Preparation, stability and in vitro evaluation of liposomes containing chloroquine / Stephnie Nieuwoudt

Nieuwoudt, Stephnie

January 2010

Malaria is currently a huge treat worldwide, as far as infections are concerned, and is responsible for thousands of deaths per annum. The dilemma associated with the development of anti–malarial drug resistance over the past few decades should be addressed as a matter of urgency. Novel drug delivery systems should be developed in order to employ new and existing anti–malarial drugs in the treatment and management of malaria. The aim of these delivery systems should include an improvement in the efficacy, specificity, acceptability and therapeutic index of anti–malarial drugs. Previous studies have suggested that liposomes have the ability to encapsulate, protect and to promote the sustained release of anti–malarial drugs. Two liposome formulations, namely liposomes and chloroquine entrapped in liposomes, were formulated during this thesis and evaluated by conducting a stability study and an in vitro study with the main focus on cell viability. The stability study consisted of a series of stability tests regarding the stability of nine liposome and nine chloroquine entrapped in liposome formulations over a period of twelve weeks. The in vitro study included three assays such as a reactive oxygen species assay, a lipid peroxidation assay and a hemolysis assay. The aims of these studies included the manufacturing of liposomes, the incorporation of chloroquine into liposomes, the determination of the stability of the formulations as well as the evaluation of the possible in vitro toxicity of liposomes. Results obtained from these studies revealed that liposomes remained more stable over the stability study period in comparison to chloroquine entrapped in liposomes. The entrapment of chloroquine within liposomes was possible, although the initial entrapment efficiency (%) of 14.55 % was much too low. The production of reactive oxygen species occurred to a small extent in the red blood cells and the infected red blood cells. Equal amounts of reactive oxygen species (%) was observed within both the red blood cells and the infected red blood cells with a maximum value of 23.27 % in the presence of the chloroquine entrapped in liposomes at varying concentrations. Red blood cells experienced the highest degree of lipid peroxidation (%) in the presence of chloroquine, at varying concentrations, entrapped in liposomes. The maximum amount of lipid peroxidation (%) was 79.61 %. No significant degree of hemolysis (%) was observed in the red blood cells neither in the presence of the liposomes nor in the presence of the chloroquine entrapped in liposomes at varying concentrations. It can be concluded that liposomes are a more stable formulation and have less toxic effects on red blood cells and infected red blood cells in comparison to the chloroquine entrapped in liposome formulations. Future studies should investigate the possibility of a more stable and less toxic chloroquine entrapped in liposome formulation. / Thesis (M.Sc. (Pharmaceutics))--North-West University, Potchefstroom Campus, 2011.

Malaria

Liposomes

Chloroquine (CQ)

Reactive oxygen species (ROS)

Lipid peroxidation (LP)

Hemolysis

Liposome

Chlorokien (CQ)

Reaktiewe suurstof spesies (ROS)

Lipied peroksidasie (LP)

Hemolise

Preparation, stability and in vitro evaluation of liposomes containing amodiaquine / Jacques C. Scholtz

Scholtz, Jacques Coenraad

January 2010

Malaria is a curable disease that claims nearly one million lives each year. Problems with the treatment of malaria arise as resistance spreads and new treatment options are becoming less effective. The need for new treatments are of the utmost importance. Liposomes combined with antimalarials are a new avenue for research as liposomes can increase the efficacy of drugs against pathogens, as well as decreasing toxicity. Amodiaquine is a drug with known toxicity issues, but has proven to be effective and is, therefore, a prime candidate to be incorporated into the liposomal drug delivery system. The aim of this study was to prepare, characterize and evaluate the toxicity of the liposomes with incorporated amodiaquine. The solubility of amodiaquine was determined and liposomes formulated with, and without, amodiaquine entrapped. Accelerated stability studies (at 5 'C, 25 'C with relative humidity of 60% and 40 'C with a relative humidity of 40%) were conducted during which the size, pH, morphology and the entrapment efficacy was determined. The toxicity was determined in vitro by analysing the levels of reactive oxidative species and lipid peroxidation caused by the formulations to erythrocytes infected with P. falciparum as well as uninfected erythrocytes with flow cytometry. The solubility study of amodiaquine in different pH buffers showed that amodiaquine was more soluble at lower pH values. Solubility in solution with pH 4.5 was 36.3359 ± 0.7904mg/ml when compared to the solubility at pH 6.8, which was 15.6052 ± 1.1126 mg/ml. A buffer with a pH of 6 was used to ensure adequate solubility and acceptable compatibility with cells. Liposomes with incorporated amodiaquine were formulated with entrapment efficacies starting at 29.038 ± 2.599% and increasing to 51.914 ± 1.683%. The accelerated stability studies showed the median sizes and span values remained constant for both liposome and amodiaquine incorporated liposomes at 5 'C. The higher temperatures, i.e. 25 'C and 40 'C, displayed increases in the median size, and decreases in the span for both formulations. The conclusion can, therefore, be made that both liposome and amodiaquine incorporated liposomes are stable at lower temperatures. The entrapment efficacy increased from initial values to nearly 100% during the course of the stability study. This was attributed to amodiaquine precipitating from the solution. The pH values of the liposomes and amodiaquine incorporated liposomes remained constant for each formulation; though the amodiaquine incorporated liposomes had a lower starting pH, the formulations are both thought to be stable in terms of the pH. Toxicity studies revealed low levels of reactive oxygen species as well as low levels of lipid peroxidation for both liposome and amodiaquine incorporated liposomes, on both erythrocyte and Plasmodium infected erythrocytes. From the toxicity studies it can be concluded that liposomes and amodiaquine incorporated liposomes are not toxic to erythrocytes and infected erythrocytes. It was concluded that liposomes incorporating amodiaquine could possibly be used as a treatment option for malaria. / Thesis (M.Sc. (Pharmaceutics))--North-West University, Potchefstroom Campus, 2011.

