binding Partner of Glutamate Carboxypetidase II

Tužil, Jan January 2013 (has links)
English Abstract The incoming paradigm of the network (or systems) biology calls for a new high throughput tool for a wide scale study of protein-protein interactions. Mass spectrometry-based proteomics have experienced a great progress in recent years and have become an indispensable technology of elementary as well as clinical research. Glutamate carboxypeptidase II (GCPII; EC 3.5.17.21) is a transmembrane protein with two known enzymatic activities. Its expression is highly upregulated in some solid tumors and also in tumor-associated neovasculature in general. Nevertheless, none of the two enzymatic activities were shown to be physiologically relevant to these cells. Some facts point at a possible receptor function of GCPII, however, no specific binding partner has been found yet. In the search for potential binding partners and/or ligands of GCPII, a series of methods have been employed, including pull-down experiment, immunoprecipitation and mass spectrometry. Sample preparation and mass spectrometry data processing methodology was specifically developed in order to identify potential binding partners. As one of the outcome of that methodology, the interaction of β-subunit of F1 ATP synthase was selected for further detailed analysis as a putative ligand of GCPII.
144

Caracterização funcional e estrutural de peroxidases dependentes de tiól da bactéria fitopatogênica Xylella fastidiosa / Functional and structural characterization of thiol-dependent peroxidases from the phytopathogenic bacterium Xylella fastidiosa

