Global ETD Search

91	Formulation, characterisation and topical application of oil powders from whey protein stabilised emulsions / Magdalena Kotze Kotze, Magdalena January 2014 (has links) The available literature indicates that to date, few research has been performed on oil powders for topical delivery. The aim of this project was to investigate the release characteristics of oil powder formulations, as well as their dermal and transdermal delivery properties. Whey protein-stabilised emulsions were used to develop oil powders. Whey protein was used alone, or in combination with chitosan or carrageenan. Nine oil powders, with salicylic acid as the active ingredient, were formulated by using the layer-by-layer method. Three different pH values (pH 4, 5 and 6) were used to prepare the formulations, because of the different charges that polymeric emulsifiers may have. The characteristics of the prepared oil powders were determined, including their droplet sizes, particle size distributions, loss on drying, encapsulation efficiencies, oil leakage and water dispersibility. Release studies (membrane diffusion studies) were conducted by utilising cellulose acetate membranes (0.2 μm pore size) and Franz-type diffusion cells over a period of eight hours. The release of the active ingredient was determined for all nine powders, their respective template emulsions, as well as their respective oil powders redispersed in water. The release of salicylic acid from the respective redispersed oil powders was then further compared to its release from the template emulsions and from the oil powders. The effect of pH and different polymer types used in preparing the oil powders, their respective redispersed oil powders and the template emulsions were determined with regards to the release of the active ingredient from all these preparations. The effect of pH and different polymers used was furthermore determined on the oil powders and their respective redispersed oil powders, with regards to their dermal and transdermal deliveries. Transdermal delivery and skin uptake were investigated on specifically selected powders only, based on the outcomes of the oil powder characterisation and release data. The qualifying formulations were chitosan pH 4, 5 and 6, whey and carrageenan pH 6 oil powders, together with their respective redispersed oil powders in water. Human abdominal skin was dermatomed (thickness 400 μm) for use in the diffusion studies. Franz-type diffusion cells were used over a period of 24 hours. The results of the membrane release studies indicated that the oil powders had achieved a significantly higher release than their respective redispersed oil powders. The release of salicylic acid from the redispersed oil powders and from their respective emulsions was similar. The transdermal delivery test outcomes showed that the effect of pH could have been influenced by the degree of ionisation, resulting in a decrease in permeation with increasing ionisation of salicylic acid, in accordance with the pH partition hypothesis. Furthermore, biopolymers, such as chitosan had demonstrated a penetration enhancing effect, which had led to the enhanced dermal and transdermal delivery of salicylic acid. A correlation was also found between the powder particle size and transdermal delivery. / MSc (Pharmaceutics), North-West University, Potchefstroom Campus, 2014 Oil powders Whey proteins Chitosan Carrageenan Topical delivery Release Salicylic acid Olie-poeiers Wei-proteïen Kitosaan Karrageenan Topikale aflewering Vrystelling Salisielsuur
92	Formulation, characterisation and topical application of oil powders from whey protein stabilised emulsions / Magdalena Kotze Kotze, Magdalena January 2014 (has links) The available literature indicates that to date, few research has been performed on oil powders for topical delivery. The aim of this project was to investigate the release characteristics of oil powder formulations, as well as their dermal and transdermal delivery properties. Whey protein-stabilised emulsions were used to develop oil powders. Whey protein was used alone, or in combination with chitosan or carrageenan. Nine oil powders, with salicylic acid as the active ingredient, were formulated by using the layer-by-layer method. Three different pH values (pH 4, 5 and 6) were used to prepare the formulations, because of the different charges that polymeric emulsifiers may have. The characteristics of the prepared oil powders were determined, including their droplet sizes, particle size distributions, loss on drying, encapsulation efficiencies, oil leakage and water dispersibility. Release studies (membrane diffusion studies) were conducted by utilising cellulose acetate membranes (0.2 μm pore size) and Franz-type diffusion cells over a period of eight hours. The release of the active