Malaria

Liposomes

Amodiaquine

Plasmodium falciparum

Stability

Toxicity

Entrapment efficacy

Size determination

Reactive oxygen species

Lipid peroxidation

Liposome

Amodiakien

Stabiliteit

Toksisiteit

Inkorporerings effektiwiteit

Groottebepaling

Reaktiewe suurstof spesies

Lipied peroksidasie

Oxidation of ascorbate by protein radicals in simple systems and in cells

Liu, Chia-chi

January 2007

Thesis (PhD) -- Macquarie University, Division of Environmental and Life Sciences, Dept. of Chemistry and Biomolecular Sciences, 2007. / Bibliography: leaves 295-322. / Generation of peroxide groups in proteins exposed to a wide variety of reactive oxygen species (ROS) requires an initial formation of protein carbon-centred or peroxyl free radicals, which can be reduced to hydroperoxides. Both protein radicals and protein hydroperoxides are capable of oxidizing important biomolecules and thus initiate biological damage. In this study, we investigated the inhibition of protein hydroperoxide formation by ascorbate and GSH in gamma-irradiated HL-60 cells.--We used HL-60 cells as a model for general protection of living organisms by ascorbate (Asc) and glutathione (GSH) from the deleterious effects of protein hydroperoxides generated by radicals produced by gamma radiation. Measurement by HPLC indicated that incubation of HL-60 cells with Asc in the presence of ascorbate oxidase resulted in the accumulation of intracellular Asc. The intracellular Asc levels were lowered by irradiation, demonstrating intracellular consumption of Asc by the radiation-generated radicals. Exposure of HL-60 cells to increasing gamma irradiation doses resulted in increasing accumulation of protein peroxides in the cells. This was measured by the FOX assay. A significant decrease in intracellular protein hydroperoxides was noted when the cells were treated with ascorbic acid before irradiation. A dose-dependent protective effect of Asc was observed. Asc loading also provided strong protection from radiation-generated protein hydroperoxides independently of the composition of the external medium, showing that only the radicals formed within the cells were effective in oxidizing the cell proteins. Similarly, protein peroxidation was inhibited in cells with enhanced levels of GSH and increased when the intracellular GSH concentration was reduced. These findings indicate that ascorbate and GSH are important antioxidants in protecting cells from oxidative stress associated with the generation of protein hydroperoxide. / Mode of access: World Wide Web. / xxix, 322 leaves ill

Free radicals (Chemistry)

Antioxidants -- Physiological effect

Oxidative stress

Oxidizing agents

Vitamin C

Glutathione

Proteins -- Peroxidation

Peroxides -- Analysis

Active oxygen

ascorbate

protein radicals

protein hydroperoxides

HL-60 cells

GSH

L'acide carnosique et le carnosol, deux super-antioxydants du romarin (Rosmarinus officinalis) : rôles, mécanismes, physiologie et applications / Carnosic acid and carnosol, two supra-antioxidant of rosemary (Rosmarinus officinalis) : roles, mecanisms, physiology and applications

Loussouarn-Yvon, Margot

07 November 2017

L’acide carnosique (CA) et le carnosol (CARN), deux diterpènes spécifiques des Lamiacées, sont en abondance dans le romarin. Le CA extrait de cette plante est largement utilisé dans l’industrie pour ses propriétés antioxydantes portées par le groupe catéchol. Malgré beaucoup d’applications, les rôles et les modes d'action de ces composés in planta n’ont reçu que peu d’attention. Des analyses par HPLC-UV et imagerie d’autoluminescence révèlent que le CA et le CARN protègent les lipides contre des oxydations in vitro par les ERO. Lors de la préservation des lipides, des analyses de MS indiquent que le CA est oxydé en une variété de dérivés alors que le CARN résiste. L’utilisation d’une sonde de spin et de la spectroscopie RPE montre que le CA est un piégeur chimique des ERO. L’action inhibitrice du CARN sur des oxydations de lipides induites in vitro ou in vivo indique que le CARN interfère avec le processus de peroxydation lipidique. Des études in vivo de deux variétés de romarin contrastées en CA exposées à un stress photooxydant montrent que le CA protège les lipides in planta. Une étude des variations de CA et de CARN en fonctions des facteurs abiotiques met en avant qu’une forte intensité lumineuse et des fluctuations de températures favorisent la réponse antioxydante du CA qui s’oxyde en CARN. Des analyses de RT-qPCR montrent que les facteurs abiotiques ne stimulent pas la voie de biosynthèse du CA. En condition de stress oxydant, le CA du romarin préserve les membranes par piégeage des ERO produisant des dérivés d’oxydation, dont le CARN, qui protègent aussi les membranes en bloquant la réaction en chaîne de la peroxydation lipidique. / Carnosic acid (CA) and carnosol (CARN), two diterpenes specific of the Lamiaceae, are highly abundant in rosemary species. CA extracted from rosemary is used by industries for its antioxidative features, endowed by it catechol group. Despite numerous applications, the role and the mode of action of CA in planta has received little attention. Analyses, using HPLC-UV and luminescence imaging revealed that CA and CARN protect lipids from in vitro oxidation by ROS. Upon ROS oxidation of lipids, MS analyses indicated that CA was oxidized into various derivatives while CARN resisted. Using spin probes and EPR detection, we confirmed that CA, rather than CARN, is a ROS quencher. The inhibitory effect of CARN on lipid peroxidation induced in vitro or in vivo indicated that CARN interferes with lipid peroxidation. In vivo studies of two rosemary varieties contrasted in their CA content exposed to photooxidative stress showed that CA protects lipids in planta. A study of CA and CARN variations in response to abiotic factors showed that high light and temperature fluctuations lead to CA oxidation into CARN. RT-qPCR analyses revealed that abiotic factors do not stimulate CA biosynthesis genes. Under oxidative stress condition, rosemary CA preserves biological membranes by ROS scavenging, hence producing a set of oxidative derivatives, including CARN, which protect biological membranes by blocking the lipid peroxidation chain reaction.