Horta, Bruno Brasil 05 August 2009 (has links)
A bactéria fitopatogênica Xylella fastidiosa é o agente etiológico da Clorose Variegada dos Citros (CVC), que causa perdas anuais estimadas em US$ 100 milhões no Brasil. Durante o processo infeccioso, a geração extracelular de espécies ativas de oxigênio é um dos principais mecanismos de defesa da planta contra o patógeno. Em contrapartida, para se defender do estresse oxidativo imposto pelo hospedeiro, os fitopatógenos possuem mecanismos de defesa que incluem enzimas antioxidantes, como as peroxirredoxinas, alquil hidroperóxido redutase subunidade C (AhpC) e proteína comigratória com bacterioferritina (Bcp). As peroxirredoxinas são proteínas que utilizam suas cisteínas ativas para catalisar a redução de hidroperóxidos. Por análise proteômica, os produtos dos genes ahpc e bcp foram identificados no extrato celular protéico de X. fastidiosa (Smolka e col., 2003). Com o intuito de caracterizar funcional e estruturalmente as proteínas AhpC e Bcp de X. fastidiosa, clonamos e expressamos seus respectivos genes em Escherichia coli e purificamos as proteínas por cromatografia de afinidade a níquel. As proteínas recombinantes apresentaram atividade dependente de tiól de redução de peróxido de hidrogênio e hidroperóxidos orgânicos. A atividade peroxidase da AhpC e Bcp são dependentes, respectivamente, de alquil hidroperóxido redutase subunidade F (AhpF) e do sistema tiorredoxina. Paradoxalmente, a flavoproteína AhpF possui atividade NAD(P)H oxidase, que resulta na produção de peróxido de hidrogênio. As constantes de segunda ordem da reação das proteínas com peróxido de hidrogênio (da ordem de 107 M-1.s-1), determinadas pelo ensaio de cinética competitiva com peroxidase de raiz forte, indicam que ambas possuem atividades peroxidase equivalentes às apresentadas por glutationa peroxidases dependentes de selênio e catalases, ao contrário do descrito na literatura. Por SDS-PAGE não-redutor e pela quantificação de cisteínas livres por DTNB, verificamos que as proteínas possuem mecanismos catalíticos distintos: AhpC é uma 2-Cys Prx típica (com formação de ponte dissulfeto intermolecular), enquanto Bcp é uma 2-Cys Prx atípica (com formação de ponte dissulfeto intramolecular). Para AhpC, a atividade catalítica envolve as cisteínas conservadas (Cys-47 e Cys-165), em contraste, apenas através de estudos de mutação sítio-dirigida e espectrometria de massas conseguimos identificar os resíduos de cisteínas envolvidos na atividade catalítica da Bcp (Cys-47 e Cys-83). A caracterização estrutural de AhpC por cromatografia de exclusão molecular e espalhamento dinâmico de luz mostram que a proteína nativa é um decâmero estável, independentemente do estado de oxidação de suas cisteínas. A caracterização da estrutura cristalográfica de Bcp C47S, inédita para 2-Cys Prx atípicas que possuem as cisteínas ativas separadas por 35 aminoácidos, indica que a proteína possui o enovelamento característico das peroxirredoxinas e que as cisteínas ativas estão localizadas a uma distância média de 12,4 Å. Baseado em dicroísmo circular, apresentamos dados que indicam que a aproximação das cisteínas deve envolver um significativo rearranjo estrutural, que provavelmente se inicia com a formação do intermediário ácido sulfênico na cisteína peroxidásica (Cys-47). Assim, conseguimos elucidar o papel catalítico dessas proteínas, bem como identificar