ingredient was determined for all nine powders, their respective template emulsions, as well as their respective oil powders redispersed in water. The release of salicylic acid from the respective redispersed oil powders was then further compared to its release from the template emulsions and from the oil powders. The effect of pH and different polymer types used in preparing the oil powders, their respective redispersed oil powders and the template emulsions were determined with regards to the release of the active ingredient from all these preparations. The effect of pH and different polymers used was furthermore determined on the oil powders and their respective redispersed oil powders, with regards to their dermal and transdermal deliveries. Transdermal delivery and skin uptake were investigated on specifically selected powders only, based on the outcomes of the oil powder characterisation and release data. The qualifying formulations were chitosan pH 4, 5 and 6, whey and carrageenan pH 6 oil powders, together with their respective redispersed oil powders in water. Human abdominal skin was dermatomed (thickness 400 μm) for use in the diffusion studies. Franz-type diffusion cells were used over a period of 24 hours. The results of the membrane release studies indicated that the oil powders had achieved a significantly higher release than their respective redispersed oil powders. The release of salicylic acid from the redispersed oil powders and from their respective emulsions was similar. The transdermal delivery test outcomes showed that the effect of pH could have been influenced by the degree of ionisation, resulting in a decrease in permeation with increasing ionisation of salicylic acid, in accordance with the pH partition hypothesis. Furthermore, biopolymers, such as chitosan had demonstrated a penetration enhancing effect, which had led to the enhanced dermal and transdermal delivery of salicylic acid. A correlation was also found between the powder particle size and transdermal delivery. / MSc (Pharmaceutics), North-West University, Potchefstroom Campus, 2014 Oil powders Whey proteins Chitosan Carrageenan Topical delivery Release Salicylic acid Olie-poeiers Wei-proteïen Kitosaan Karrageenan Topikale aflewering Vrystelling Salisielsuur
93	Analyse der in-vivo Funktion der Transkriptionsfaktoren TGA2.1 und TGA2.2 aus Tabak nach Fusion mit einer konstitutiven Aktivierungsdomäne / In vivo functional analysis of the tobacco transcription factors TGA2.1 and TGA2.2 fused to a constitutive activation domain Lenk, Ingo 02 May 2001 (has links) No description available. 570 Biowissenschaften, Biologie Mathematics and Computer Science as-1 ASF-1 SARP TGA2.1 TGA2.2 plant VP16 transcription salicylic acid pathogen 42.13 Molekularbiologie WD
94	Conception et caractérisation de microréacteurs photocatalytiques / Design and characterization of a photocatalytic microreactor Charles, Guillaume 25 February 2011 (has links) L'objectif général du travail de recherche était l'amélioration de la compréhension de la réaction de dégradation photocatalytique de l’acide salicylique choisi comme polluant modèle. Un réacteur ouvert ayant un canal parallélépipédique, de largeur et de profondeur de l'ordre du millimètre, imprégné de catalyseur TiO₂ , a permis de caractériser la dégradation de l’acide salicylique en fonction des dimensions du canal, du débit, de la concentration en polluant et de l’intensité d'irradiation UV. La fraction dégradée d’acide salicylique diminue avec le débit, la concentration d’entrée et augmente avec l’intensité d’irradiation UV. Pour un temps de passage donné, la réduction de la profondeur et la largeur du microcanal, améliore l’efficacité de la dégradation. En effet, d'une manière générale, la vitesse de la réaction de dégradation est proportionnelle à la surface catalytique sur le volume réactionnel. Le rapport de la surface imprégnée sur le volume du microcanal est augmenté par la miniaturisation du canal ce qui entraine une meilleure dégradation. Un modèle basé sur le modèle de Langmuir-Hinshelwood et tenant compte du transfert de matière permet de rendre compte des résultats expérimentaux. Ce modèle met en évidence que la limitation de la réaction de dégradation par le transfert de matière est plus importante aux plus faibles débits (< 10 ml/h) et quand le canal devient plus profond. La simulation prédit des taux de conversion de l’ordre de 90 %, soit en agissant sur la géométrie (réacteur multicanaux, longueur totale des canaux de l’ordre du mètre), soit sur le procédé (réacteur à recyclage fermé) / The overall objective of the research work was to improve the understanding of the photocatalytic reaction of salicylic acid degradation chosen as model pollutant. An open reactor having a parallelepiped channel, of width and depth near millimetre size, coated