The TRC8 hereditary kidney cancer gene product is regulated by sterols and modulates SREBP levels /

Lee, Jason Philip.

January 2007

Thesis (Ph.D. in Human Medical Genetics) -- University of Colorado Denver, 2007. / Typescript. Includes bibliographical references (leaves 117-126). Free to UCD affiliates. Online version available via ProQuest Digital Dissertations;

Enhanced Liver X Receptor and Decreased Sterol Regulatory Element Binding Transcription Factor 2 Activities May Control Luteolysis of the Human Corpus Luteum

Xu, Yafei, Xu, Yafei

January 2017

The mechanisms causing luteolysis of the primate corpus luteum are unknown. There is an increase in expression of liver x receptor (LXR) target genes and reduced low density lipoprotein receptor (LDLR) during spontaneous luteolysis in primates. The LXRs belong to the nuclear receptor superfamily and increase cholesterol efflux by inducing transcription of their target genes. Uptake of cholesterol into primate luteal cells occurs primarily via LDL, and LDLR transcription is regulated by sterol regulatory element binding transcription factor 2 (SREBF2). Luteinizing hormone (LH) and human chorionic gonadotropin (hCG) maintain luteal function by binding to the LH/CG receptor (LHCGR), which stimulates progesterone (P4) synthesis via protein kinase A (PKA). It has also been previously reported that there is an increase in 27-hydroxycholesterol (27OH) concentrations during spontaneous luteolysis in primates. Pregnenolone and P4 inhibit the enzyme activity of CYP27A1 (cytochrome p450, family 27, subfamily A, polypeptide 1), which converts cholesterol into 27OH, an oxysterol that is a natural LXR agonist and SREBF2 inhibitor. Therefore, the overall hypothesis is that LXR-induced cholesterol efflux and reduced LDL uptake via inhibition of SREBF2 activity mediate luteolysis of the human CL. The objective of study 1 is to determine the effects of LXR activation and SREBF2 inhibition on P4 production, cholesterol metabolism and gene expression; and how hCG signaling via PKA regulates these effects in human luteinized granulosa cells. Basal and hCG-stimulated P4 secretion were significantly decreased by the combined actions of the LXR agonist T0901317 (T09) and the SREBF2 inhibitor fatostatin, which was associated with alterations in cholesterol metabolism leading to reduced intracellular cholesterol storage. Expression of LXR target genes in the presence of T09 was significantly reduced by hCG, while hCG significantly increased LDLR expression. These effects of hCG were reversed by a specific PKA inhibitor. Chronic hCG exposure had similar effects on LXR target gene and LDLR expression without an exogenous LXR agonist. The objective of study 2 is to determine the effects of 27OH on P4 production and cholesterol metabolism; and to determine if inhibiting the conversion of cholesterol into pregnenolone increases LXR and decreases SREBF2 target gene expression via CYP27A1 in human luteinized granulosa cells. During luteolysis in primates and sheep, CYP27A1 expression significantly increased. 27OH significantly decreased hCG-stimulated P4 secretion and enhanced cholesterol efflux. Aminoglutethimide, which inhibits the conversion of cholesterol to pregnenolone, significantly increased ABCA1 and decreased LDLR. Knock-down of CYP27A1 resulted in a significant increase in P4 secretion, but did not prevent aminoglutethimide-induced effects on ABCA1 and LDLR. Knock-down of steroidogenic acute regulatory protein (STAR), which controls cholesterol transport into the mitochondria where CYP27A1 resides, significantly decreased LDLR transcription. Collectively, the data from study 1 support the hypothesis that LXR-induced cholesterol efflux and reduced LDL uptake via inhibition of SREBF2 activity mediates luteolysis in primates, which is reversed by hCG. Data from study 2 indicates that 27OH produced via CYP27A1 may contribute to reductions in P4 synthesis during luteolysis, partially by serving as a dual LXR agonist and SREBF2 inhibitor, although other oxysterols are also likely involved.