seus sistemas redutores, obtendo informações que podem ser relevantes para o entendimento do mecanismo da patogenicidade da X. fastidiosa. Os resultados apresentados neste trabalho podem contribuir para o desenvolvimento de novas técnicas de controle de praga para a doença CVC em citrus e outras que envolvam a bactéria X. fastidiosa. / The phytopathogenic bacterium Xylella fastidiosa is the etiological agent of Citrus Variegated Chlorosis (CVC) that causes losses of about 100 millions dollars per year in Brazil. During infection, reactive oxygen species play a central role in plant pathogen defense. To survive under oxidative stress imposed by the host, microorganisms express antioxidant proteins, including the peroxiredoxins alkyl hydroperoxide reductase subunit C (AhpC) and bacterioferritin comigratory protein (Bcp). Peroxiredoxins are peroxidases, which rely on an activated cysteine residue to catalyze the reduction of hydroperoxides. By proteome analysis, Smolka et al. (2003) identified the products of ahpc and bcp genes present in whole cell extract of X. fastidiosa. To characterize the function and structure of AhpC and Bcp protein, their genes were cloned in Escherichia coli and the corresponding proteins purified by nickel affinity chromatography. Recombinant proteins presented thiol-dependent peroxidase activity against hydrogen peroxide and organic hydroperoxides. AhpC and Bcp peroxidase activities are dependent on alkyl hydroperoxide reductase subunit F (AhpF), and on thioredoxin system, respectively. Paradoxically, AhpF flavoenzyme possesses hydrogen peroxide-forming oxidase activity. Contrary to classical assumptions, competitive kinetics employing horseradish peroxidase assays showed that the second-order rate constants of AhpC and Bcp reaction with hydrogen peroxide are in the order of 107 M-1.s-1, as fast as the activity of selenium-dependent glutathione peroxidases and catalases. Non-reducing SDS-PAGE and cysteine quantification using DTNB indicated different peroxidasic mechanisms: AhpC is a typical 2-Cys peroxiredoxin (with intermolecular disulfide bond formation), while Bcp is an atypical 2-Cys peroxiredoxin (with intramolecular disulfide bond formation). In contrast to the well-conserved AhpC cysteines responsible for the peroxidase activity (Cys-47 and Cys-165), only through site-specific mutagenesis and mass spectrometry we could identified the cysteine residues involved in the Bcp peroxidase activity (Cys-47 and Cys-83). Structural characterization by size exclusion chromatography and dynamic light scattering revealed that AhpC native protein forms stable and redox state independent decamers. The crystal structure of Bcp C47S, the first 2-Cys Prx with a 35-residue between the active cysteines ever characterized, shows that protein contains the common fold of peroxiredoxins and that active cysteines lies ~12.4 Å away one from the other. Based on circular dichroism, we presented data indicating that disulfide bond formation may require significant conformational changes, which probably is triggered by the peroxidatic cysteine oxidation to sulfenic acid. In conclusion, we elucidated the catalytic mechanisms and reduction systems of AhpC and Bcp proteins that may help to understand the pathogenicity mechanism of X. fastidiosa. These results can contribute to the development of plague control methods against X. fastidiosa.
145

