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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.
61

The effect of citric acid supplementation on growth performance, carcass weight, tibia bone breaking strength, and ash content of male ross 308 broiler chickens

Thokwane, Judith January 2023 (has links)
Thesis (M.Sc. (Animal Production)) -- University of Limpopo, 2023 / Two experiments were conducted to determine the effect of citric acid inclusion level in the diet on growth performance, carcass weight, tibia bone breaking strength and ash content of male Ross 308 broiler chickens aged one to 35 days. The first experiment determined the effect of citric acid inclusion level in the diet on growth performance traits of male Ross 308 broiler chickens aged one to 21 days. The experiment commenced with 200 male day-old Ross 308 broiler chickens with an initial average live weight of 40±1.6g per chick. The chicks were assigned to five treatment groups in a completely randomized design, each replicated five times, and each replicate having ten chicks. The citric acid inclusion levels were at 0, 12.5, 25 or 50g per kg DM of feed. The second experiment determined the effect of citric acid inclusion level in the diet on growth performance, carcass weight, tibia bone breaking strength and ash content traits of male Ross 308 broiler chickens aged 22 to 35 days. The experiment commenced with 180 male Ross 308 broiler chickens aged 22 days. The chickens were assigned to four treatment groups, each having three replicate pens of eight chickens per replicate in a completely randomized design. Data was analysed using the General Linear model (GLM) procedures of the Statistical Analysis of System, version 9.3.1 software program. Where there were significant differences (P<0.05) between the treatment means, Tukey Multiple Comparison Test was used for mean separation. Citric acid inclusion in the starter diets improved (P<0.05) live weight and growth rate of male Ross 308 broiler chickens aged one to 21 days. Citric acid inclusion in the starter diets did not affect (P>0.05) daily feed intake, body weight gain and feed conversion ratio of male Ross 308 broiler chickens aged one to 21 days. The inclusion of citric acid did affect (P<0.05) live weight, body weight gain, feed conversion ratio and growth rate of chickens aged 22 to 35 days. Citric acid inclusion levels used in the present study influenced (P<0.05) DM and CP digestibility, ME intake and N-retention of male broiler chickens aged 22 to 35 days. The results of the current study showed that citric acid inclusion in a diet improved (P<0.05) chicken bone morphology. Thus, positive relationships were observed between citric acid inclusion level and right tibia bone weight, diameter, calcium, phosphorous and Magnesium contents of chicken bones aged 35 days. There were positive relationships between citric acid inclusion level and breast weight of male Ross 308 broiler chickens aged 35 days. Further studies are recommended to ascertain these findings. / National Research Foundation (NRF)
62

Implications of plasticization on the properties of hot-melt extruded oral dosage forms

Schilling, Sandra Ursula 27 May 2010 (has links)
The influence of plasticization and other formulation factors on the properties of hot-melt extruded dosage forms for the controlled release of water-soluble active compounds was investigated. Citric acid monohydrate was demonstrated to function as a solid-state plasticizer in hot-melt extruded Eudragit® RS PO tablets and in cast films when concentrations below the compatibility limit were employed. Melting of the organic acid and solubilization in the polymer during extrusion were necessary to observe the plasticizing effect. The release rate of diltiazem hydrochloride, used as a high-melting, water-soluble model drug, from melt extruded Eudragit® RS PO matrix tablets increased and became independent of the original drug particle size in the presence of citric acid monohydrate. Thermal analysis of physical mixtures demonstrated that citric acid promoted drug melting during extrusion by interaction and melting point depression. Diltiazem hydrochloride remained amorphous in the final dosage form, and leaching of citric acid monohydrate enhanced drug diffusion by increasing the matrix porosity. Delayed-release matrix pellets with particle sizes below one mm were prepared by hot-melt extrusion, and the influence of the matrix forming polymer and the type and level of plasticizer on the processibility and release properties was investigated. Pellets complied with the USP requirement for delayed release articles to release less than 10% drug at pH 1.2 after 2 hours when plasticized Eudragit® S100 was used as the release-controlling material. High levels of efficient plasticizers had to be employed to decrease the polymeric melt viscosity, increase the process yield and enable extrusion at moderate temperatures to avoid instabilities during processing and storage. The aqueous solubility of the plasticizer further impacted the drug release rate in acid. A novel application of hot-melt extrusion for the preparation of monolithic matrices comprising enteric coated particles was studied. The influence of the mechanical strength of the multiparticulates, pellet loading and nature of the hydrophilic carrier material on the preservation of the delayed-release properties after extrusion was investigated. Soft particles coated with brittle films remained intact when low-melting carriers that did not solubilize the enteric film during extrusion were used, and the dissolution profile was stable over one year. / text
63

Determination of the molecular and physiological basis of citric acid tolerance in spoilage yeast