with TiO₂ catalyst, was used to characterize the salicylic acid degradation in function of channel dimensions, flow rates, inlet pollutant concentrations and UV irradiation intensities. The degraded fraction of salicylic acid decreases with the flow rate, inlet concentration while it increases with UV irradiation intensity. For a given residence time, the reduction of the microchannel depth and width improve the degradation efficiency. Indeed, the reaction rate of degradation generally increases with the ratio of catalyst area on reaction volume. The ratio of coated area on microchannel volume is increased by miniaturization of the channel which leads to a larger degradation. A model based on the Langmuir-Hinshelwood approach which takes into account the mass-transfer account very well for the experimental results. This model highlights that reaction limitation by mass-transfer is larger at the lowest flows (< 10 mL/h) and when the channel becomes deeper. The simulation allows us to predict that conversion ratio of about 90%, can be reach by both acting on the geometry (multichannel reactor, total length of channels of the order of meter) or on the process (batch recirculation reactor) Photocatalyse Microréacteur Stéréolithographie TiO₂ déposé Transfert de matière Acide salicylique Langmuir-Hinshelwood Intensification Procédés Photocatalysis Microreactor Stéréolithographie TiO₂ coated Mass-transfert Salicylic acid Langmuir-Hinshelwood Intensification Process
95	INVESTIGATING THE FUNCTIONAL ROLE OF MED5 AND CDK8 IN ARABIDOPSIS MEDIATOR COMPLEX Xiangying Mao (6714896) 02 August 2019 (has links) <p>The Mediator (Med) complex comprises about 30 subunits and is a transcriptional co-regulator in eukaryotic systems. The core Mediator complex, consisting of the head, middle and tail modules, functions as a bridge between transcription factors and basal transcription machinery, whereas the CDK8 kinase module can attenuate Mediator’s ability to function as either a co-activator or co-repressor. Many Arabidopsis Mediator subunit has been functionally characterized, which reveals critical roles of Mediator in many aspects of plant growth and development, responses to biotic and abiotic stimuli, and metabolic homeostasis. Traditional genetic and biochemical approaches laid the foundation for our understanding of Mediator function, but recent transcriptomic and metabolomic studies have provided deeper insights into how specific subunits cooperate in the regulation of plant metabolism. In Chapter 1, we highlight recent developments in the investigation of Mediator and plant metabolism, with emphasis on the large-scale biology studies of <i>med</i> mutants.</p> <p>We previously found that MED5, an Arabidopsis Mediator tail subunit, is required for maintaining phenylpropanoid homeostasis. A semi-dominant mutation (<i>reduced epidermal fluorescence 4-3</i>, <i>ref4-3</i>) that causes a single amino acid substitution in MED5b functions as a strong suppressor of the pathway, leading to <a>decreased soluble phenylpropanoid accumulation, reduced lignin content and dwarfism</a>. In contrast, loss of MED5a and MED5b (<i>med5</i>) results in increased levels of phenylpropanoids. In Chapter 2, we present our finding that <i>ref4-3</i> requires CDK8, a Mediator kinase module subunit, to repress plant growth even though the repression of phenylpropanoid metabolism in <i>ref4-3 </i>is CDK8-independent. Transcriptome profiling revealed that salicylic acid (SA) biosynthesis genes are up-regulated in a CDK8-dependent manner in <i>ref4-3,</i> resulting in hyper-accumulation of SA and up-regulation of SA response genes. Both growth repression and hyper-accumulation of SA in <i>ref4-3</i> require CDK8 with intact kinase activity, but these SA phenotypes are not connected with dwarfing. In contrast, mRNA-sequencing (RNA-seq) analysis revealed the up-regulation of a DNA J protein-encoding gene in <i>ref4-3</i>, the elimination of which partially suppresses dwarfing. Together, our study reveals genetic interactions between Mediator tail and kinase module subunits and enhances our understanding of dwarfing in phenylpropanoid pathway mutants.</p> <p>In Chapter 3, we characterize other phenotypes of <i>med5</i> and <i>ref4-3</i>, and find that in addition to the up-regulated phenylpropanoid metabolism, <i>med5</i> show other interesting phenotypes including hypocotyl and petiole elongation as well as accelerated flowering, all of which are known collectively as the shade avoidance syndrome (SAS), suggesting that MED5 antagonize shade avoidance in wild-type plants. In contrast, the constitutive <i>ref4-3 </i>mutant protein inhibits the process, and the stunted growth of <i>ref4-3 </i>mutants is substantially alleviated by the light treatment that triggers SAS. Moreover, <i>ref4-3</i> mimics the loss-of-function <i>med5</i> mutants in maintaining abscisic acid (ABA) levels under both normal and drought growth conditions. The phenotypic characterization of <i>med5</i> mutants extend our understanding of the role of Mediator in SAS and ABA signaling, providing further insight into the physiological and metabolic responses that require MED5.