27-hydroxycholestrol

human chorionic gonadotropin

Human luteinized granulosa cells

Liver x receptor

Luteolysis

Changes in Lipid Distribution During Aging and Its Modulation by Calorie Restriction

Kim, Ji Y., Kim, Dae Hyun, Choi, Jaehun, Park, Jin K., Jeong, Kyu Shik, Leeuwenburgh, Christiaan, Yu, Byung Pal, Chung, Hae Young

01 June 2009

Adipogenesis and ectopic lipid accumulation during aging have a great impact on the aging process and the pathogenesis of chronic diseases with age. However, at present, information on the age-related molecular changes in lipid redistribution patterns and their potential nutritional interventions is sparse. We investigated the mechanism underlying age-related lipid redistribution and its modulation using 5-, 17-, and 24-month-old male Fischer 344 rats fed ad libitum (AL) or a 3-week-long CR (40% less than AL) diet. Results revealed that the activities of adipogenic transcription factors were decreased in the white adipose tissue (WAT) of aged AL rats. In contrast, the skeletal muscle of aged AL rats showed increased fat accumulation through decreased carnitine palmitoyltransferase-1 activity, which was blunted by short-term CR. This study suggests an age-related shift in lipid distribution by reducing the adipogenesis of WAT while increasing intramyocellular lipid accumulation, and that CR can modulate age-related adipogenesis and ectopic lipid accumulation.

aging

calorie restriction

lipid accumulation

skeletal muscle

KGF Induces Lipogenic Genes Through a PI3K and JNK/SREBP-1 Pathway in H292 Cells

Chang, Yongsheng, Wang, Jieru, Lu, Xiaojun, Thewke, Douglas P., Mason, Robert J.

01 December 2005

Lipid synthesis is required for cell growth and is subject to pharmacologic regulation. Keratinocyte growth factor (KGF) stimulates proliferation and lipogenesis in H292 cells, a pulmonary epithelial cancer cell line, but the signaling pathways are not known. KGF stimulated the expression of the transcription factors sterol-regulatory element binding protein-1 (SREBP-1), CCAAT/enhancer binding protein α (C/EBPα), and C/EBPδ and two key enzymes involved in lipogenesis, FAS and stearoyl coenzyme A desaturase-1 (SCD-1). We found that KGF induced rapid activation of Akt, p70 S6K, JNK, and extracellular signal-regulated (ERK). Induction of SREBP-1, SCD-1, and FAS by KGF was inhibited by the JNK inhibitor SP600125 and the phosphatidylinositol 3-kinase (PI3K) inhibitor LY294002 but not by the ERK inhibitor PD98059. Using FAS and SCD-1-luciferase promoter constructs, we observed that KGF stimulated the transcription of these promoters and that exogenous cholesterol inhibited the induction. Mutation of the SREBP-1 binding site in the SCD-1 promoter abolished the effect of KGF on SCD-1 transcription. In addition, overexpression of active SREBP-1 directly stimulated SCD-1 and FAS. Conversely, adenovirus-mediated overexpression of a dominant negative form of SREBP-1 inhibited the KGF effect on FAS and SCD-1 expression. In summary, we conclude that KGF requires both PI3K and JNK signaling pathways to induce SREBP-1, which in turn induces SCD-1 and FAS expression in H292 cells.

H292 cells

keratinocyte growth factor

lipogenesis

lung cancer

phosphatidylinositol 3-kinase

Biomedical Sciences

Role of fungal ARV-1 protein in sterol metabolism and pathogenicity of the chestnut blight fungus Cryphonectria parasitica