Acide carnosique

Carnosol

Diterpènes phénolique

Antioxydants

Ero

Stress oxydant

Peroxydation lipidique

Carnosic acid

Carnosol

Phenolic diterpenes

Antioxidants

Ros

Oxidative stress

Lipid peroxidation

581

Avaliação de parâmetros espermatícos e de estresse oxidativo frente à homegeneização de doses de sêmen suíno armazenadas em diferentes diluentes / Assessment of sperm and oxidative stress parameters upon homogenization of liquid-stored boar semen in different extenders

Menegat, Mariana Boscato

January 2016

A homogeneização das doses de sêmen suíno e a ressuspensão dos espermatozoides durante o armazenamento têm sido considerados como procedimentos benéficos para a qualidade espermática. Contudo, os fundamentos acerca dessa recomendação não estão completamente elucidados. O objetivo deste estudo é avaliar o efeito da homogeneização nos parâmetros espermáticos e status oxidativo das doses de sêmen suíno durante o armazenamento. Vinte e um ejaculados suínos normospérmicos foram diluídos em split sample nos diluentes Androstar® Plus (AND) e Beltsville Thawing Solution (BTS) e as doses de sêmen foram submetidas aos protocolos sem homogeneização (NoHom) ou com homogeneização manual duas vezes ao dia (2xHom) durante o armazenamento a 17ºC por 168 h. Os parâmetros espermáticos foram avaliados de acordo com motilidade espermática, cinética espermática e integridade de membrana com as sondas fluorescentes SYBR-14/PI através do sistema CASA, integridade de acrossoma sob microscopia óptica com contraste de fase, teste de termorresistência a 38ºC por 30 min e 120 min, e pH das doses de sêmen. O status oxidativo foi determinado pela peroxidação lipídica, oxidação proteica, teor de grupos sulfidrila, espécies reativas intracelulares, potencial antioxidante total e atividade enzimática da superóxido dismutase (SOD). As doses inseminantes submetidas a NoHom ou 2xHom foram semelhantes (P>0,05) na maioria dos parâmetros espermáticos e oxidativos avaliados, para ambos os diluentes. A NoHom foi superior (P<0,05) à 2xHom quanto à motilidade e cinética espermáticas após o teste de termorresistência por 30 min, à manutenção do pH e à preservação da atividade da SOD. Além disso, melhores resultados nos parâmetros espermáticos e status oxidativo foram evidenciados no diluente AND em comparação ao BTS, exceto na motilidade total e progressiva, que diferiu apenas no final do período de armazenamento, e para espécies reativas intracelulares. Considerando que a homogeneização manual duas vezes ao dia não aprimorou a qualidade espermática e o status oxidativo, este procedimento não é necessário para o armazenamento de doses de sêmen normospérmicas por 168 h, tanto para o diluente Androstar® Plus quanto para o BTS. / Homogenization of diluted boar semen and resuspension of spermatozoa during storage have always been regarded as beneficial for semen quality. Nevertheless, the fundamental basis for its recommendation remains unclear. The aim of this study was to verify the effect of homogenization on spermatic parameters and oxidative status of boar semen doses during storage. One normospermic ejaculate from each of 21 boars was diluted in a split sample design with Androstar® Plus (AND) and Beltsville Thawing Solution (BTS) and semen doses were submitted to no-homogenization (NoHom) or twice-a-day manual homogenization (2xHom) during storage at 17°C for 168 h. Spermatic parameters were assessed upon motility, kinematics and membrane integrity with SYBR-14/PI with CASA system, acrosome integrity under phase-contrast microscopy, thermoresistance test at 38ºC for 30 min and 120 min, and pH. Oxidative status was determined by lipid peroxidation, protein oxidation, sulfhydryl content, intracellular reactive species, total radical-trapping antioxidant potential, and superoxide dismutase (SOD) activity. NoHom and 2xHom of liquid-stored semen doses were similar (P>0.05) in most of the spermatic and oxidative parameters for both AND and BTS extenders. NoHom was superior (P<0.05) to 2xHom regarding sperm motility and kinematics after thermoresistance test for 30 min, pH maintenance, and SOD activity preservation. Additionally, better results were evident for spermatic parameters and oxidative status in AND compared to BTS, except for total and progressive motility, which differed only at the end of the storage period, and intracellular reactive species. Taking into account that no beneficial effects for sperm motility traits and oxidative status were observed following twice-a-day homogenization, its use is not necessary for storage of semen doses for 168 h in both short- and long-term tested extenders.