</p> <p>In Chapter 4, we explore the function of MED5 and CDK8 in gene expression regulation by investigating the effect of mutations in Mediator including <i>med5</i>, <i>ref4-3</i>, <i>cdk8-1</i> and <i>ref4-3 cdk8-1</i> on genome-wide Pol II distribution. We find that loss of MED5 results in loss of Pol II occupancy at many target genes. In contrast, many genes show enriched Pol II levels in <i>ref4-3</i>, some of which overlap with those showing reduced Pol II occupancy in <i>med5</i>. In addition, Pol II occupancy is significantly reduced when CDK8 is disrupted in <i>ref4-3</i>. Our results help to narrow down the direct gene targets of MED5 and identify genes that may be closely related to the growth deficiency observed in <i>ref4-3</i> plants, providing a critical foundation to elucidate the molecular function of Mediator in transcription regulation.</p> Molecular Biology Bioinformatics Plant Biology phenylpropanoid biosynthetic pathway Mediator complex Salicylic acid dwarfing shade avoidance syndrome Chip-Seq
96	Estudo das alterações da parede celular durante ativação de mecanismos de defesa em Momordica charantia como fator de produção de metabólitos secundários bioativos / Study of cell wall changes during activation of defense mechanisms in Momordica charantia as factor of production of bioactive secondary metabolites Santos, Vitor Francisco dos 26 September 2014 (has links) Momordica charantia é uma espécie de planta pertencente à família Cucurbitaceae. No Brasil, é conhecida pelo nome popular de Melão de São Caetano. É encontrada em grande parte do globo terrestre, sendo que no Brasil é observada nas regiões litorâneas e principalmente nas regiões do interior do país. Escolhemos o estudo com Momordica charantia devido suas propriedades terapêuticas conhecidas serem de grande interesse. Ela vem ganhando cada vez mais reconhecimento através de pesquisas científicas realizadas, visto que, já é utilizada a milhares de anos através da cultura popular. Tais pesquisas têm confirmado e entendido cada vez mais as propriedades medicamentosas desta planta e os mecanismos responsáveis por tais funções nesta espécie, sendo as propriedades antidiabéticas, antivirais e anticancerígenas as de maior destaque. Os experimentos realizados em torno da Momordica charantia, na busca destes compostos foram todos realizados utilizando extratos retirados dos próprios tecidos já diferenciados na planta adulta (sementes, folhas, raízes e frutos). Neste trabalho, foi realizado a pesquisa de metabólitos secundários produzidos pela cultura de células em suspensão de Momordica charantia durante a fase de crescimento desta e após a realização de ensaios de elicitação com Ácido Salicílico (AS). Nosso laboratório vem se dedicando aos estudos da composição da parede celular vegetal e suas alterações, bem como dos mecanismos de defesa empregados pelas células em suspensão em condições de estresse biótico e abiótico. O ácido salicílico é um dos hormônios vegetais envolvido em vários mecanismos de respostas que envolve o estresse vegetal e de desenvolvimento da planta tais como o de garantir resistência a patógenos por exemplo. Quando ocorre algum processo de infecção ou lesivo para a planta, ocorre um aumento na concentração de AS no interior da planta. Esse aumento leva a ativação de certas vias metabólicas que culminam na produção de metabólitos secundários e na degradação, fragmentação ou espessamento da parede celular. Como reposta dos ensaios de elicitação realizados podemos comprovar os efeitos do AS mediados na produção de metabólitos secundários que foram aumentados conforme a concentração de AS. Foi utilizado para os ensaios de elicitação AS nas concentrações de 0,5 , 1,0 e 5 mmol/L. Para o monitoramento da cultura e averiguação da efetividade dos ensaios de elicitação foi utilizado a monitoria através da dosagem de proteínas totais, compostos fenólicos totais e açúcares redutores totais tanto liberados para o meio extracelular quanto produzidos no meio intracelular. Foi determinado as variações dos componentes da parede celular durante a fase de crescimento e após os ensaios de elicitação onde foi comprovado que quanto maior a concentração de AS, maiores são os fragmentos de açúcares fragmentados da parede celular. Foi evidenciado também a presença de triterpenos na cultura celular (em comparação com os padrões isolados da planta), tanto na fase de crescimento e também após a indução com os ensaios de elicitação com AS. / Momordica charantia is a plant