Kundu, Soumyadip

12 May 2023

Intracellular sterol redistribution is an important step in the lipid homeostasis of organisms, a process directly linked to the organizational arrangement in the plasma membrane (PM) of cells. Previous studies in the budding yeast Saccharomyces cerevisiae have demonstrated that the ARV1 (ACAT-related enzyme-2 required for viability 1) protein is a major regulator of sterol transport from the endoplasmic reticulum to the plasma membrane, contributing to the structural organization of the PM, rendering it resistant to anti-fungal compounds as well as maintaining ER integrity. This study assessed the significance of ARV1 in the plant pathogenic fungus Cryphonectria parasitica (Cparv1) and investigated its role in the pathogenesis and virulence of the fungus. C. parasitica is the causative agent of Chestnut blight, which has wreaked havoc on the American chestnut species. Genomic analysis revealed that the Cparv1 gene is very closely linked to another gene that putatively encodes a cyanamide hydratase (Cpcah). An initial gene deletion event resulted in the elimination of both genes and a highly deformed phenotype in C. parasitica that was fully recoverable by complementation. PCR-based expression analysis determined that the lack of Cparv1 was responsible for the debilitated phenotype of the double mutant, with no transcript detectable from Cpcah. Subsequent complementation of the Cparv1 gene was also observed to restore the wildtype phenotype. Mass spectrometry-based (MS) results indicated a decrease in sterol content of the DCparv1 mutant strain compared to wildtype EP155 thus confirming a role for Cparv1 in sterol homeostasis. It has been shown that infection of C. parasitica with virulence-attenuating hypoviruses altered intracellular lipid content and protein secretion. Ultrastructure studies conducted on the Cparv1 strain showed disrupted organelle integrity and the presence of cytoplasmic double membrane stretches. Decreased sterol content in C. parasitica infected with CHV1-EP713 was observed similar to DCparv1 suggesting a connection between the hypovirus-infected phenotype and Cparv1. Furthermore, a non-targeted metabolomic study on all three strains identified 324 metabolites. Through the subsequent pathway analysis, we have investigated the pleiotropic effects in the C. parasitica strains and established a mechanistic linkage between this the activity of the ARV-1 protein and the hypovirus-infected phenotype.

Fungus

Chestnut

Metabolomics

Sterol redistribution

Ergosterol

ARV-1

Single-ion monitoring

Hypovirulence

Non-targeted metabolomics

Pathway analysis

Biology

Sensibilidade a fungicidas e adaptabilidade de Lasiodiplodia theobromae patogênico ao mamão

PEREIRA, Alba Valéria da Silva

16 March 2009