Parâmetros espermatícos

Estresse oxidativo

Sêmen : Armazenamento

Semen : Suinos

Peroxidacao lipidica

Viabilidade espermática

CASA system

Insemination doses

Lipid peroxidation

Sperm viability

Storage

Adrenoleucodistrofia ligada ao cromossomo x e estresse oxidativo : papel do transplante de células hematopoiéticas e da interleucina 6

Rockenbach, Francieli Juliana

January 2012

Objetivos. Avaliar o papel do transplante de células hematopoiéticas (TCH) e da interleucina 6 (IL – 6) sobre vários parâmetros de estresse oxidativo em pacientes com Adrenoleucodistrofia ligada ao cromossomo X (X-ALD). Métodos. A concentração de malondialdeído (MDA), o conteúdo de carbolinas e sulfidrilas e a concentração de ácido hexacosanóico (C26:0) foram quantificados no plasma de pacientes X-ALD antes e após serem submetidos ao TCH. E, a concentração de MDA, a formação de carbonilas e a concentração de IL-6 foram quantificados em plasma e o conteúdo de glutationa reduzida (GSH) foi quantificado em eritrócitos de pacientes X-ALD com fenótipos cerebral infantil (cALD) ou assintomáticos no momento diagnóstico. Resultados. Observamos um aumento significativo na concentração de MDA em plasma de pacientes X-ALD antes e após o TCH em comparação ao grupo controle e uma redução significativa nesses valores após o transplante em comparação aos anteriores ao procedimento. Verificamos uma redução significativa no conteúdo de sulfidrilas no plasma de pacientes X-ALD antes do TCH em comparação ao grupo controle e um aumento significativo desses níveis após o TCH. Não observamos diferenças significativas no conteúdo de carbonilas no plasma de X-ALD antes e após o TCH, em comparação aos controles, apesar de observarmos uma redução significativa nesta determinação nos pacientes após o transplante em relação a antes do TCH. Os pacientes X-ALD apresentam níveis plasmáticos de C26:0 significativamente aumentados antes do TCH em comparação aos controles e, após o TCH, as concentrações de C26:0 foram reduzidas. Observamos uma correlação negativa significativa entre a medida do conteúdo de sulfidrilas e os níveis plasmáticos de C26:0 de indivíduos X-ALD antes do TCH. Também evidenciamos elevados níveis de MDA e da formação de carbonilas no plasma de pacientes cALD e assintomáticos em comparação ao grupo controle. Ainda, observamos redução significativa do conteúdo de GSH nos dois grupos testados comparados aos controles. A quantificação de IL-6 foi significativamente maior nos pacientes cALD, o que não foi observado nos pacientes assintomáticos, apesar destes mostrarem uma tendência de aumento da concentração de IL-6. Conclusões. Os resultados obtidos a partir do plasma de pacientes X-ALD antes e após o TCH demonstram que esta terapia, quando bem indicada e bem sucedida, tem alta efetividade em reduzir a concentração plasmática de C26:0 e é eficaz em reduzir a peroxidação lipídica e o dano oxidativo às proteínas nos pacientes X-ALD. Ainda, é possível relacionar o acúmulo de C26:0 e o dano oxidativo na patogênese da X-ALD. Nossos dados permitem sugerir que a lipoperoxidação e o dano oxidativo às proteínas possam de alguma forma estar envolvidos na fisiopatologia da X-ALD. Além disso, podemos presumir que, nos pacientes X-ALD assintomáticos estudados, o dano oxidativo e os aspectos inflamatórios desempenham papéis importantes na evolução e nas futuras manifestações do fenótipo neuronal. Também podemos supor que a administração de antioxidantes deve ser considerada como uma terapia adjuvante potencial para os pacientes assintomáticos e sintomáticos afetados pela X-ALD, inclusive para aqueles submetidos ao TCH. / Objective. We aimed to evaluate the role of hematopoietic stem cell transplantation (HSCT) and interleukin 6 (IL – 6) on various parameters of oxidative stress in X-linked adrenoleukodystrophy (X-ALD) patients. Methods. Malondialdehyde (MDA), sulfhydryl, carbonyl and hexacosanoic acid (C26:0) levels were measured in plasma from X-ALD patients before and after HSCT. And, MDA, carbonyl and IL-6 levels were measured in plasma and reduced glutathione (GSH) content was measured in erythrocytes from X-ALD patients with different phenotype (asymptomatic and childhood cerebral (CCER patients) at diagnosis moment. Results. We observed increased levels of MDA in plasma from X-ALD before and after HSCT compared to control group, but there was a significant reduction in MDA values after transplantation compared to levels found before the procedure. We verified a significant decrease in sulfhydryl content in plasma of X-ALD patients before HSCT compared with the control group and we also verified a significant increase in the levels of sulfhydryl content after HSCT. No significant differences were observed in carbonyl content in plasma of X-ALD before and after HSCT, compared to controls. However, we observed a significant reduction of plasma carbonyl content from X-ALD patients after HSCT compared to before HSCT. X-ALD patients presented a significant increase of C26:0 plasma level before HSCT when compared to controls and an important reduction of C26:0 plasma concentration in X-ALD patients after HSCT when compared to before HSCT C26:0 levels. We observed an inverse significant correlation between sulfhydryl content and plasma C26:0 levels of X-ALD individuals before HSCT. We also evidenced high levels of MDA and carbonyl formation in plasma from CCER and asymptomatic patients compared to controls. Still, we observed a significant decrease of GSH content in both groups tested compared to controls. The quantification of IL-6 is significantly higher in CCER patients, which is not observed in asymptomatic patients, despite these patients show a tendency of increased concentration of IL-6. Conclusions. The results obtained from plasma of X-ALD patients before and after HSCT demonstrate that this therapy, when well indicated and successful, has high effectiveness in reducing C26:0 plasma and is effective in reducing lipid peroxidation and oxidative damage to proteins in X-ALD patients. Still, it is possible to relate the accumulation of C26:0 and oxidative damage in the pathogenesis of X-ALD. Our data also suggest that lipid peroxidation and protein damage may somehow be involved in the pathophysiology of X-ALD. Moreover, we can assume that in our asymptomatic X-ALD patients, oxidative damage and inflammatory issues seem to play an important role in the evolution and future manifestations of neuronal phenotype. We can also assume that the administration of antioxidants should be considered as a potential adjuvant therapy for asymptomatic and symptomatic patients affected by X-ALD, including those that are submitted to HSCT.