from the Cucurbitaceae family. In Brazil, it is known by the popular name of Melão de São Caetano. It is found across the whole world, and in Brazil it can be found in coastal and interior regions of the country. The aim to study Momordica charantia is due to its known therapeutic properties that are already used for thousands of years through popular culture. The studies have confirmed and understood various drug-like properties of this plant and the mechanisms responsible for such functions in this species, such as antidiabetic, antiviral and anticancer properties. The researches with Momordica charantia were all performed using extracts obtained from seeds, leaves, roots and fruit. In this work, the isolation and characterization of metabolites as standards from leaves and stems of Momordica charantia was performed. The research of secondary metabolites produced in cell culture suspension of Momordica charantia without elicitor or after elicitation with salicylic acid (SA) was conducted. Salicylic acid is a plant hormone involved in various mechanisms of responses. When the plant suffers an infection or injury, it is followed by an increase in AS concentration. This increase leads to activation of certain metabolic pathways that culminate in the production of secondary metabolites and degradation, fragmentation or cell wall thickening. AS was utilized for the elicitation experiments at 0.5, 1.0 and 5 mmol/L. For the monitoring of plant cell culture, it was determinate the total protein, phenolic compounds and reducing sugars content, into the extra and intra cellular medium. Where it was verified that AS modulates the production of these molecules in culture. After this, we determined the variation in the oligosaccharides in the extracellular medium obtained in the presence or absence of AS. It was observed the degree of polymerization of oligosaccharides higher when increase AS concentration in the medium. In conclusion, this study can demonstrate the effects of SA on the production of secondary metabolites in plant cell culture, which were increased as the concentration of AS increased. The presence of triterpenes in cell culture was confirmed to compare the molecules obtained from culture with that isolated from plant standards. Ácido Salicilico Bioquímica de Carboidratos Carbohydrate Biochemistry Elicitor Elicitor Hypersensitive Response Metabólitos secundários Momordica charantia L Momordica charantia L Resposta de Hipersensibilidade Salicylic acid Secondary metabolites Triterpenes Chemistry of Triterpenos
97	Expressão e caracterização de metacaspases e estudos mitocondriais em plantas superiores / Expression and characterization of metacaspases and mitochondrial studies in higher plants Souza, Wagner Rodrigo de 17 December 2009 (has links) RESUMO A morte celular programada (PCD) é um processo vital que ocorre em todos os eucariotos. Em plantas, os mecanismos básicos que governam a PCD não estão esclarecidos. Sabe-se que a PCD em plantas é ativada pelo acúmulo de ácido salicílico e influxo de íons cálcio, bem como pela geração de ERO que ocorre nos cloroplastos e nas mitocôndrias. Além disso, as plantas possuem um grupo de proteases denominadas metacaspases, que assemelham-se estruturalmente com as caspases, proteínas que executam PCD em animais. Apesar destes conhecimentos, os mecanismos que governam a ativação da PCD são desconhecidos. Nesse contexto, o presente trabalho procurou investigar alguns fatores possivelmente envolvidos em PCD vegetal. Com esse objetivo, foram isoladas e caracterizadas mitocôndrias de cultura de células em suspensão de Rubus fruticosus. Foram avaliados os efeitos do Ca2+ e do AS sobre as funções mitocondriais, dentre elas a geração de ERO, diminuída pelo AS, porém aumentada por Ca2+. Um mecanismo foi proposto para explicar a diminuição de ERO pelo AS e as respostas observadas para AS e Ca2+ sobre as mitocôndrias são discutidas com base no possível envolvimento na PCD vegetal. A segunda parte do trabalho envolveu a expressão e caracterização de metacaspases (AtMCPs) em Arabidopsis thaliana. As proteases demonstraram autoprocessamento quando superexpressas in planta, assim como ocorre com as caspases em animais. A expressão de AtMCPs nesse modelo não produziu nenhum fenótipo de morte celular, sugerindo que o fenômeno ocorra por meio da integração de duas ou mais metacaspases. Foram estudadas também as propriedades biológicas de AtMCPs recombinantes em E. coli, demonstrando-se diferentes efeitos. Nossos estudos visam contribuir para a melhor compreensão de mecanismos básicos possivelmente envolvidos na PCD em plantas superiores. / ABSTRACT Programmed cell death (PCD) is a fundamental process that occurs in all eukaryotes. In plants, such phenomenon is not well understood. It is known that PCD in plants is activated through salicylic acid (SA) accumulation, Ca2+ ion fluxes, as well as reactive oxygen species (ROS) generation, which occurs mainly in chloroplasts and mitochondria. Besides, plants have a family of proteases, named metacaspases, which are proteases structurally similar to the caspases, members of proteins involved in animal PCD execution. In despite of this knowledge, the mechanism by which plant PCD is activated remains elusive. In this context, the aim of this work was to investigate some factors potentially involved in plant PCD. To this purpose, mitochondria from cell suspension cultures of Rubus fruticosus were isolated and characterized. It was investigated the effects of SA and Ca2+ on mitochondrial functions, as well. We have focused on ROS generation, which are important signals involved in plant PCD. It was shown that Ca2+ increased ROS generation, while SA decreases such production. A mechanism was proposed to explain the SA effects on isolated mitochondria, and the responses obtained from Ca2+ and SA addition on the organelle are discussed, based on the possible involvement of these effects in plant PCD. In the second part of this work, it was investigated the expression of metacaspases (AtMCPs) in the model plant Arabidopsis thaliana. The proteases have demonstrated self-processing when expressed in planta, similar to the animal caspases. Such expression did not cause any cell death phenotype, suggesting that PCD could be activated through the integration of two or more MCPs, if they are involved. It was investigated the effects of recombinant AtMCPs in E. coli, as well, demonstrating different responses. Our work contributes to a better understanding of factors potentially involved in plant PCD. Ácido salicílico Cálcio Calcium Espécies reativas de oxigênio Higher plants Metacaspases Metacaspases Mitochondria Mitocôndria Plantas superiores Programme reactive oxygen species Salicylic acid
98	Validação de metodologias analíticas para determinação quantitativa de princípios ativos em formulações farmacêuticas empregadas para \"peelings\" químicos / Validation of analytical methodologies for quantitative determination of drugs in pharmaceutical formulations employeds to chemical \"peelings\" Ramos, Tatiane Rodrigues 15 June 2004 (has links) Os \"peelings\" químicos são formulações esfoliantes utilizadas na terapêutica de queratoses actínicas, rugas, discromias pigmentares, acne vulgar e rosácea. A solução de Jessner (SJ) é amplamente usada como agente em peelings químicos. Na presente pesquisa foram empregadas formulações farmacêuticas de SJ como amostras para a determinação quantitativa simultânea das substâncias ativas. A solução alcoólica é composta de resorcinol (14%), ácido salicílico (14%) e ácido láctico (14%). Duas amostras de gel são compostas de resorcinol (30%) e ácido salicílico (20%), respectivamente. Foram desenvolvidos e validados métodos espectrofotométricos na primeira e segunda derivada no UV para a quantificação de ácido salicílico e resorcinol, respectivamente na SJ, utilizando etanol como branco e foram desenvolvidos métodos espectrofotométricos na primeira derivada no UV para a quantificação de resorcinol e ácido salicílico nas amostras em gel, utilizando ácido sulfúrico 0,1 N como branco. Quando o etanol foi utilizado como branco, as curvas de calibração foram lineares em uma faixa de concentração de 22,0 a 34,0 µg/mL (resorcinol) e de 12,0 a 24,0 µg/mL (ácidos salicílico), para os métodos na segunda e primeira derivada no UV (usando etanol como branco), ambos com coeficientes de correlação de 0,9999. Quando o ácido sulfúrico 0,1N foi utilizado como branco, as curvas de calibração foram lineares em uma faixa de concentração de 18,0 a 42,0 µg/mL (resorcinol) e de 8,0 a 32,0 µg/mL (ácido salicílico), para o método na primeira derivada no UV com coeficientes de correlação de 0,9999 e 0,9998 respectivamente. Os resultados nas amostras alcoólicas de SJ (amostras A e B) foram 104,4% de resorcinol (DPR 0,83%) e 103,2% de ácido salicílico (DPR 0,68%) enquanto que nas amostras em gel (amostras E e F) foram 101,9% de resorcinol (DPR 0,34%) e as amostras em gel C e D, 100,7% de ácido salicílico (DPR 0,28%). / Chemical peelings are exfoliating formulations used in the treatment of actinic keratosis, wrinkles, dyschromies, acne vulgaris and rosacea acne.The Jessner Solution (JS) sample is widely used as chemical peeling agent. In this research we selected a JS pharmaceutical preparation for simultaneous quantitative determination of the active components. The alcoholic solution sample is composed of resorcinol (14%), salicylic acid (14%) and lactic acid (14%); two gel samples are composed of resorcinol (30%) and salicylic acid (20%), respectively. First and second derivative UV spectrophotometric methods were developed and validated for quantitative determination of