Submitted by (lucia.rodrigues@ufrpe.br) on 2017-02-16T14:00:28Z No. of bitstreams: 1 Alba Valeria da Silva Pereira.pdf: 458155 bytes, checksum: 80e5a16e6ef2e1ee3b97cac4fbc53703 (MD5) / Made available in DSpace on 2017-02-16T14:00:28Z (GMT). No. of bitstreams: 1 Alba Valeria da Silva Pereira.pdf: 458155 bytes, checksum: 80e5a16e6ef2e1ee3b97cac4fbc53703 (MD5) Previous issue date: 2009-03-16 / Conselho Nacional de Pesquisa e Desenvolvimento Científico e Tecnológico - CNPq / Application of fungicide is the main measure of management to stem-end rot and there is no information on the sensitivity and on the fitness costs arising from the reduction in sensitivity of its causal agent, Lasiodiplodia theobromae. One hundred and twenty monosporic isolates collected in producing areas of the Northeast region of Brazil, were divided into six populations. We evaluated the in vitro sensitivity (inhibition of mycelial growth) of the isolates to class the fungicides belonging to two groups: benzimidazoles and sterol demethylation inhibitors (DMIs). We also evaluated the fitness of isolates with different levels of sensitivity the fungicides both in vitro and in vivo (mycelial growth and aggressiveness). The average EC50 for DMIs ranged from 0,141 to 4,054, 0,045 to 0,691 and from 0,001 to 1,529 for tebuconazole, prochloraz and imazalil, respectively. The level of sensitivity to DMIs did not differ among populations. For the benzimidazoles EC50 of 91.6% of the isolates ranged from 0,002 to 0,14 and 0,36 in 1,272 (benomyl and thiabendazole,respectively).The 8.4% isolates, classified as not sensitive (NS) were not inhibited at the highest concentration evaluated (100μg ml of a.i-1). All NS isolates were from the same population. The aggressiveness of NS isolated was lower. / A aplicação de fungicida é a principal medida de manejo para podridão peduncular e não há informações sobre a sensibilidade e custos adaptativos decorrentes da redução de sensibilidade do seu agente causal, Lasiodiplodia theobromae. Cento e vinte isolados monospóricos, coletados em áreas produtoras da região Nordeste do Brasil, foram divididos em seis populações. Avaliou-se a sensibilidade in vitro (inibição de crescimento micelial) dos isolados aos fungicidas das classes dos benzimidazois e inibidores da biossíntese de ergosterol (IBEs) e a adaptabilidade in vitro e in vivo (crescimento micelial e agressividade) de isolados com níveis distintos de sensibilidade aos fungicidas testados. A CE50 média para os IBEs variou de 0,141 a 4,054, 0,045 a 0,691 e 0,001 a 1,529 para o tebuconazol, prochloraz e imazalil, respectivamente. O nível de sensibilidade aos IBEs não diferiu entre populações. Para os benzimidazóis a CE50 de 91,6% dos isolados variou de 0,002 a 0,14 e 0,36 a 1,272(benomyl e tiabendazol, respectivamente). Os 8,4%, classificados como não sensíveis (NS), não foram inibidos na maior concentração avaliada (100μg de i.a. ml-1). Todos os isolados NS foram oriundos de uma mesma população. A agressividade dos isolados NS foi menor. Para os IBEs, não foi detectado nenhum custo adaptativo.