Adrenoleucodistrofia

Estresse oxidativo

Radicais livres

Hematopoietic stem cell transplantation

Adrenoleukodystrophy

Oxidative stress

Free radicals

Lipid peroxidation

Protein damage

IL-6

Reduced glutathione.

Características fisiológicas e bioquímicas das bananeiras Prata , Japira e Vitória

Santos, Priscilla Nobres dos

22 February 2011

Made available in DSpace on 2016-12-23T13:48:27Z (GMT). No. of bitstreams: 1 Dissertacao de Priscilla Nobres dos Santos.pdf: 2094546 bytes, checksum: c80405345425c181dbb6a9991aee2f2a (MD5) Previous issue date: 2011-02-22 / Banana s culture in Brazil and in the state of Espírito Santo presents, in parts, an essential peculiar character, constituting an important source of income for small rural producers. Besides biotical factors, temperature and pluviousity are directly related to the banana tree s growing, because they provoke an effect upon the speed of most metabolic processes, influencing the vegetative cycle, the photosynthetic activity and the breathing activity. Therefore, this assignment has the purpose to evaluate the physiological and biochemical responses of banana trees grown in situ Prata (AAB), Japira (AAAB) and Vitória (AAAB) in two cycles of development stage Mother-plant and Child-plant. The results show that the photochemical behavior of the three cultivars leaves got very compromised in June, a month when temperatures are usually low. A smaller use of energy might have been caused by a bigger destabilization of the membranes, which, as a consequence, might have been determinant for obtaining a smaller rate of total chlorophylls. Among the cultivars analyzed, the physiological behavior of cultivar Prata were the less tolerant to the changes in the non-biotical factors. The cultivars Japira and Vitória presented similar physiological responses, which can be explained for its philogenetic proximity. The nutrients contents did not present significant differences between the months and the cultivars. However, they were pretty significant when ones check the fruit formation. The cultivars Japira and Vitória established, before harvest, a good chemical performance that possibly have favored the fruits formation / A bananicultura no Brasil e no estado do Espírito Santo apresenta, em parte, caráter essencialmente familiar, constituindo-se como uma importante fonte de renda para os pequenos produtores rurais. Além dos fatores bióticos, a temperatura e a pluviosidade são fatores relacionados diretamente com o crescimento da bananeira, pois exercerem efeito sobre a velocidade da maioria dos processos metabólicos, no ciclo vegetativo e na atividade fotossintética e respiratória. Dessa forma, este trabalho tem por objetivo avaliar as respostas fisiológicas e bioquímicas de bananeiras cultivadas in situ Prata (AAB), Japira (AAAB) e Vitória (AAAB) em dois do estádio do desenvolvimento (Planta-Mãe e Planta- Filha). Os resultados mostram que o desempenho fotoquímico das folhas das três cultivares ficou bastante comprometido no mês de junho, período caracterizado por temperaturas mais baixas. Um menor aproveitamento de energia pode ter sido causado por uma maior desestabilização das membranas, que, consequentemente, pode ter sido determinante para a obtenção de um menor índice de clorofilas totais. Das cultivares analisadas, a cv. Prata foi a que apresentou uma resposta fisiológica menos tolerante às alterações nos fatores abióticos. As cultivares Japira e Vitória apresentaram respostas fisiológicas bem semelhantes, o que pode ser explicado pela sua maior proximidade filogenética. Os teores de nutrientes não apresentaram diferenças significativas entre os meses e as cultivares. No entanto, em relação à formação do fruto foram bastante significativas. As cultivares Japira e Vitória estabeleceram, na fase pré-colheita, um bom rendimento químico que, possivelmente, favoreceu a formação dos frutos