salicylic acid and resorcinol, respectively. In JS alcoholic solution, ethanol was used as background. A first derivative UV spectrophotometric method was developed for quantitative determination of resorcinol and salicylic acid in gel samples using 0.1N sulfuric acid as background. Calibration curves were linear within a concentration range from 22.0 to 34.0 µg/mL (resorcinol) and from 12.0 to 24.0 µg/mL (salicylic acid), for second and first derivative UV spectrophotometric method (ethanol as background) with a correlation coefficients of 0.9999 and 0.9999, respectively. Calibration curves were linear within a concentration range from 18,0 to 42,0 µg/mL (resorcinol) and from 8.0 to 32.0 µg/mL (salicylic acid), for first derivative UV spectrophotometric method (0.1N sulfuric acid as background) with correlation coefficients of 0.9999 and 0.9998, respectively. The alcoholic samples of JS (sample A and B) presented 104.4% of resorcinol (RSD 0.83%) and 103.2% of salicylic acid (RSD 0.68%) while the gel samples (sample E and F) presented 101.9% of resorcinol (RSD 0.34%) and gel sample C and D, 100.7% of salicylic acid (RSD 0.28%). Ácido salicílico Chemical "peelings" Esfoliação química Espectrofotometria (Aplicações) Resorcinol Resorcinol Salicylic acid Spectrophotometry (Applications) Validação Validation
99	Estudo do efeito de respostas de hipersensibilidade sobre a parede celular em cultura de células de amora-preta (Rubus fruticosus) / study of the effects of hypersensitive response on cell wall in blackberry-black cell culture (Rubus fruticosus) Souza, Fernando Aparecido Mariano de 23 February 2007 (has links) Como os outros organismos, as plantas têm a habilidade de se defenderem através do reconhecimento de patógenos (resposta de hipersensibilidade - RH), causando a morte imediata das células no sítio primário da infecção, desta maneira oferecendo resistência ao seu crescimento. A RH é caracterizada pela necrose dos tecidos neste local, através de muitos sinais ainda não completamente elucidados, como a formação de radicais livres, incluindo o peróxido de hidrogênio (H2O2), e o reforço da parede celular. O objetivo deste estudo foi estabelecer a relação entre esses sinais em cultura de células de amora-preta (Rubus fruticosus). As condições experimentais para a análise da parede celular, das espécies reativas de oxigênio (EROs) e do H2O2 foram padronizadas. O polissacarídeo ácido (ramnoglucuronogalactana, F-I), o ácido salicílico (AS), e o metil jasmonato (MeJA), bem estabelecidos efetores da resposta da defesa, foram usados como elicitores. A produção das EROs e do H2O2 foram ativadas por F-I e pelo AS, seguidos da liberação de fragmentos de dissacarídeos da parede celular, aparentemente devido a sua degradação. Por outro lado, uma produção pequena de EROs e de H2O2 foram observadas na presença de MeJA, assim como um aumento de fragmentos de massa molecular mais elevada, que podem funcionar como sinais para o reforço da parede celular, indução de enzimas e para a produção de outra moléculas de defesa. Quando da elicitação, concomitante, com dois elicitores, AS + MeJA, houve a inibição da produção de EROs causada pelo MeJA e foi mantida a liberação de compostos extracelulares de massa molecular mais elevada. / Like the other organisms, plants have the ability to self-defend through recognition of pathogens (hypersensitive response - HR), causing immediate cell death at the primary infection site, thus offering resistance to their grown. The HR is characterized by necrosis of tissues in this site via many signals still not completely elucidated, like formation of free radicals including H2O2 and reinforcement of cell wall. The aim of this study was to establish the relationship between these signals in blackberry-black cell culture (Rubus fruticosus). The experimental conditions for analysis of cell wall, reactive oxygen species (ROS) and H2O2, were established. Acid polysaccharide (rhamnoglucuronogalactan, F-I), salicylic acid (SA), and methyl jasmonate (MeJA), well established effectors of the defense response, were used as elicitors. ROS and H2O2 production was activated by F-I and SA, followed by release of fragments like disaccharides from the cell wall, apparently due to its degradation. By contrast, a small production of ROS and H2O2 was observed in presence of MeJA, as well as an increase of high molecular weight fragments, that may function as signals for reinforcement of cell wall, enzyme induction and production of others defense molecules. Together, the two elicitors SA and MeJA inhibited the ROS production, caused by MeJA, while sustaining release of the extra cellular compounds of high molecular weight. ácido salicílico cell wall elicitores elicitors EROs H2O2 H2O2 hypersensitive response methyl jasmonate metil jasmonato parede celular ramnoglucuronogalactana resposta de hipersensibilidade rhamnoglucuronogalactan ROS Rubus fruticosus Rubus fruticosus salicylic acid