Carica papaya

Podridao peduncular

Resistência

Inibidores da biossíntese ergosterol

Benzimidazóis

Resistance

Sterol demethylation inhibitors

Benzimidazoles

Stem-end rot

Mamão

Fitopatologia

FITOSSANIDADE::FITOPATOLOGIA

Mapeamento de proteínas alvo para novos antifúngicos na fração microssomal e citosólica do patógeno humano Aspergillus fumigatus / Mapping target proteins for new antifungals in the microsomal and cytosolic fraction of the human pathogen Aspergillus fumigatus

Ivy Ortega Medeiros Zanon da Silva

21 March 2013

Coordenação de Aperfeiçoamento de Pessoal de Nível Superior / A incidência de infecções fúngicas invasivas vem aumentando nos últimos anos. Estas infecções, em geral, apresentam altas taxas de mortalidade. A profilaxia com antifúngicos ainda é a estratégia mais comum na contenção da mortalidade e prevenção contra infecções fúngicas invasivas, porém, apresenta baixa eficiência, e relatos de resistência às drogas. Além disso, a terapia antifúngica é limitada a um pequeno grupo de drogas, como os polienos, azóis e equinocandinas. Desta forma, a busca de novos alvos de drogas é fundamental para o desenvolvimento de novos antifúngicos. Estudos in silico indicaram quatro genes como potenciais alvo de drogas em fungos patogênicos. Neste contexto, o objetivo deste trabalho foi verificar a expressão das proteínas codificadas por dois destes possíveis genes alvo, a proteína erg6, na fração microssomal, e trr1, na fração citosólica, em hifas de A. fumigatus. Visando alcançar este objetivo, foram primeiramente padronizadas todas as etapas de fracionamento celular visando isolar estas duas subfrações celulares de A. fumigatus. Posteriormente, foi otimizado o protocolo de extração e reidratação de proteínas microssomais bem como reidratação de proteínas citosólicas. Estes extratos foram submetidos a diferentes protocolos de fracionamento proteico em um sistema de eletroforese OFFGEL (OGE). Os resultados de Western immunoblot mostraram que estas duas proteínas, erg6 e trr1, são de fato expressas na fase filamentosa de A. fumigatus. O extrato proteico da fração microssomal submetido ao OGE em doze subfrações apresentou três subunidades da proteína erg6, reconhecidas pelo anticorpo monoclonal, com massas moleculares e pI distintos: uma subunidade de aproximadamente 79 kDa com pI entre 5,91 e 6,49, e outras duas subunidades de aproximadamente 35 kDa e 32 kDa, ambas com pI entre 6,49 e 7,08. A enzima erg6 foi descrita como um homotetrâmero em outros fungos. Porém, nossos resultados sugerem que, em A. fumigatus, a erg6 possui uma estrutura heterotetramérica. Quanto à proteína trr1, tanto no extrato total quanto nas frações resultantes do fracionamento em OGE, uma banda única de aproximadamente 40 kDa, com pI na faixa de 4,79 e 5,33, foi reconhecida pelo anticorpo policlonal. Desta forma, esta proteína parece ter uma estrutura homodimérica, assim como descrito em outros micro-organismos. / The invasive fungal infections incidence has increased in recent years. These infections usually presents high mortality rates. Antifungal prophylaxis remains the most common clinical strategy to decrease mortality and prevent invasive fungal infections, however, it has low efficiency and drug resistance reports. Furthermore, antifungal therapy is limited to a small group of drugs such as polyenes, azoles, and echinocandins. Thus, the search for new drug targets is imperative for the new antifungal agents development. In silico studies have indicated four genes as potential drug target in pathogenic fungi. In this context, our aim was to investigate the expression of two proteins encoded by two putative target genes, erg6 in the microsomal fraction, and trr1 in the cytosolic fraction of A. fumigatus hyphae. To achieve this goal, we first standardized all steps of cell fractionation to isolate these two fractions of A. fumigatus hyphae. Subsequently, was optimized the protein extraction and rehidratation protocols of these two subfractions, such as cytosolic proteins rehidratation. These extracts were submitted to different protocols for protein fractionation in an OFFGEL electrophoresis system (OGE). The Western immunoblot results showed that these two proteins, erg6 and trr1, are expressed in filamentous phase of A. fumigatus. The microsomal protein extract submitted to the OGE in twelve fractions, showed three erg6 protein subunits recognized by monoclonal antibody, with distincts molecular weight and pI: a subunit with approximately 79 kDa, with pI in the range of 5,91 and 6,49, and others two subunits with 35 kDa and 32 kDa, both with pI between 6,49 and 7,08. The enzyme erg6 was described as a homotetramer in other fungi, however, our results suggest that in A. fumigatus the erg6 has a heterotetrameric structure. Regarding trr1 protein, in both, total and fractionated (OGE) extracts, a single band of approximately 40 kDa, with pI in the range of 4.79 and 5.33, was recognized by the polyclonal antibody, suggesting that this protein appears to have a homodimeric structure, as described in other microorganisms.

Aspergillus fumigatus

Microssoma

Citosol

Eletroforese OFFGEL

Esterol-c-24-metiltransferase

Tioredoxina redutase

Aspergillus fumigatus

Microsome

Cytosol

OFFGEL electrophoresis

Sterol-c-24-methyltransferase

Tioredoxin reductase

MICOLOGIA

Determinação da origem da matéria orgânica sedimentar através de marcadores moleculares lipídeos (alcoóis lineares e esteróis) no sistema lacunar Mundaú- Manguaba –AL