McGuire, Lynne I. January 2009 (has links)
The ability of yeasts to grow and adapt under extreme environmental conditions including within the presence of weak organic acid preservatives has led to substantial economic losses through manufactured food and beverage spoilage. The food industry has employed the use of various weak organic acids such as sorbic, benzoic and acetic acid as preservatives to help prevent spoilage by yeasts and moulds. The mechanisms by which S. cerevisiae is able to adapt to these weak organic acids have been extensively studied. A lesser studied weak organic acid preservative is citric acid. The aim of this study was to gain further information on the mechanisms of citric acid adaptation and through this identify potential targets for new preservation strategies. Current knowledge indicates the involvement of the HOG pathway in citric acid adaptation. A citric acid sensitivity screen from a previous study also isolated a SR protein kinase Sky1p, involved in polyamine metabolism, which has been connected with other crucial cellular processes including modulation of ion homeostasis and osmotic shock. In this study we have undertaken a systematic screen for genes that confer increased sensitivity to citric acid paying particular attention to those involved in polyamine metabolism and those known to encode proteins which have evidence of interactions with Sky1p. Many of the deletion strains tested exhibited hypersensitivity to citric acid including Δsky1. Protein-protein interaction maps for Sky1p highlighted an interesting secondary interacting protein Nmd5p, an importin crucial for the nuclear localization of Hog1p. This information suggested there may be the possibility of linkage between Sky1p and Hog1p and their roles in citric acid tolerance, perhaps through Nmd5p. This provided an incentive to perform a range of experiments to test this theory. Proteomic and phosphoproteomic analyses were carried out to study protein expression and phosphorylation changes in response to citric acid stress. Comparative proteomic analyses for Δsky1, Δhog1 and BY4741a with and without citric acid identified four instances of analogous protein expression responses in both Δsky1 and Δhog1, suggesting functional overlap upon exposure to citric acid. Epistasis studies of Δhog1Δsky1 suggested that the two protein kinases do not function on the same pathway. However, overexpression analyses did suggest some functional interaction between Hog1p and Sky1p in mediating citric acid resistance since overexpression of Sky1p in Δhog1 resulted in partial rescue of growth. Further supporting evidence for some functional interaction or linkage was provided by Hog1p phosphorylation and localisation studies. Δsky1 exhibited dual phosphorylation of Hog1p in the absence of citric acid stress; implying that loss of SKY1 results in dual phosphorylation of Hog1p by either prompting phosphorylation or perhaps by interfering with dephosphorylation of Hog1p. Localisation studies of Hog1p proved that like osmotic stress, citric acid stress results in nuclear translocation of Hog1p and deletion of SKY1 seemed to interfere with this localisation to some extent. In light of the results attained in this study we believe we have evidence to propose a novel role for Sky1p in mediating resistance to citric acid and that there is also substantial evidence to suggest that Sky1p shares some functional redundancy and perhaps functional linkage with Hog1p in citric acid adaptation.
64

Influência do tratamento da dentina radicular com três substâncias irrigadoras ácidas no vedamento marginal apical de obturações endodônticas. / The influence of root dentin treatment with three acid irrigating solutions in apical marginal sealing of endodontic fillings.

Carlik, Jaime 21 December 2000 (has links)
Analisou-se a influência da aplicação do ácido cítrico em três concentrações, EDTA-T e EDTA-C no vedamento marginal apical de canais radiculares em 90 caninos humanos extraídos. O preparo químico-cirúrgico dos canais radiculares foi realizado pela técnica de Paiva & Antoniazzi, sendo esses dentes posteriormente distribuídos aleatoriamente em seis grupos. Cada grupo de dentes recebeu um tratamento químico específico efetuado pela repleção do canal radicular por 3 minutos com uma das seguintes substâncias: soro fisiológico, ácido cítrico a 10%, ácido cítrico a 15%, ácido cítrico a 20%, EDTA-T a 17% e EDTA-C a 17%. Posteriormente, todos os canais radiculares foram obturados com cones de guta-percha e cimento N-Rickert pela técnica de cones múltiplos com condensação vertical. Foi observado um aumento crescente de infiltração do corante azul-de-metileno nos canais tratados com ácido cítrico correspondente ao aumento da concentração do ácido. A maior média de infiltração verificada ocorreu nos canais radiculares tratados com EDTA-C e as menores registradas naqueles tratados com soro fisiológico ou EDTA-T. As diferenças entre as médias de infiltração apical nos seis grupos experimentais, analisadas conjuntamente, não foram estatisticamente significantes. Em comparações individualizadas, houve diferença significante (p < 0,05) entre o grupo G6 (EDTA-C) tanto em relação ao grupo G5 (EDTA-T) quanto ao grupo G1 (soro fisiológico). / Ninety extracted human teeth were analysed in this work to verify the influence of citric acid application under three concentrations, EDTA-T and EDTA-C in the apical marginal sealing of root canals. Chemical and surgical root canal preparations were performed by Paiva & Antoniazzi technique, being these teeth randomly distributed in six groups. Each group had specific chemical treatment of filling the root canal for 3 minutes with one of the following substances: saline solution, 10% citric acid, 15% citric acid, 20% citric acid, 17% EDTA-T and 17% EDTA-C. All root canals were filled with gutta-percha cones and N-Rickert cement by the multiple cone technique with vertical condensation. A crescent increase of methylene blue dye penetration could be observed in the root canals treated with citric acid equivalent to the increase in acid concentration. The highest penetration mean was shown in the root canals treated with EDTA-C and the lowest in those treated wint saline solution or EDTA-T. The differences between the apical penetration means in the six experimental groups that had been together analysed showed no statistical significance. When individually compared, there was a significant difference (p<0,05) between group G6 (EDTA-C), group G5 (EDTA-T) and group G1 (saline solution).
65