Estudo da invasão trofoblástica na parede tubária em gestações ampulares: parâmetros associados e predição da profundidade / Study of trophoblastic invasion into the tubal wall in ampular pregnancies: associated parameters and its prediction

Cabar, Fabio Roberto 29 March 2006 (has links)
INTRODUÇÃO: A definição de fatores preditivos de lesão morfológica e funcional da tuba uterina poderia colaborar na escolha do tratamento de pacientes com gestação ectópica. O objetivo deste estudo foi verificar o comportamento do tecido trofoblástico em relação à sua penetração na parede da tuba uterina em gestações ampulares, relacionar a profundidade dessa penetração com idade gestacional, concentração de beta-hCG, tipo de imagem ultra-sonográfica e dimensão da massa ectópica à ultra-sonografia e avaliar a possibilidade de predição dessa invasão pelos parâmetros estudados. MÉTODOS: realizou-se estudo retrospectivo, entre 1° de janeiro de 2000 a 31 de março de 2004, com 105 pacientes com gestação tubária ampular submetidas à salpingectomia. As imagens ectópicas foram classificadas pelo aspecto ultra-sonográfico em anel tubário, massa complexa e embrião com atividade cardíaca e sua dimensão foi obtida pela medida do maior eixo. Histologicamente a invasão trofoblástica na parede tubária foi classificada em grau I: quando limitada à mucosa da tuba uterina; grau II: até a camada muscular; grau III: invasão de toda a espessura da tuba uterina. RESULTADOS: 29 pacientes tiveram infiltração tubária grau I, 30 pacientes infiltração grau II e 46 pacientes infiltração grau III. Os graus de invasão trofoblástica não estiveram associados à idade gestacional (p = 0,53) nem ao maior diâmetro da imagem à ultra-sonografia (p = 0,43). Os diferentes graus de invasão trofoblástica apresentaram diferença significativa da beta-hCG (p < 0,001). O grau I apresentou valores menores que os graus II e III (p < 0,05) e o grau II valores menores que o grau III (p < 0,05). Houve associação entre o grau de invasão trofoblástica e a descrição do tipo de imagem identificada à ultra-sonografia (p = 0,001). Embrião com atividade cardíaca foi mais prevalente nos casos de invasão grau III. O valor de 2 400 mUI/ml apresentou sensibilidade de 82,8%, especificidade de 85,5%, valor preditivo positivo de 68,6% e valor preditivo negativo de 92,7% (acurácia de 84,8%) para determinar invasão trofoblástica grau I. beta-hCG de 5 990 mUI/ml foi o melhor ponto de corte para predição de invasão trofoblástica grau III: sensibilidade de 82,6%, especificidade de 74,6%, valor preditivo positivo de 71,7% e valor preditivo negativo de 84,6% (acurácia de 78,1%). CONCLUSÕES: Em gestações ampulares, o tecido trofoblástico se desenvolve a partir de sua penetração na parede tubária, a profundidade da penetração do trofoblasto na tuba uterina relaciona-se às concentrações séricas de beta-hCG e ao tipo de imagem ultra-sonográfica, sendo que a concentração sérica da beta-hCG é a melhor preditora da profundidade da invasão na tuba uterina. / INTRODUCTION: The definition of predictive factors of morphologic and functional damage to the Fallopian tube may help in the choice of treatment for patients with ectopic pregnancy. The objective of the present study was to verify the presence of trophoblastic invasion into the tubal wall in ampular pregnancies, correlate the depth of penetration of trophoblastic tissue into the tubal wall with gestational age, beta-hCG concentration, type of ultrasonographic image and dimension of the ectopic mass upon ultrasound, and to evaluate the possible prediction of this invasion based on the parameters studied. METHODS: A retrospective study was conducted on 105 patients with ampular pregnancy submitted to salpingectomy between January 1, 2000 and March 31, 2004. Ectopic images were classified based on ultrasonographic findings in tubal ring, complex mass and embryonic heart activity. The dimension of the mass was determined by measuring the major axis. Histologically, trophoblastic invasion into the tubal wall was classified as grade I when limited to the tubal mucosa, grade II when reaching the muscle layer, and grade III when comprising the full thickness of the Fallopian tube. RESULTS: Twenty-nine patients had tubal infiltration grade I, 30 had grade II and 46 had grade III. The level of trophoblastic invasion was associated neither with gestational age (p = 0.53) nor with a greater diameter of the ultrasound image (p = 0.43). The different levels of trophoblastic invasion were significantly associated with beta-hCG concentration (p < 0.001), with lower concentrations being observed for grade I compared to grades II and III (p < 0.05) and for grade II compared to grade III (p < 0.05). There was an association between the level of trophoblastic invasion and the type of ultrasonographic image (p = 0.001). Embryos with heart activity were more prevalent in cases of grade III invasion. beta-hCG levels of 2 400 mIU/ml showed 82.8% sensitivity, 85.5% specificity, a positive predictive value of 68.6% and a negative predictive value of 92.7% (84.8% accuracy) for the diagnosis of grade I trophoblastic invasion. A beta-hCG titer of 5990 mIU/ml was the best cut-off for the prediction of grade III trophoblastic invasion: 82.6% sensitivity, 74.6% specificity, positive predictive value of 71.7% and negative predictive value of 84.6% (78.1% accuracy). CONCLUSIONS: trophoblastic tissue penetrate tubal wall in ampular pregnancies, the depth of penetration of trophoblastic tissue is correlated with beta-hCG concentration and type of ultrasonographic image and beta-hCG titer is the best predictor of the depth of penetration into tubal wall.
146