Ribeiro, Maria Antônia Tinoco Santos Branco

13 September 2017

Submitted by Biblioteca de Pós-Graduação em Geoquímica BGQ (bgq@ndc.uff.br) on 2017-09-13T16:47:10Z No. of bitstreams: 1 Dissertação Maria Antonia.pdf: 1558722 bytes, checksum: 45d44953fdc50328a4c365482547773f (MD5) / Made available in DSpace on 2017-09-13T16:47:10Z (GMT). No. of bitstreams: 1 Dissertação Maria Antonia.pdf: 1558722 bytes, checksum: 45d44953fdc50328a4c365482547773f (MD5) / Universidade Federal Fluminense. Instituto de Química. Programa de Pós-Graduação em Geoquímica, Niterói, RJ / O sistema estuarino-lagunar Mundaú Manguaba é um ecossistema costeiro tropical raso, localizado nas margens da cidade de Maceió, nordeste do Brasil, que sofre impactos antropogênicos provenientes principalmente da urbanização e ocupação de suas margens, do cultivo extensivo da cana-de-açúcar e do despejo de esgoto sanitário e rejeitos industriais, que fertilizam suas águas. Nesse contexto, este trabalho teve como objetivo avaliar a origem e o comportamento da matéria orgânica sedimentar do sistema, e, em última instância, o seu grau de contaminação fecal. Para tal, foram quantificados marcadores moleculares orgânicos (álcoois lineares e esteróis) por cromatografia gasosa acoplada a espectrometria de massa (CG/EM), juntamente com diversos parâmetros físico-químicos e orgânicos do sedimento (granulometria, teor de matéria orgânica, C, N, entre outros) em amostras coletadas ao longo do eixo longitudinal das lagoas Mundaú e Manguaba, das fontes fluviais (rios Mundaú, Sumaúma e Paraíba do Meio), em uma amostra de solo e nos canais de ligação com o mar. A distribuição dos compostos analisados mostrou que a matéria orgânica sedimentar das lagoas tem origem essencialmente da sua própria produção primária fitoplantônica. Nas fontes fluviais e próximo a suas desembocaduras há uma influência da matéria orgânica terrígena, acarretando em uma mistura entre a matéria orgânica autóctone e alóctone. Os álcoois lineares de cadeia longa se mostraram ferramentas eficientes para avaliar a influência terrestre, o que não pode ser afirmado para os esteróis. Estes últimos foram mais eficazes para determinar o grau de contribuição da matéria orgânica fecal, que foi considerável próximo à cidade de Maceió (4,4 μg de coprostanol por grama de sedimento seco), e suas razões (estanol/estenol) puderam evidenciar as transformações diagenéticas da matéria orgânica, especialmente a autóctone. A região dos canais apresentou teores insignificantes para todos os marcadores moleculares, provavelmente em função de sua maior hidrodinâmica que favorece a predominância de material mais grosso (areias), em detrimento da deposição de finos, ao qual geralmente a matéria orgânica está preferencialmente associada. / Mundaú- Manguaba is a tropical, shallow coastal lagoon system, located at Maceió, the capital of Alagoas, northeast Brazil. This ecosystem suffers anthropogenic impacts originating mainly from urbanization and occupation of its margins, the extensive sugar-cane monoculture and the dispoasal of sludge and industrial waste, which fertilize its waters. The aim of this study is to evaluates the origin and the behaviour of the sedimentary organic matter, and also its degree of faecal contamination. Organic molecular markers (fatty alcohols and sterols), together with physical and organic bulk parameters (grain size, organic matter, C, N, and others) were quantified on sediment samples of the Mundaú and Manguaba lagoons, its fluvial sources (Mundaú, Sumaúma and Paraíba do Meio Rivers), a soil sample and on the channels connecting to the sea. The distribution of those compounds showed that the sedimentary organic matter of the lagoons originates essentially from its phytoplankton primary production. Fluvial sources and river mouths are both influenced by terrigenous materials, with a mix of authoctonous and allochtonous organic compounds. The long chain fatty alcohols served as efficient tools to evaluate the terrestrial influence. In contrast, the sterols were more efficient to determine the amount of faecal contribution close to Maceió´s waste disposal, with coprostanol attaining 4,4 μg/g of dry weight. Moreover, stanol/sterol ratios evidenced the early diagenesis of organic materials, specially those of autochthonous origin. The channel system presented low organic matter contents devoid of significant concentrations of the molecular markers, due to stronger advective exchange within the channels, favouring the predominance of sandy materials, rather than fine grained sediments, the last generally are associated to organic matter.