Purificação da fosfolipase A2 e análise bioquímica do plasma seminal de ovinos e caprinos / Purification of phospholipase A2 and biochemical analyis of seminal plasma from bucks rams

Franco, Hélio José Antunes 22 April 2010 (has links)
A quantificação dos componentes bioquímicos como frutose, ácido cítrico e proteína total existentes no plasma seminal de caprinos e ovinos localizados na região Centro-Oeste do Brasil é uma forma de avaliar a atividade fisiológica e bioquímica espermáticas. Estes dados servem como indicadores de prováveis problemas com os testículos e glândulas acessórias desses animais e de sua respectiva fertilidade. A frutose e o ácido cítrico são importantes para o sêmen como fonte de energia metabólica e como componente de sistema tampão, respectivamente. A frutose é um marcador da função secretora das vesículas seminais, e é um componente importante para a sobrevivência dos espermatozóides em condições anaeróbicas e está estreitamente relacionada com a motilidade inicial das células espermáticas. Sendo assim, os objetivos do presente projeto foram analisar quantitativamente esses componentes do plasma seminal de bodes e carneiros sob latitude 20&deg;31\'S em quatro épocas do ano e purificar, através de técnicas cromatográficas, a enzima fosfolipase A2, importante proteína presente no plasma seminal. As análises bioquímicas foram feitas usando-se um espectrofotômetro UV/Vis para obtenção da curva padrão e para a determinação das concentraçõoes mensais e da concentração anual média dos constituintes analisados. A purificação da PLA2 foi feita por cromatografia líquida preparativa usando-se como fase estacionária a coluna Superdex 75-16/60 (GE HealthCare) de exclusão por tamanho e membranas semipermeáveis de 10 e 30 kDa. Como resultado das análises bioquímicas, obteve-se a concentração anual média de proteínas totais de 3,27 &plusmn; 0,60 g/dL para ovinos e de 5,02 &plusmn; 0,43 para caprinos, ácido cítrico de 1015,33 &plusmn; 66,50 µg/mL para ovinos e de 1584,35 &plusmn; 143,90 µg/mL para caprinos e frutose de 23,40 &plusmn; 4,80 mg/dL para ovinos e 72,73 &plusmn; 18,50 mg/dL para caprinos. Os resultados mostraram que a PLA2 extraída do plasma seminal de ovinos tem massa molecular próxima de 13,8 kDa e a PLA2 do plasma seminal de caprinos tem massa molecular próxima a 12,8 kDa. / Quantification of biochemical components in seminal plasma including fructose, citric acid and total protein of goat and sheep of the Midwest region of Brazil is one way of evaluating the biochemical and physiological activity of the sperm. These data serve as indicators of potential problems with the testicles and accessory glands of these animals and their relative fertility. The fructose and citric acid are important for the semen as a source of metabolic energy and as a component of a buffer, respectively. Fructose is a marker of secretory function of seminal vesicles, important for the survival of spermatozoa under anaerobic conditions, and is closely related to the initial motility of sperm cells. Therefore, the objectives of this project were to quantitatively analyze these components in the seminal plasma of goats and sheep in latitude 20&deg;31\'S 3 1\'S in four seasons and purify by chromatographic techniques the enzyme phospholipase A2, an important protein in the seminal plasma. Biochemical analysis were done using a spectrophotometer UV / Vis to obtaining the standard curve and to determine the monthly and annual average concentration of the constituents analyzed. The purification of PLA2 was performed by preparative liquid chromatography using the column as stationary phase Superdex 75-16/60 (GE HealthCare) by size exclusion and semipermeable membranes 10 and 30 kDa. As a result of biochemical analysis, we obtained the annual average concentration of total protein of 3,27 &plusmn; 0,60 g / dL for sheep and 5,02 &plusmn; 0,43 g/dL for goats, citric acid of 1015,33 &plusmn; 66, 50 g / mL for sheep and 1584,35 &plusmn; 143,90 g / mL for goats and fructose 23,40 &plusmn; 4,80 mg / dL for sheep and 72,73 &plusmn; 18,50 mg / dL for goats. The results showed that the PLA2 extracted from seminal plasma of sheep has a molecular mass of 13,8 kDa and the next PLA2 from goat seminal plasma has a molecular mass close to 12,8 kDa.
66

Avaliação do efeito de diferentes agentes quelantes e desmineralizantes sobre a microdureza da dentina radicular / Evaluation of the effect of different chelating agents and demineralizing on the microhardness of root dentin.