100	Identificação de genes diferencialmente expressos em tomateiro induzidos por ácido salicílico e por Fusarium oxysporum f. sp. lycopersici AMARAL, Daniel Oliveira Jordão do 14 June 2007 (has links) Submitted by (ana.araujo@ufrpe.br) on 2017-02-07T16:48:16Z No. of bitstreams: 1 Daniel Oliveira Jordao do Amaral.pdf: 1158857 bytes, checksum: e7a95fb82b8780bf1c190ef328318925 (MD5) / Made available in DSpace on 2017-02-07T16:48:16Z (GMT). No. of bitstreams: 1 Daniel Oliveira Jordao do Amaral.pdf: 1158857 bytes, checksum: e7a95fb82b8780bf1c190ef328318925 (MD5) Previous issue date: 2007-06-14 / To identify tomato plant (Lycopersicon esculentum Mill), cv. BRH, genes which answer to plant pathogen Fusarium oxysporum f. sp. lycopersici and salicylic acid, the carrier molecule for activation of responses of plant defense, it was used the suppression subtractive hybridization (SSH) technique, from leaf cDNAs, 24h after salicylic acid, library denominated AS, and root cDNA, 72h after inoculation with F. oxysporum f. sp. lycopersici, incompatible interaction, library denominated FO. This work represents the first report of global gene expression of tomato plant induced by salicylic acid and F. oxysporum f. sp. lycopersici, using SSH technique; it was identified a total of 307 clones in the two subtractive libraries, being 143 obtained in the AS library and 164 in the FO library. Probable functions for genes were obtained by sequencing of clones and subsequent homology research at datas. These isolated genes are involved in several processes related to resistance against plant pathogen such as: hypersensitive response, programmed cell death, synthesis and transport of antimicrobial metabolites, signal perception and transduction, synthesis of pathogenesis-related proteins, lipid metabolism and selective degradation of proteins. It was identified in FO library a higher number of defense-related genes (26%) than in AS library (24%). In relation to the number of genes encoding antimicrobial proteins, they were only found in FO library (7%). However, genes involved in secondary compound metabolism were higher in AS library (13%) in relation to FO library (4%). These genes related to controlled degradation of proteins were also higher in AS library (3%) than in FO library (1%). The results suggest that the resistance of tomato plant induced by salicylic acid and by plant pathogen occur by distinct mechanisms. / Com o propósito de identificar genes no tomateiro (Lycopersicon esculentum Mill), cv. BRH, que respondem ao fitopatógeno Fusarium oxysporum f. sp. lycopersici e ao ácido salicílico, molécula mensageira na ativação de resposta de defesa em plantas, foi utilizada a técnica de hibridização subtrativa por supressão (HSS), a partir de cDNAs de folhas, 24h após o tratamento com ácido salicílico, biblioteca denominada (AS), e cDNAs de raízes, 72h após a inoculação com Fusarium oxysporum f. sp. lycopersici, interação incompatível, biblioteca denominada (FO). Esse trabalho representa o primeiro relato da expressão gênica global no tomateiro induzido pelo ácido salicílico e pelo F. oxysporum f. sp. lycopersici, utilizando a técnica HSS. Foram identificados um total de 307 clones nas duas bibliotecas subtraídas, sendo 143 clones obtidos na biblioteca (AS) e 164 clones na biblioteca FO. As prováveis funções dos genes foram obtidas pelo sequenciamento dos clones e subseqüente pesquisa de homologia em bancos de dados. Os genes encontrados estão envolvidos em diversos processos relacionados à resistência contra fitopatógenos como: resposta de hipersensibilidade, morte celular programada, síntese e transporte de metabólicos antimicrobianos, percepção e transdução de sinal, síntese de proteínas relacionadas à patogênese, metabolismo de lipídeos e degradação controlada de proteínas. Foram identificados na biblioteca FO um número maior de genes implicados em mecanismos de defesa (26%), do que na biblioteca AS (24%). Em relação ao número de genes codificadores de proteínas antimicrobianas foram encontrados apenas na biblioteca FO (7%). Entretanto, os genes envolvidos no metabolismo de compostos secundários foi maior na biblioteca AS (13%) em relação a biblioteca FO (4%). Os genes relacionados a degradação controlada de proteínas também foi maior na biblioteca AS (3%) do que na biblioteca FO (1%). Os resultados obtidos sugerem que a resistência no tomateiro induzido pelo ácido salicílico e pelo patógeno ocorre por mecanismos distintos. Lycopersicum esculentum Fusarium oxysporum f. sp. lycopersici Tomate Genética vegetal Ácido salicílico Hibridação Salicylic acid Suppression subtractive hybridization FITOTECNIA::MELHORAMENTO VEGETAL

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