Caracterização físico-química da foliculotrofina humana (hFSH) recombinante e de suas subunidades, por cromatografia líquida de alta eficiência (HPLC) em fase reversa: comparação com a preparação de referência de hFSH de origem hipofisária do \"National Hormone and Pituitary Program\" dos EUA / Physico-chemical characterization of human recombinant follicle-stimulating hormone (hFSH) and its subunits by reversed-phase high-performance liquid chromatography (RP-HPLC): comparison with pituitary hFSH reference preparation from National Hormone and Pituitary Program from USA

Renan Fernandes Loureiro 06 November 2006 (has links)
Um método de cromatografia líquida de alta eficiência por fase reversa (RP-HPLC) para análise qualitativa e quantitativa do hormônio folículo estimulante humano íntegro (hFSH), foi estabelecido e validado quanto à exatidão, precisão e sensibilidade. O FSH humano é um hormônio glicoprotéico dimérico largamente utilizado em medicina reprodutiva tanto para diagnóstico quanto para terapia. A metodologia desenvolvida preserva a integridade da proteína, permitindo a análise da forma heterodimérica intacta, e não somente de suas subunidades, como é normalmente obtida na maioria das condições geralmente empregadas. Esta técnica foi também utilizada para a comparação da hidrofobicidade relativa de preparações de hFSH hipofisária, urinária e derivadas de células de ovário de hamster chinês (CHO) bem como de outros dois hormônios glicoprotéicos, sintetizados na hipófise anterior: hormônio humano estimulante da tireóide (hTSH) e hormônio luteinizante humano (hLH). O menos hidrofóbico dos três hormônios analisados foi o hFSH, seguido do hTSH e do hLH. Uma diferença significativa (p<0,005) foi observada entre o tempo de retenção (tR) das preparações hipofisária e recombinante de hFSH, refletindo diferenças estruturais nas suas cadeias de carboidratos. Duas isoformas principais foram detectadas no hFSH urinário, incluindo uma forma que foi significativamente diferente (p<0,005) das preparações hipofisária e recombinante. Foram demonstradas linearidade da curva dose-resposta (r=0,9965, n=15) para esta metodologia de RP-HPLC, bem como uma precisão inter-ensaio, cujo coeficiente de variação é menor que 4%, para a quantificação de diferentes preparações de hFSH e uma sensibilidade da ordem de 40 ng. Foram também analisados o comportamento cromatográfico e a hidrofobicidade relativa das subunidades individuais das preparações recombinantes e hipofisária de hFSH. Além disso, a exata massa molecular das subunidades individuais de hFSH e do heterodímero foram simultaneamente determinadas por espectrometria de massa MALDI-TOF. A presente metodologia representa, em nossa opinião, uma ferramenta essencial para a caracterização e controle de qualidade deste hormônio, que ainda não consta das principais farmacopéias. / A reversed-phase high-performance liquid chromatography (RP-HPLC) method for the qualitative and quantitative analysis of intact human follicle-stimulating hormone (hFSH) was established and validated for accuracy, precision and sensitivity. Human FSH is a dimeric glycoprotein hormone widely used as a diagnostic analyte and as therapeutic product in reproductive medicine. The technique developed preserves the protein integrity, allowing the analysis of the intact heterodimeric form rather than just of its subunits, as it is the case for the majority of the conditions currently employed. This methodology has also been employed for comparing the relative hydrophobicity of pituitary, urinary and two Chinese hamster ovary (CHO)-derived hFSH preparations, as well as of two other related glycoprotein hormones of the anterior pituitary: human thyroid-stimulating hormone (hTSH) and human luteinizing hormone (hLH). The least hydrophobic of the three glycohormones analyzed was hFSH, followed by hTSH and hLH. A significant difference (p<0.005) was observed in tR between the pituitary and recombinant hFSH preparations, reflecting structural differences in their carbohydrate moieties. Two main isoforms were detected in urinary hFSH, including a form which was significantly different (p<0.005) for the pituitary and recombinant preparations. The linearity of the dose-response curve (r = 0.9965, n = 15) for this RP-HPLC methodology, as well as an inter-assay precision with relative standard deviation less than 4% for the quantification of different hFSH preparations and a sensitivity of the order of 40 ng, were demonstrated. The chromatographic behavior and relative hydrophobicity of the individual subunits of the pituitary and recombinant preparations were also analyzed. Furthermore, the accurate molecular mass of the individual hFSH subunits and of the heterodimer were simultaneously determined by matrix-assisted laser desorption ionization time-of-flight mass spectral analysis (MALDI-TOF-MS). The present methodology represents, in our opinion, an essential tool for characterization and quality control of this hormone that is not yet described in the main pharmacopoeias.
147

Análise in vitro da capacidade de cobertura da vacina em desenvolvimento contra  Streptococcus pyogenes / \"in vitro\" analysis of the coverage capacity of the vaccine under development against most frequent strains of Streptococcus pyogenes