Pimenta, Josilaine Amaral 17 October 2011 (has links)
O presente estudo teve como objetivo avaliar a ação das soluções de quitosana, EDTA e ácido cítrico sobre a microdureza da dentina radicular. Utilizaram-se 10 incisivos centrais superiores humanos, os quais tiveram suas coroas seccionadas transversalmente e desprezadas. As raízes foram incluídas em resina acrílica de rápida polimerização e o bloco formado raiz/resina adaptado a máquina de corte. Desprezou-se o primeiro corte transversal da porção cervical e dividiu-se o segundo, em quatro quadrantes. Cada quarto foi destinado à confecção do corpo de prova obtendo-se 4 espécimes para cada raiz, um para cada solução (n=10): G1- EDTA 15%; G2- ácido cítrico; G3- quitosana 0,2% e G4- controle. Os espécimes receberam 50 &mu;L da solução por 5 minutos, sendo em seguida, lavados com água deionizada. Utilizou-se um microdurômetro (dureza Knoop) com carga de 10 g durante 15 segundos. Os resultados mostraram que todas as soluções avaliadas apresentaram capacidade de reduzir a microdureza da dentina radicular de forma semelhante entre si e estatisticamente diferente a do grupo controle (p<0,01). Concluiu-se as soluções de quitosana 0,2%, EDTA 15% e ácido cítrico 10% apresentam efeito semelhante na redução da microdureza dentinária. / The aim of this study was to evaluate the action of solutions: chitosan, EDTA and citric acid on the microhardness of the root dentin. There were used 10 human maxillary central incisors which ones had their crown cross-sectioned and discarded. The roots were embedded in acrylic resin of rapid polymerization and the block formed root/resin suitable by cutting machine. Neglecting the first cross-section of the cervical portion and the second was divided in four quadrants. Each quarter was destined to the confection of the specimen and it was got 4 specimen to each root, one for each solution (n=10): G1- EDTA 15%; G2- citric acid;G3- chitosan 0,2 % and G4- control. The specimen received 50 &mu;L of the solution for 5 minutes, and following up they were washed by deionized water. It was used a microhardness (Knoop hardness) with a load of 10g during 15 seconds. The results showed that all the solutions evaluated presented a capacity to reduce the microhardness of the root dentin in a similar way between them, and statically differ from the control group (p<0,01). It was concluded that chitosan 0,2% EDTA 15% and the citric acid 10% presented a similar effect in the reduction of the dentin microhardness.
67

Efeito da desmineralização do enxerto ósseo autógeno particulado no reparo de defeitos críticos em calvária de ratos. Estudo microscópico e microtomográfico / Effect of demineralization of particulate autogenous bone graft in critical size defects in rat calvaria. Microscopic and microtomográfic study