Fluorescência da clorofila a

Pigmentos

Peroxidação lipídica

Nutrientes e póscolheita

Chlorophyll a fluorescence

Pigments

Lipid peroxidation

Nutrients and after harvest

Simulação dos produtos da oxidação lipídica em bicamadas

Paulista Neto, Antenor José

January 2015

Orientador: Prof. Dr. Rodrigo Maghdissian Cordeiro / Dissertação (mestrado) - Universidade Federal do ABC, Programa de Pós-Graduação em Ciência & Tecnologia - Química, 2015. / Os componentes lipídicos das membranas celulares são substratos comuns de ataque oxidativo. Durante uma oxidação não-enzimática, tanto os fosfolipídios quanto o colesterol podem reagir com moléculas de 1O2 geradas fotodinamicamente via adição ene, produzindo hidroperóxidos de fosfolipídios e colesterol, respectivamente. Os efeitos citotóxicos e apoptóticos desses hidroperóxidos estão relacionados com a sua influência sobre as propriedades biofísicas das membranas fosfolipídicas, assim como na sua habilidade em disseminar o stress oxidativo. Estas habilidades relacionam-se fortemente com a estrutura química destes hidroperóxidos. Contudo, os mecanismos moleculares subjacentes ainda não estão bem compreendidos. Aqui, foram realizadas simulações de dinâmica molecular de diferentes produtos da oxidação dos fosfolipídios e hidroperóxidos de colesterol em bicamadas de fosfatidilcolina monoinsaturadas. O efeito combinado da peroxidação do colesterol e fosfolipídio também foi investigado. Depois da oxidação, tanto o núcleo rígido de esterol quanto as cadeias acila sn-2 dos fosfolipídios reorientam-se e os grupos hidrofílicos inseridos formam ligações de hidrogênio com os grupos carboniléster dos fosfolipídios. Para o colesterol, esta reorientação provocou a perda das propriedades de condensação e ordenação, com possíveis implicações à formação de domínios laterais na membrana. No caso dos radicais peroxila de colesterol, pequenas mudanças na orientação foram observadas dependendo da posição dos grupos -OO no núcleo de esterol. As possíveis implicações para as habilidades do radical propagar a reação em cadeia foram discutidas. / Lipid components of cell membranes are common substrates for oxidative attack. During a non-enzymatic oxidation, both phospholipids as well as cholesterol molecules can react with photodynamically generated 1O2 via ene addition, producing phospholipids and cholesterol hydroperoxides, respectively. The cytotoxic and apoptotic effects of these hydroperoxides are related to their influence on the biophysical properties of phospholipid membranes, as well as their ability to disseminate oxidative stress. These abilities relate strongly to the chemical structure of these hydroperoxides. However, the underlying molecular mechanisms are not well understood. Here, molecular dynamics simulations of different oxidation products of phospholipids and cholesterol hydroperoxides in monounsaturated phosphatidylcholine bilayers have been performed. The combined effect of phospholipid and cholesterol peroxidation was also investigated. After oxidation, both the rigid ring sterol and the sn-2 acyl chains of the phospholipids tilt themselves and the inserted hydrophilic groups form h-bonds with carbonylester groups of phospholipids. For cholesterol, this tilting caused the loss of condensation and ordering properties, with possible implications for the formation of lateral domains in the membrane. In the case of cholesterol peroxyl radicals, small changes in orientation were observed depending on the position of -OO groups in the sterol ring. The possible implications for the radical skill to propagate the chain reaction were discussed.

PEROXIDAÇÃO LIPÍDICA

STRESS OXIDATIVO

SIMULAÇÕES DE DINÂMICA MOLECULAR

LIPID PEROXIDATION

MOLECULAR DYNAMICS SIMULATIONS

OXIDATIVE STRESS

QUANTIFICAÇÃO DE α-TOCOFEROL, RETINOL E CAROTENÓIDES E SEUS POSSÍVEIS EFEITOS SOBRE A PEROXIDAÇÃO LIPÍDICA EM TRABALHADORES EXPOSTOS A SOLVENTES / QUANTIFICATION OF α-TOCOPHEROL, RETINOL E CAROTENOIDS AND THEIR POSSIBLES EFFECTS ON LIPID PEROXIDATION IN WORKERS EXPOSED TO SOLVENTS