De Amicis, Karine Marafigo 08 May 2013 (has links)
O Streptococcus pyogenes (Grupo A de Lancefield) é uma bactéria Gram positiva e beta-hemolítica, responsável por infecções, tais como Faringite, Sepse, Fasciíte Necrotizante e Síndrome do Choque Tóxico Estreptocócico. Indivíduos suscetíveis podem desenvolver sequela não supurativa auto-imune pós-estreptocócica, como a Febre Reumática, Doença Reumática Cardíaca e a Glomerulonefrite Aguda. A proteína M é o principal antígeno bacteriano. Consiste em aproximadamente 450 resíduos de aminoácidos dispostos em quatro regiões (A, B, C e D), contendo alguns blocos de repetições. As regiões C e D são conservadas e a N-terminal (regiões A e B) é polimórfica. Atualmente, existem mais de 250 genótipos de emm conhecidos em todo o mundo, de acordo com o Centers for Disease Control and Prevention. Há vários anos, o desenvolvimento de uma vacina contra S. pyogenes (StreptInCor - identificação médica) foi iniciado, com base na região conservada da proteína M, com o objetivo de proteger o indivíduo vacinado contra infecções estreptocócicas, sem causar reações autoimunes. No presente estudo foi analisada a capacidade \"in vitro\" de anticorpos anti-StreptInCor neutralizarem/opsonizarem as cepas de S. pyogenes mais freqüentes em São Paulo, através da análise do reconhecimento das cepas por soros de camundongos imunizados com StreptInCor. Também foi avaliada por Western blotting a presença de anticorpos de reação cruzada dirigidos ao tecido cardíaco valvular humano. Anticorpos anti-StreptInCor foram capazes de neutralizar/opsonizar, pelo menos, cinco diferentes cepas mostrando que a imunização com StreptInCor pode ser eficaz contra várias cepas de S. pyogenes, assim como prevenir a infecção e sequelas subsequentes, sem causar reações auto-imunes. / Streptococcus pyogenes (Group A) is a Gram positive and beta-hemolytic bacteria, responsible for infections such as Pharyngitis, Sepsis, Necrotizing Fasciitis and Streptococcal Toxic Shock Syndrome. Susceptible individuals may develop post-streptococcal non-suppurative autoimmune sequelae such as Rheumatic Fever, Rheumatic Heart Disease and Acute Glomerulonephritis. The M protein is the major bacterial antigen. It consists of approximately 450 amino acid residues arranged in four regions (A, B, C and D), containing some repeated blocks. C and D regions are conserved and the N-terminus (regions A and B) is polymorphic. Currently there are over 250 known emm genotypes worldwide, according to the Centers for Disease Control and Prevention. Several years ago the development of a vaccine against S. pyogenes (StreptInCor - medical identification) was initiated, based on the M protein conserved region, aiming to protect against streptococcal infections without causing autoimmune reactions. In the present study we analyzed the \"in vitro\" ability of anti-StreptInCor antibodies to neutralize/opsonize the most frequent S. pyogenes strains in Sao Paulo by examining the strains recognition by sera from StreptInCor immunized mice. We also evaluated the presence of cross reactive antibodies directed to the human heart valve tissue by Western blotting. Anti-StreptInCor antibodies were able to neutralize/opsonize at least 5 strains, showing that the immunization with StreptInCor can be effective against several S. pyogenes strains as well as preventing infection and subsequent sequelae, without causing autoimmune reactions.
148

"Hipogonadismo hipogonadotrófico: diagnóstico pré-puberal e papel das isoformas e variantes gênicas do hormônio luteinizante no fenótipo da doença" / Hypogonadotropic hypogonadism : pre-pubertal diagnosis and the role of the isoforms and allelic variants of the luteinizing hormone in the disease phenotype