Paulus, Jefrey Elias Rojas 18 May 2016 (has links)
O processo de desmineralização óssea tem sido mostrado vantajoso em procedimentos de enxertia óssea empregando blocos osseos, porem a sua utilização na periodontia em enxertos osseos autógenos particulados não esta ainda descrita na literatura. De acordo com a literatura é possível observar que existem diferentes agentes demineralizantes na pratica clinica os quais podem ser empregados no processo de desmineralização óssea, razão pela qual este estudo teve como objetivo comparar dois diferentes agentes desmineralizantes de enxertos ósseos autógenos particulados (ácido cítrico pH1 a 50% e tetraciclina hidroclorada a 50mg/ml) em diferentes tempos de aplicação, quanto ao efeito produzido no reparo de defeitos críticos em calvária de ratos. Foram utilizados 120 ratos adultos machos com aproximadamente 4 meses de vida. Neste estudo foi utilizado o modelo de defeito crítico de 8 mm, esses animais foram divididos em 8 grupos de estudo formados por 15 animais (5 em cada período experimental): CN (controle negativo): os defeitos permaneceram sem enxerto; CP (controle positivo): os defeitos foram preenchidos por osso particulado não desmineralizado; AC 15: os defeitos foram preenchidos com osso particulado desmineralizado por ácido cítrico durante 15 segundos; AC 30: os defeitos foram preenchidos com osso particulado desmineralizado por ácido cítrico durante 30 segundos; AC 60: os defeitos foram preenchidos com osso particulado desmineralizado por ácido cítrico durante 60 segundos; TCN 15: os defeitos foram preenchidos com osso particulado desmineralizado por tetraciclina durante 15 segundos; TCN 30: os defeitos foram preenchidos com osso particulado desmineralizado por tetraciclina durante 30 segundos; TCN 60: os defeitos foram preenchidos com osso particulado desmineralizado por tetraciclina durante 60 segundos. Foi realizada aeutanasia dos animais aos 7, 30 e 60 dias para realização de microtomografia computadorizada e analise histomorfometrica, para avaliar a área, volume e densidade óssea nos defeitos após os tempos experimentais definidos. Aos 7 dias, não era esperada formação de tecido ósseo significante, mas surpreendentemente, os espécimes desmineralizados com ácido cítrico demonstraram precocidade na produção de eventos regenerativos já nesse período. Durante os períodos experimentais foi possível observar como os espécimes tratados com acido cítrico apresentavam maior formação óssea nos defeito quando comparados com os controles e com os grupos onde empregados tetraciclina. Efeito provavelmente relacionado com a eliminação da parte mineral do osso e liberação de Proteinas morfogeneticas ósseas e fatores de crescimentos, liberados a partir da matriz ossea Concluiu-se que a desmineralização com ácido cítrico do osso autógeno particulado enxertado em defeitos críticos promoveu maior área, volume e densidade de formação óssea do que a desmineralização com tetraciclina e do que a não desmineralização. Observando-se melhores resultados aos 15 e 30 segundos de desmineralização. / Bone demineralization process has been shown useful in bone grafting procedures using onlay bone grafting, however its use in periodontics in bony autogenous particulate graft is not yet described in the literature. According to the literature you can see that there are different demineralizantes agents in clinical practice which can be used in bone demineralization process, which is why this study was to compare two different demineralization agents of bone autogenous particulate graft (citric acid pH1 the 50% tetracycline Hydrochloride and 50mg / ml) in different application time, the effect produced in the repair of critical defects in rat calvarium. 120 adult male rats with approximately 4 months of age were used. In this study we used the 8mm critical defect model, the animals were divided into 8 study groups consisting of 15 animals (5 in each experimental period): CN (negative control): the defect remained free graft; CP (positive control): the defects were filled by nondemineralized bone particles; AC 15: The defects were filled with demineralized bone particles of citric acid for 15 seconds; AC 30: defects were filled with demineralized bone particles of citric acid for 30 seconds; AC 60: The defects were filled with demineralized bone particles of citric acid for 60 seconds; TCN 15: defects were filled with demineralized bone particles tetracycline for 15 seconds; TCN 30: defects were filled with demineralized bone particles tetracycline for 30 seconds; TCN 60: defects were filled with demineralized bone particles tetracycline for 60 seconds. aeutanasia animals was performed at 7, 30 and 60 days for performing computed microtomography and histomorphometric analysis to assess the area, bone volume and density of the defects after the defined experimental times. At 7 days, it was not expected significant formation of bone tissue, but surprisingly, samples demineralized with citric acid demonstrated earliness in the production of regenerative events already during this period. During the experimental periods was possible to observe how the specimens treated with citric acid showed increased bone formation in defects when compared to controls and to groups where employees tetracycline. Effect probably related to the disposal of the mineral part of bone and release of bone morphogenetic proteins and factors of growth, released from the bone matrix concluded that the demineralisation by citric acid particulate autogenous bone graft in critical defects caused greater area, volume formation and bone density than tetracycline demineralization and demineralization that do not. Observing better results at 15 and 30 seconds demineralization.
68

Efeitos de antioxidantes e radiação gama na qualidade de cana-de-açúcar minimamente processada / Effects of antioxidants and gamma radiation on the quality of minimally processed sugarcane