Charão, Mariele Feiffer

18 February 2011

Coordenação de Aperfeiçoamento de Pessoal de Nível Superior / Oxidative stress is a process characterized by the antioxidant defense system decrease and/or an excessive reactive species (RS) production. RS are substances capable of attacking proteins, lipids and DNA. The oxidative damage caused to lipids is known as lipid peroxidation, which leads to the increase of malondialdehyde (MDA) levels. Oxidative stress is involved in the pathogenesis of many chronic diseases, including diabetes, cancer, Parkinson s disease and damaged tissue in exposed to chemical agents, such as neurotoxicity, hematotoxicity and nefrotoxicity. It is known that there is a close relation between organic solvents, present in paints, and oxidative stress. Thus, the body has an elaborate antioxidant defense system, the exogenous antioxidants, such as lipid soluble vitamins, and the endogenous system, such as antioxidant enzymes. In this study a method has been validated and optimized for simultaneous quantification of retinol, α-tocopherol, lycopene and β- carotene using high performance liquid chromatography (HPLC-UV/fluorescence). The analytical parameters of validation analyzed were linearity, precision, accuracy, recovery and limits of detection (LOD) and quantification (LOQ). For all the vitamins analyzed, the linear regression coefficients were > 0.99, CV% < 5%;% bias < ± 6% recovery > 92% and the LOD and LOQ values obtained were satisfactory for routine clinical application for all analytes. The validated method was applied to a group of occupationally exposed to paints (n = 45) and a non-exposed group (control group, n = 30). The results indicated that all vitamins, except vitamin E, were significantly lower in the exposed group. Moreover, the possible correlation between endogenous and exogenous antioxidants and lipid damage was evaluated. Quantifications were done to assess endogenous antioxidants, reduced glutathione (GSH) in erythrocytes, the enzymes superoxide dismutase (SOD) and catalase (CAT) in whole blood through spectroscopic methods, and malondialdehyde (MDA) levels in plasma through HPLC-VIS in both study groups, exposed (n=42) and controls (n=28). The biological monitoring was performed by measurement of blood toluene, since in previous studies, it was suggested that this solvent would be the major inducer of lipid peroxidation. Despite the low levels of toluene found, exposed workers presented higher levels of MDA and the antioxidant enzymes (SOD and CAT) activities were significantly elevated when compared with the control group; and this increase was accompanied by depletion of GSH levels. Also, several correlations were observed between MDA and the enzymatic (SOD and CAT) and non-enzymatic antioxidants (GSH), and with lipid-soluble vitamins as well, except vitamin E. Through statistical tests the antioxidants which have a greater influence on the levels of MDA were evaluated. Among the antioxidants tested, GSH and carotenoids (mainly β- carotene) were suggested as main responsible for the reduction of lipid peroxidation. Thus, it can be suggested that high intakes of exogenous antioxidants, such as carotenoids,, tend to decrease lipid damage in occupationally exposed individuals to solvents constituent of paints. / O estresse oxidativo é um processo caracterizado pela diminuição do sistema de defesa antioxidante e/ou por uma produção excessiva de espécies reativas (ERs). As ERs são substâncias capazes de lesar proteínas, lipídios e DNA. Quando os lipídios são atingidos ocorre um processo chamado de peroxidação lipídica que leva ao aumento nos níveis de malondialdeído (MDA). O estresse oxidativo está envolvido com a patogênese de muitas doenças crônicas, como diabetes, câncer, doença de Parkinson e em danos teciduais em expostos a agentes químicos, como neurotoxicidade, hematotoxicidade e nefrotoxicidade. Sabe-se que existe uma estreita relação entre os solventes orgânicos, presentes em tintas, e o estresse oxidativo. Diante disso, o organismo dispõe de um elaborado sistema de defesa antioxidante, os antioxidantes exógenos, como as vitaminas lipossolúveis e o sistema endógeno como enzimas antioxidantes. Dessa forma, nesse estudo foi primeiramente otimizada e validada metodologia para simultânea quantificação de antioxidantes exógenos: retinol, α-tocoferol, licopeno e β-caroteno, utilizando cromatografia líquida de alta eficiência (CLAE-VIS/fluorescência). Os parâmetros analíticos de validação analisados foram linearidade, precisão, exatidão, recuperação e limites de detecção (LD) e quantificação (LQ). Para todas as vitaminas analisadas, os coeficientes de regressão linear foram > 0,99; CV% < 5%; bias% < ± 6%; recuperação > 92% e os valores de LD e LQ obtidos foram satisfatórios para aplicação na rotina clínica. O método validado foi aplicado em um grupo de expostos ocupacionalmente a tintas (n=45) e um grupo de não expostos (controle, n=30). Os resultados indicaram que todas as vitaminas, exceto a vitamina E, foram significativamente menores no grupo exposto. Além disso, avaliou-se o possível efeito protetivo de antioxidantes exógenos e endógenos sobre o dano lipídico. Foram realizadas as dosagens dos antioxidantes endógenos, glutationa reduzida (GSH) em eritrócitos, das enzimas superóxido dismutase (SOD) e catalase (CAT) em sangue total por métodos espectrofotométricos e os níveis de malondialdeído (MDA) em plasma por CLAE-VIS nos dois grupos de estudo, expostos (n=42) e controles (n=28). A monitorização biológica foi realizada através da dosagem de tolueno sanguíneo, uma vez que, em trabalhos prévios, foi sugerido que este solvente seria o principal indutor de peroxidação lipídica. Apesar dos baixos níveis de tolueno sanguíneo encontrados, os trabalhadores expostos apresentaram níveis de MDA e atividade das enzimas antioxidantes (SOD e CAT) significativamente elevados, quando comparados com o grupo controle e esse aumento foi acompanhado de depleção nos níveis de GSH. Ainda, foram observadas várias correlações entre os níveis de MDA e os antioxidantes endógenos enzimáticos (SOD e CAT) e não enzimático (GSH) e ainda com as vitaminas lipossolúveis, exceto vitamina E. Através de testes estatísticos foram avaliados quais antioxidantes teriam uma maior influência nos níveis de MDA. Dentre os antioxidantes analisados, a GSH e os carotenóides (principalmente o β- caroteno) foram sugeridos como principais responsáveis pela redução da peroxidação lipídica. Com isso, pode-se sugerir que aumento nos níveis de carotenóides, via dieta, tendem a diminuir o dano lipídico em indivíduos ocupacionalmente expostos a solventes constituintes de tintas.

Vitaminas lipossolúveis

Exposição ocupacional

Peroxidação lipídica

Estresse oxidativo

Antioxidantes

Lipid-soluble vitamins

Occupational exposure

Lipid peroxidation

Oxidative stress

Antioxidants

CNPQ::CIENCIAS BIOLOGICAS::FARMACOLOGIA

Parâmetros de estresse oxidativo no sangue, fígado e rins de ratos diabéticos tratados com curcumina e/ou insulina / Oxidative stress parameters in blood, liver and kidney of diabetic rats treated with curcumin and / or insulin