Mundaú Manguaba

Marcadores Moleculares

Alcoóis Lineares

Esteróis

Mundaú Manguaba

Marcadores Moleculares

Alcoóis Lineares

Esteróis

Produção intelectual

Mundaú Manguaba

molecular markers

fatty alcohol

sterol

Constru??o de um modelo de previs?o de atividade para o planejamento e s?ntese de triaz?is promissores para inibi??o dda CYP51 do Trypanosoma cruzi / Construction of a theorical model for prediction of activity for the design and synthesis of promising triazoles as inhibitors of Trypanosoma cruzi CYP51

CASTRO, Larissa Henriques Evangelista

02 December 2016

Submitted by Jorge Silva (jorgelmsilva@ufrrj.br) on 2017-09-12T18:24:02Z No. of bitstreams: 1 2016 - Larissa Henriques Evangelista Castro.pdf: 3738174 bytes, checksum: 04e651a55fa9b4054c2810389592be67 (MD5) / Made available in DSpace on 2017-09-12T18:24:02Z (GMT). No. of bitstreams: 1 2016 - Larissa Henriques Evangelista Castro.pdf: 3738174 bytes, checksum: 04e651a55fa9b4054c2810389592be67 (MD5) Previous issue date: 2016-12-02 / CAPES / CNPq / FAPERJ / Trypanosoma cruzi is the parasite that causes american trypanosomiasis (or Chagas disease), a neglected tropical disease previously restricted to South and Central Americas and Mexico, but now with several cases around the world. Currently in Brazil, the treatment of Chagas disease is done, only using benznidazole, which is not effective for the disease?s chronic phase and causes aggressive side effects, which explains the necessity of researches to find novel anti-Chagas compounds. A strategy adopted for the development of bioactive compounds against T. cruzi consists on the inhibition of the sterol 14?-demethylase enzyme (CYP51), which is essential for the parasite?s cellular membrane integrity. The inhibition can be achieved by a complexation of heterocyclic ring-containing compounds with the iron atom of heme group, present on CYP51. Thus, molecular modeling techniques were used on this study to analyze the interaction of a heterocyclic compounds (with known activity) with T. cruzi CYP51 in order to obtain the necessary information to construct an effective model for the theoretical activity prediction of these and also novel compounds. The proposed model presented a good multiple correlation coefficient (r? = 0.84) with the terms used to its construction. The model was used to help the design of novel piperine derivatives with a triazole ring, that presented promising theorical activities against T. cruzi CYP51, calculated by the model. The most promising compounds were selected and synthesized with the purpose of being tested in vitro and in vivo against T. cruzi. / O Trypanosoma cruzi ? o parasito causador da tripanossom?ase americana (Doen?a de Chagas), uma doen?a tropical negligenciada antes restrita ? Am?rica do Sul, Am?rica Central e M?xico, mas que vem apresentando um n?mero cada vez maior de casos no mundo. Atualmente, o tratamento da Doen?a de Chagas no Brasil ? limitado ao uso do f?rmaco benzonidazol, que ? pouco eficaz para a fase cr?nica da doen?a e causa efeitos colaterais agressivos, o que torna a pesquisa por novos f?rmacos imprescind?vel. Uma estrat?gia adotada para o desenvolvimento de compostos bioativos contra T. cruzi consiste na inibi??o de uma enzima essencial para a integridade da membrana celular do parasito, a enzima esterol 14?-desmetilase (CYP51), causada pela coordena??o de compostos contendo an?is heteroc?clicos com o ?tomo de ferro do grupo heme presente na enzima, fundamental para a atividade. Dessa maneira, foram utilizadas nesse estudo t?cnicas de modelagem molecular, incluindo docagem molecular e c?lculos qu?nticos semi-emp?ricos, para analisar a intera??o de uma s?rie de compostos heteroc?clicos de atividade conhecida sobre a CYP51 do T. cruzi e com isso se obter informa??es necess?rias para a constru??o de um modelo efetivo para a previs?o te?rica da atividade destes compostos. O modelo proposto apresentou um bom coeficiente de correla??o m?ltipla com os termos utilizados para sua constru??o, com um r?=0,84. Esse modelo foi utilizado para o planejamento de novos triaz?is derivados da piperina, com atividade te?rica calculada promissora contra a CYP51 de T. cruzi. Alguns dos melhores compostos foram selecionados e sintetizados neste projeto, com a proposta de serem avaliados em testes in vitro e in vivo contra a doen?a de Chagas.