Spoto, Rodrigo Fillet 21 February 2019 (has links)
A cana-de-açúcar é um alimento bem aceito por toda a população em geral, podendo ser consumido na forma de toletes (in natura) ou na forma de caldo, podendo ser apreciado com gelo somente, ou adicionado de sucos cítricos, mas nem sempre tratada com algum sanitizante ou outro produto para manutenção de sua qualidade. A cana-de-açúcar também pode ser consumida na forma de minimamente processada, sanitizada e embalada, facilitando sua utilização em redes de alimentação. Embora o processamento mínimo de vegetais aumente a suscetibilidade ao ataque de microrganismos e escurecimento enzimático, essas alterações podem ser reduzidas com o uso de tratamentos adequados, como sanitizantes e agentes antioxidantes. Em vista disso, procurou-se nesse trabalho avaliar a qualidade da cana-de-açúcar minimamente processada, tratada com antioxidantes e radiação gama. Os tratamentos aplicados para a conservação dos toletes de cana-de-açúcar foram: ácido cítrico nas concentrações de 1,5% e 3,0%; cloridato de L-cisteína a 1,0% e 2,0%; radiação gama com as doses de 2,0 e 4,0 kGy. Antes de receberem os tratamentos, os toletes de cana-de-açúcar foram processados e sanitizados com solução de hipoclorito de sódio. Após a drenagem, os toletes foram acondicionados em embalagens de polietileno de alta densidade e refrigerados a 4°C. Os produtos foram analisados após 1, 7 e 14 dias de armazenamento. Todos os tratamentos apresentaram-se em condições sanitárias adequadas para o consumo, independente das concentrações e dosagens. Os toletes de canas-de-açúcar tratados com ácido cítrico e cloridrato de L-cisteína apresentaram os melhores resultados quanto à inibição das enzimas de escurecimento, polifenoloxidase e peroxidase, sendo a cana-de-açúcar tratada com L-cisteína a que apresentou o caldo com melhores resultados quanto à inibição de seu escurecimento e níveis de açúcares. Todos os tratamentos inibiram o desenvolvimento de microrganismos / Sugar cane is a well-accepted food for the general population and can be consumed in the form of straw (in natura) or in the form of juice, which can be enjoyed with ice only, or added with citrus juice, but always treated with some sanitizing agent or other product to maintain its quality. Sugarcane can also be consumed in the form of minimally processed, sanitized and packaged sugarcane, improving its use in food networks. Unless, minimal processing of vegetables increases susceptibility to microorganism attack and enzymatic browning, but such changes can be reduced with the use of appropriate treatments such as sanitizers and antioxidants. The aim of this work was to evaluate the quality of minimally processed sugar cane treated with antioxidants or gamma radiation. The treatments applied for the preservation of sugarcane straw were: citric acid at concentrations of 1.5% and 3.0%; L-cysteine at concentrations of 1.0% and 2.0%, and gamma irradiation at doses of 2.0 and 4.0 kGy. Before receiving the treatments, the sugar cane straws were processed and sanitized with sodium hypochlorite solution. After draining, the straws were packed in high-density polyethylene packages and refrigerated at 4°C. The products were analyzed after 1, 7 and 14 days of storage. All treatments were in sanitary conditions suitable for the consumption, independent of the concentrations and dosages. The sugarcane treated with citric acid and L-cysteine presented the best results regarding the inhibition of the darkening enzymes, polyphenoloxidase and peroxidase. Sugarcane treated with L-cysteine presented the juice with better sugar levels and inhibition of browning. All treatments showed effective inhibiton of the microorganisms development
69

Efeito da desmineralização óssea sobre parâmetros de superfície e sobre o comportamento de pré-osteoblastos em cultura: estudo em microscopia eletrônica de varredura e confocal / Effect of bone demineralization on surface parameters and on behavior of pre-osteoblasts in culture: study in scanning electron microscopy and confocal microscopy