Berger, Karina 09 June 2006 (has links)
A resposta do LH e do FSH ao estímulo com GnRH, realizado em estádio pré-puberal em pacientes com hipopituitarismo acompanhados até a idade puberal, são úteis para predizer o diagnóstico da deficiência de gonadotrofinas, principalmente nas meninas. O estudo da região codificadora do gene LH em pacientes com hipogonadismo hipogonadotrófico e concentrações normais de LH revelou 5 variantes alélicas. A freqüência das variantes alélicas Arg8 e Thr15 foi similar entre hipogonádicos e adultos normais e a sua presença não interferiu nas concentrações séricas do LH. O estudo das isoformas do LH mostrou um predomínio das isoformas ácidas do LH em hipogonádicos e indivíduos normais, não permitindo atribuir à sua presença a baixa atividade biológica do LH imunorreativo encontrado em 13% dos hipogonádicos / LH and FSH responses to GnRH stimulation carried out in the pre-pubertal stage in patients with hypopituitarism followed until the pubertal stage are useful tools for predicting the gonadotropin deficiency diagnosis, especially in girls. The study of the codifying region of the LH gene in patients with hypogonadotropic hypogonadism and normal LH levels disclosed 5 allelic variants. The frequencies of the allelic variants Arg8 and Thr15 were similar between hypogonadic and normal adults, and their presence did not alter serum LH levels. The study of LH isoforms showed a predominance of acid LH isoforms in hypogonadic and normal subjects, which does not allow us to ascribe to their presence the low biological activity of the immunoreactive LH, found in 13% of the hypogonadic individuals
149

Análise citoarquitetônica e imunoistoquímica de estruturas do sistema visual de macacos-prego (Cebus apella) / Cytoarchitectural and immunohistochemical analysis of the visual system of tuffed capuchin (Cebus apella).

Frazão, Renata 11 June 2008 (has links)
O estudo do sistema visual de macacos-prego representa importante questão devido ao aspecto evolutivo que a espécie apresenta. Foram utilizados cinco macacos-prego, 2 kg. Foi efetuda injeção intra-ocular de 100 <font face=\"symbol\">ml de solução aquosa de toxina colérica subunidade B (CTb) a 1%, sendo a perfusão realizada 15 dias após a injeção intra-ocular. As retinas intactas e os encéfalos foram submetidos à procedimento de imunoistoquímica para análise. A caracterização da retina evidenciou dois tipos distintos de células bipolares, além disto, subunidades de receptores gabaérgicos co-localizam em retinas de macacos-prego, diferente dos resultados apresentados em outras espécies. As projeções retinianas foram observadas em todas as estruturas do sistema visual primário, óptico acéssório e de temporização circadiana, além de projeções para áreas adicionais. Os resultados evidenciam diferenças interespecíficas sugerindo que a extrapolação dos resultados adquiridos em diferentes espécies devam ser extrapolados com cautela. / The diurnal habits and its complex SNC, make the tufted capuchin monkey an important subject for the study of the visual system. In the present study, five tufted capuchins received a single intraocular neuronal tracer subunit B of cholera toxin (CTb) injection and perfused 15 days later. The retina and brain were removed from the animals and processed with immunohistochemical techniques. The CTb analysis showed that the retina send projections to several structures, such as primary visual, optical accessory and circadian control systems. The immunohistochemical characterization also showed two different types of bipolar cells in the retina. These cells, differently from other species, were co-localized with gabaergic receptors. Overall our results showed several interspecies differences suggesting that comparison of the visual system between species must be undertaken with great caution.
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Rôle du facteur d’initiation eIF3h dans la réinitiation de la traduction et dans la pathogénèse virale chez les plantes / The role of eukaryotic initiation factor eIF3h in translation reinitiation and viral pathogenesis