Chagas disease

docking

sterol 14alfa-demethylase

triazolic compounds

Doen?a de Chagas

docagem

m?todo semi-emp?rico

esterol 14alfa-desmetilase

compostos triaz?licos

semi-empirical

Qu?mica Org?nica

Mécanismes du transport lipidique par les protéines ORP/Osh / Mechanisms of lipid transport by the ORP/Osh proteins

Moser von Filseck, Joachim

16 December 2014

Une distribution lipidique hétérogène est essentielle à l’identité et fonction des organelles, mais l’échange par trafic vésiculaire tend à annuler cette distribution. Il existe donc des mécanismes qui assurent l’homéostasie des lipides. Les protéines Osh (S. cerevisiae) et les OSBP-Related Proteins (ORP, H. sapiens), sont des transporteurs de lipides. Osh4 est capable d’échanger de l’ergostérol contre le phosphatidylinositol-4-phosphate (PI4P), présent sur l’appareil de Golgi. Utilisant des outils fluorescents mesurant avec une précision inégalée le transport de stérol et de PI4P, nous démontrons qu’Osh4 transporte du stérol contre son gradient de concentration en utilisant l’énergie d’un gradient de PI4P. Un couplage au métabolisme du PI4P permettrait à Osh4 d’alimenter le Golgi avec du stérol, ainsi créant le gradient de stérol entre ces organelles. La protéine OSBP participe, via sa capacité à connecter la membrane du RE à celle du trans-Golgi, à la création de jonctions entre ces organelles. Nous avons montré qu’OSBP, par échange stérol/PI4P, utilise le PI4P pour transférer du cholestérol au Golgi, mais également pour autoréguler sa capacité à former les jonctions. Osh6 lie la phosphatidylsérine, nous permettant d’étudier un nouveau mécanisme d’échange. Nous avons résolu la structure cristallographique d’un complexe Osh6/PI4P et avons pu observer l’échange de ces deux ligands par Osh6 entre deux membranes. Cette étude nous permet de suggérer que l’échange de PI4P avec divers lipides, via les protéines Osh/ORP, serait un mécanisme général permettant aux cellules de maintenir le gradient lipidique entre le RE et les membranes tardives de la voie sécrétoire. / An uneven lipid distribution is essential for the function of eukaryotic organelles. However, exchange of material by vesicular trafficking has a tendency to perturb this distribution; mechanisms must though exist to ensure lipid homeostasis. Osh proteins (S. cerevisiae) and OSBP-Related Proteins (ORPs, H. sapiens), are lipid transfer proteins (LTPs). Osh4 is capable of exchanging ergosterol for phosphatidylinositol 4-phosphate (PI4P), found on the Golgi. Using novel fluorescent tools to measure with unprecedented precision the transport of sterol and PI4P, we find that Osh4 can transport sterol against its concentration gradient using the energy of a PI4P gradient. Coupled to phosphoinositide metabolism, this allows Osh4 to transport sterol to the trans-Golgi and create the sterol gradients observed between these organelles. OSBP participates in the creation of membrane contact sites (MCSs) via its capacity to connect ER membranes to those of the trans-Golgi. We have shown that it uses PI4P for transporting cholesterol from the ER to the trans-Golgi by sterol/PI4P counterexchange, hence also autoregulating its tethering activity. Finally, the identification of phosphatidylserine as a ligand for Osh6 allowed us to analyze the possible extrapolation of the PI4P counterexchange mechanism. We have solved the crystal structure of Osh6 in complex with PI4P and have been able to follow counterexchange of PI(4)P and PS in vitro. Concluding, our studies allow us to suggest a general mechanism for ORP/Osh-mediated counterexchange of PI4P for other lipids to maintain lipid gradients between the ER and late membranes of the secretory pathway.

Protéines de transfert lipidique

Protéines Osh

OSBP

Stérol

Phosphatidylinositol-4-phosphate

Phosphatidylsérine

Lipid transfer protein

Osh proteins

OSBP

OSBP-related proteins

Sterol

Phosphatidylinositol 4-phosphate

Phosphatidylserine