Salmeron, Samira 02 April 2015 (has links)
A desmineralização óssea superficial tem se demonstrado favorável à consolidação de enxertos e ao comportamento celular, entretanto os mecanismos envolvidos ainda não estão esclarecidos. Os subsídios para o embasamento biológico da desmineralização, proporcionado por publicações anteriores, sugeriram que modificações na superfície óssea teriam influenciado o comportamento de pré-osteoblastos em cultura. Assim, este estudo objetivou comparar o efeito de duas concentrações de ácido cítrico na desmineralização de superfícies ósseas onde foram cultivadas células pré-osteoblásticas (MC3T3-E1), e analisar parâmetros de superfície comparando superfícies desmineralizadas a não desmineralizadas. Setenta amostras ósseas bicorticais foram removidas das calvárias de 35 ratos e divididas em grupos para as análises: 1) Microscopia Eletrônica de Varredura (MEV) para avaliação da área de recobrimento e espessura da camada de células sobre as amostras (n = 15) durante 24, 48 e 72 horas: Grupo AC.10 amostras desmineralizadas por 30 segundos com ácido cítrico 10 %; Grupo AC.50 amostras desmineralizadas por 30 segundos com ácido cítrico 50 %; e Grupo C (controle) amostras não desmineralizadas; 2) Microscopia Confocal para análise da área de expressão e intensidade de fluorescência das BMP-2, -4 e -7: AC.10 seis amostras desmineralizadas conforme item 1); AC.50 seis amostras desmineralizadas conforme item 1); C três amostras não desmineralizadas; 3) Microscopia Confocal para análise da rugosidade superficial média (Ra e Sa): Grupos AC.10 e AC.50 com cinco amostras cada, desmineralizadas conforme o item 1), sendo cada amostra seu próprio controle (análises antes e depois da desmineralização). Também foram avaliadas as distâncias entre picos (P-P) e entre picos e vales (P-V) antes e depois da desmineralização; 4) Microscopia Eletrônica de Varredura / Espectroscopia de Energia Dispersiva (MEV / EDS) para análise da composição superficial: mesmas amostras do item 3) foram avaliadas antes e depois da desmineralização quanto à porcentagem atômica (%A) de carbono, oxigênio, magnésio, fósforo, enxofre e cálcio. Análises estatísticas foram feitas adotando nível de significância de 95 %. Amostras desmineralizadas apresentaram células morfologicamente em estágios mais avançados de diferenciação do que as não desmineralizadas. A área de recobrimento superficial foi significantemente maior após 24 horas de cultura nos grupos teste do que no controle e a espessura da camada de células também foi maior nos grupos teste às 48 e 72 horas. Houve significantemente maior expressão de BMP-2 e -7 nos grupos teste do que no controle e, apenas AC.10 demonstrou maior expressão de BMP-4 do que os demais grupos, sem significância em relação a AC.50. Os parâmetros de superfície Ra e Sa foram inconclusivos, mas P-P e P-V diminuíram consideravelmente após a desmineralização para distâncias compatíveis com superfícies favoráveis à adesão e diferenciação celular. A análise da composição química superficial revelou diminuição da %A de enxofre e magnésio nos grupos teste. A concentração do ácido, embora não tenha apresentado diferença significante para a maioria das análises, pareceu ter influência positiva nos resultados para o ácido cítrico 10 %. Concluiu-se que a desmineralização superficial parece promover a proliferação e diferenciação celular, proporcionando superfícies com características de composição e topografia que favorecem o comportamento celular verificado. / The superficial bone demineralization has proved to be a favorable procedure for bone grafts consolidation and cell behavior, however the underlying mechanisms have not been clarified yet. Therefore, this study aimed to compare the effect of two concentrations of citric acid on demineralization of bone surfaces where pre-osteoblastic cells (MC3T3-E1) were cultivated, and analyze surface parameters comparing demineralized bone surfaces with non-demineralized surfaces. Seventy bicortical bone samples were harvested from the calvaria of 35 rats and divided into groups as follows: 1) Scanning Electron Microscopy (SEM) to evaluate the coating area and thickness of cells layers cultured on the samples (n = 15) for 24, 48, and 72 hours: Group CA.10 samples demineralized for 30 seconds with 10 % citric acid; Group CA.50 samples demineralized for 30 seconds with 50 % citric acid, and Group C (control) non-demineralized samples; 2) Confocal Microscopy for analysis of expression area and intensity of fluorescence of BMP-2, -4, and -7: CA.10 six samples demineralized as item 1); CA.50 six samples demineralized as item 1); Group C three non-demineralized samples; 3) Confocal Microscopy for surface mean roughness analysis (Ra and Sa): Groups CA.10 and CA.50 made up of five samples each and demineralized according to item 1), each sample was its own control (analysis before and after demineralization). The distances between peaks (P-P) and between peaks and valleys (P-V) were also evaluated before and after demineralization; 4) Scanning Electron Microscopy / Energy dispersive Spectroscopy (SEM / EDS) to analyze the surface composition: the same samples of item 3) were evaluated before and after demineralization for atomic percentage (%A) of carbon, oxygen, magnesium, phosphorus, sulfur and calcium. Statistical test was made by adopting the 95 % significance level. Demineralized samples showed cells with morphology in the later stages of differentiation than non-demineralized ones. The coating surface area by cells was significantly higher after 24 hours of culture in the test groups than in the control and the thickness of the layers were also greater in the test groups at 48 and 72 hours of evaluation. There was significantly higher expression of BMP-2 and -7 in test groups than in the control group, and only the CA.10 group showed higher BMP-4 expression than the other groups, but the difference was not statistically significant compared to the CA.50 group. Ra and Sa surface parameters were inconclusive, however P-P and P-V decreased considerably after demineralization to distances compatible with surfaces favorable to cell adhesion and cell differentiation. The chemical composition analysis of the surfaces revealed a decrease in the %A for sulfur and magnesium in test groups. Although the acid concentration did not shown significant difference for most analysis, it seemed to have a positive influence for the results with citric acid 10 %. It was concluded that the surface demineralization seems to promote cell proliferation and differentiation, providing surfaces with composition and topography that can favor observed cell behavior.
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Efeito da desmineralização óssea superficial na consolidação de enxertos ósseos autógenos: estudo histomorfométrico e imunohistoquímico em calvária de ratos / Effect of superficial bone demineralization on the consolidation of autogenous bone grafts: histomorphometric and immunohistochemical study in calvaria of rats