Makarian, Joelle 02 December 2016 (has links)
La réinitiation de la traduction est un mécanisme permettant de traduire des ORF qui sont présents dans la région leader de différents ARNm cellulaires (uORF). La majorité des cas de réinitiation de la traduction chez les eucaryotes concerne des uORF de petite taille. Des stratégies alternatives ont été développées, entre autres par les virus, afin de réinitier la traduction après un long uORF. Le virus de la mosaïque du chou-fleur (CaMV) exprime un ARNm polycistronique codant la totalité des protéines virales. L’une d’entre elle, la protéine TAV (TransActivateur/Viroplasmine) est un facteur essentiel qui rend possible la réinitiation de la traduction après de longs ORF et qui, de plus, active la protéine kinase TOR. La sous-unité h du facteur d’initiation de la traduction eIF3, requise pour promouvoir la reinitiation après un petit ORF chez les plantes, a été identifiée comme étant une nouvelle cible de phosphorylation de la voie de signalisation de TOR. L’objectif principal de ma thèse a été d’élucider la fonction de la protéine eIF3h dans la réinitiation après un petit ORF ainsi que dans la réinitiation de la traduction, assurée par TAV, après un long ORF. Nous avons exploité les lignées transgéniques eif3h-1 d’Arabidopsis exprimant la protéine eif3h tronquée de son extrémité C-terminale, qui sont déficientes pour la réinitiation mais pas pour l’initiation de la traduction. Nous avons montré que la phosphorylation de eIF3h est essentielle pour stabiliser eIF3 au niveau des ribosomes durant l’élongation, ce qui favorise la ré-acquisition par le ribosome de facteurs nécessaires à la réinitiation de la traduction, et que la délétion de sa région Ct abolit son intégration dans le complexe eIF3. De plus, nous avons montré que eIF3h, la cible de la voie de signalisation de TOR, interagit avec S6K1. Des protoplastes préparés à partir des plantes mutantes eif3h-1 sont incapables de promouvoir la réinitiation après de longs ORF en présence de TAV. La surexpression de eIF3h, indifféremment de son état de phosphorylation, est indispensable pour restaurer la reinitiation assurée par TAV dans les protoplastes eif3h-1. Par ailleurs, les plantes eif3h-1 déficientes dans la réinitiation, sont résistantes à l’infection par le CaMV démontrant l’importance de eIF3h pour la réplication du CaMV. En revanche, ces plantes eif3h-1 peuvent être infectées par d’autres virus dont la traduction de l’ARN génomique est coiffe- ou IRES-dépendante. Ainsi, nos résultats suggèrent que eIF3h est un facteur de reinitiation important aussi bien pour la reinitiation après un petit qu’après un long ORF (controlée par TAV), et que TAV exploite cette machinerie cellulaire, et plus particulièrement TOR et eIF3h, pour exprimer ses propres protéines par réinitiation de la traduction. / Translation of mRNAs that harbor upstream open reading frames (uORFs) within their leader regions operates via a reinitiation mechanism. In plants, reinitiation is up regulated by the target of rapamycin (TOR) signaling via phosphorylation of the subunit h of initiation factor 3 (eIF3). The eif3h-1 mutant expressing the C-terminally truncated eIF3h while maintaining high translation initiation efficiency is not active in reinitiation. Cauliflower mosaic virus (CaMV) pregenomic polycistronic RNA is translated via an exceptional mechanism of reinitiation after long ORF translation under control of CaMV protein TAV, which ensures activation of TOR. To find the link between underlying mechanisms, we examined eIF3h function in cellular and viral context. Here we show that eIF3h, if phosphorylated, has a role in recruitment of eIF3 into actively translating ribosomes that is a prerequisite for formation of reinitiation-competent ribosomal complexes. C-terminal truncation of eIF3h abolished its integration into the eIF3 complex and eIF3 loading on polysomes as manifested by the eIF3 core subunit c. We also show that eIF3h as a putative target of TOR/S6K1 binds S6K1 in vitro. eIF3h phosphorylation is not required for eIF3 complex formation. We demonstrated that eIF3h is essential for TAV to activate reinitiation after long ORF translation. Protoplasts derived from eif3h-1 mutant failed to support TAV function in reinitiation, which is restored only upon overexpression of recombinant eIF3h indifferent to its phosphorylation status. eif3h-1 mutant defective in reinitiation was found resistant to CaMV infection suggesting that eIF3h is critical for virus amplification. In contrast, viruses that evolve translation initiation dependent on either cap or the internal ribosome entry site infect reinitiation deficient mutant. Thus, we conclude that TAV exploits the basic cell reinitiation machinery, particularly TOR and eIF3h, to overcome cellular barriers to reinitiation after long ORF translation.

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