Carvalho, Érika Beatriz Spada de 04 September 2017 (has links)
Dados recentes apontam que a desmineralização óssea pode promover a consolidação de enxertos e a proliferação e diferenciação de pré-osteoblastos, mas os mecanismos biológicos envolvidos nesse processo precisam ser esclarecidos. Neste estudo foram investigados, em calvária de 126 ratos Wistar, os efeitos da desmineralização óssea sobre o reparo de enxertos ósseos em bloco cujas superfícies de contato foram desmineralizadas por tetraciclina hidroclorada (TCN) na concentração de 50mg/ml ou ácido cítrico (AC) a 10% (pH=1) por 15, 30 ou 60 segundos (n=6). Enxertos controle foram realizados sem desmineralização. Após 7, 30 e 60 dias, blocos teciduais contendo os enxertos foram removidos dos animais e processados histotecnicamente para coloração com hematoxilina e eosina. Os espécimes de 30 dias de pós-operatório também forneceram amostras para avaliação imunohistoquímica para osteocalcina (OCN) e fosfatase ácida tartarato resistente (TRAP), marcadores de formação e reabsorção óssea respectivamente. A análise qualitativa demonstrou estágios mais avançados no processo de reparo ósseo desde os 7 dias nos grupos desmineralizados em relação ao controle, com consolidação ocorrendo a partir dos 30 dias de pós-operatório, em especial nos espécimes desmineralizados com TCN por 60 segundos. A análise quantitativa demonstrou aumento significante da área de osso neoformado e de superfícies de consolidação óssea com o tempo (ANOVA a dois critérios, p<0,05). Maior porcentagem de área de osso neoformado ocorreu nos grupos AC15 e TCN60 quando comparados ao grupo controle em todos os períodos avaliados (p = 0,02). Aos 30 dias, o grupo C apresentou menor porcentagem de extensão de superfícies consolidadas em relação aos grupos TCN60, TCN30 e AC15 (p = 0,0015). Aos 60 dias, o grupo AC60 apresentou a totalidade das superfícies ósseas do enxerto e do leito consolidadas ao osso neoformado na interface com diferença em relação ao grupo controle (p = 0,0015), que também apresentou menores resultados em relação aos grupos AC15, TCN15 e TCN60. A análise imunohistoquímica foi inconclusiva para explicar os achados histomorfométricos. A relação OCN/TRAP foi maior nos grupos controle, AC30, TCN30 e TCN60, mas a localização da imunomarcação margeando as superfícies do osso neoformado e no interior dos espaços medulares sugere que a observação revela fenômenos de remodelação óssea normal, sem distinção entre os grupos. Concluiu-se que a desmineralização das superfícies ósseas de contato entre o enxerto ósseo e o leito receptor com AC ou TCN durante 15, 30 ou 60 segundos promoveu maior área de tecido ósseo neoformado na interface enxerto-leito do que a não desmineralização, principalmente nos períodos mais precoces de reparação. A consolidação do osso neoformado ao enxerto e ao leito receptor também foi maior em todos os grupos desmineralizados em relação ao controle. Os melhores resultados, entretanto foram apresentados pelos grupos AC15 e TCN60. / Recent data suggest that bone demineralization may promote graft consolidation and proliferation as well as differentiation of pre-osteoblasts, but the biological mechanisms involved in this process need to be clarified. In this study, the effects of bone demineralization were studied on the repair of onlay bone grafts whose contact surfaces were demineralized by tetracycline hydrochloride (TCN) at a concentration of 50mg / ml or citric acid (AC) a 10% (pH = 1) for 15, 30 or 60 seconds (n = 6). Control grafts were performed without demineralization. After 7, 30 and 60 days, tissue blocks containing the grafts were removed from the animals and processed histotechnically for hematoxylin and eosin staining. The 30-day post-operative specimens also provided samples for immunohistochemical evaluation for osteocalcin (OCN) and tartrate resistant acid phosphatase (TRAP), markers of formation and bone resorption respectively. The qualitative analysis demonstrated more advanced stages of bone repair early in the 7 days evaluation in the demineralized groups in relation to the control. The quantitative analysis showed a significant increase in the area of newly formed bone and bone consolidation with time (two way ANOVA, p<0.05). A higher percentage area of newly formed bone occurred in the AC15 and TCN60 groups when compared to the control group in all the evaluated periods (p = 0.02). At 30 days, group C had lower percentage of consolidated surfaces than groups TCN60, TCN30 and AC15 (p = 0.0015). At 60 days, the AC60 group presented bone surfaces totally consolidated to the newly formed bone at the interface with difference in relation to the control group (p = 0.0015), which also presented lower results in relation to the AC15, TCN15 and TCN60. The immunohistochemical analysis was inconclusive to explain the histomorphometric findings. The OCN / TRAP ratio was higher in the control, AC30, TCN30 and TCN60 groups, but the localization of the immunostaining, lining the surfaces of the newly formed bone and within the medullary spaces, suggests that the observation reveals normal bone remodeling phenomena. It was concluded that the demineralization of the bone surfaces of contact between The bone graft and the receptor bed with AC or TCN for 15, 30 or 60 seconds promoted a greater area of newly formed bone tissue at the graft-bed interface than non-demineralization, especially in the earlier periods of healing. The consolidation of the newly formed bone to the graft and to the recipient bed was also higher in all the demineralized groups in relation to the control. The best results, however, were presented by groups AC15 and TCN60.

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