Palma, Heloisa Einloft

01 March 2013

Diabetes mellitus (DM) is an important health problem that affects worldwide human population and is commonly observed in small animal clinics. Many studies show that hyperglycemia is the pivotal cause of DM complications, including cataract, nephropathy and neuropathy. Hyperglycemia leads to generation of reactive oxygen species (ROS) and increases oxidative damage of lipids, DNA and proteins in many tissues. Oxidative stress is increased in cells in response to a depletion of antioxidant enzymes, superoxide dismutase (SOD) and catalase (CAT) that scavenge oxygen reactive species. Curcumin is the main component of Curcuma longa and has been used traditionally as an antidiabetic agent; and there are evidences that this substance presents high activity of ROS scavenger. Considering that diet is part of diabetic state treatment and that curcumin is considered and antioxidant agent, this study aimed to evaluate the effects of curcumin and/or insulin on oxidative stress parameters in streptozotocin-induced diabetic rats. In addition, it was performed a histopathological analysis of the liver and kidney of healthy and diabetic rats treated with these compounds. For this, the animals were divided into six groups, with six animals each: Control (C); Control/Curcumin (CCur); Diabetic/Saline (D); Diabetic/Insulin (DIns); Diabetic/Curcumin (DCur), and Diabetic/Insulin/Curcumin (DInsCur). Curcumin was diluted in corn oil and administered at the dosage of 60mg/kg once a day and insulin was administered twice a day, at the dosage of 1.5IU/rat in the morning and 2.5IU/rat in the afternoon, for a period of 30 days. In groups D and DCur, the histological analysis of the liver revealed elevated number of binucleated hepatocytes and alterations in hepatic trabeculae. In kidney there were vacuolization of tubular cells, glomerular congestion and mononuclear inflammatory focus. The treatment with insulin ameliorate renal and hepatic lesions from both DIns and DInsCur groups. Thiobarbituric acid reactive substances (TBARS) levels were increased in serum of D and DInsCur groups and in hepatic and renal tissue of group D (P<0.05). CAT activity was low in liver and kidney of groups D, DIns and DCur; there was significant increase in kidney of DInsCur group; in blood, catalase activity was high in groups D and DInsCur (P<0.05). SOD activity in blood was decreased in groups D and DInsCur and increased in groups DIns and DCur (P<0.05). In liver, SOD activity was increased in groups D and DInsCur. Delta aminolevulinic acid dehydratase (δ-ALA-D) activity was reduced in liver and kidney of group D and treatment with insulin and/or curcumin prevented the decrease of the activity in hepatic tissue from groups DIns, DInsCur and DCur, and renal tissue from groups DCur and DInsCur. Thus, treatments with curcumin or insulin prevented oxidative stress in blood of diabetic rats, through modulation of antioxidant defenses. Regarding lipid peroxidation, both substances presented positive effect in serum, liver and kidney, except in serum from group DInsCur, revealing a negative effect when curcumin and insulin were associated. With this experiment, it was possible to demonstrate the importance of insulin as primary treatment of DM, once this drug prevented cell damage in organs analyzed by histopathology. Furthermore, this study contributed to comprehend that antioxidants from medicinal plants, such as curcumin, can be used as adjuvant in treatment of this endocrinopathy and not as a single therapy. / O diabetes mellitus (DM) é um importante problema de saúde que afeta a população humana e é comumente observada na clínica de pequenos animais. Diversos estudos relatam que a hiperglicemia é a principal causa das complicações do DM, tais como catarata, nefropatia e neuropatia. A hiperglicemia causa a geração de espécies reativas de oxigênio (EROs) e aumenta o dano oxidativo de lipídios, DNA e proteínas em diversos tecidos. O estresse oxidativo está aumentado nas células como resultado da depleção de enzimas antioxidantes, especialmente a superóxido dismutase (SOD) e catalase (CAT) removedoras de EROs. A curcumina é o principal componente da Curcuma longa e tem sido usada tradicionalmente como antidiabético e há evidências científicas que esse composto apresenta uma alta atividade antioxidante. Considerando que a dieta faz parte do tratamento do paciente diabético e que a curcumina é um agente antioxidante, este estudo teve como objetivo avaliar os efeitos desse composto, associado ou não à insulinoterapia, sobre os parâmetros de estresse oxidativo em ratos diabéticos induzidos com estreptozotocina. Em adição, também foi avaliada a histopatologia do fígado e rim dos ratos sadios e diabéticos tratados com estes compostos. Para isso, os ratos foram distribuídos em seis grupos, cada um com seis animais: grupo controle (C), grupo controle curcumina (CCur), grupo diabético (D), grupo diabético curcumina (DCur), grupo diabético insulina (DIns) e grupo diabético insulina e curcumina (DInsCur). A curcumina foi diluída em óleo de milho e administrada na dose de 60mg/kg, uma vez ao dia e a insulina aplicada a cada 12 horas nas doses de 1,5UI/rato pela manhã e 2,5UI/rato à tarde por um período de 30 dias. Nos grupos D e DCur, a análise histológica do fígado mostrou número elevado de hepatócitos binucleados e alterações nas trabéculas. Nos rins, havia vacuolização das células tubulares, congestão glomerular e focos inflamatórios mononucleares. O tratamento com insulina reduziu as lesões renais e hepáticas dos grupos DIns e DInsCur. Os níveis de substâncias reativas ao ácido tiobarbitúrico (TBARS) apresentaram-se elevados no soro dos grupos D e DInsCur e nos tecidos hepático e renal do grupo D (P<0,05). A atividade da CAT foi baixa no fígado e rins dos grupos D, DIns and DCur; também houve um aumento significativo na atividade desta enzima nos rins do grupo DInsCur. Já no sangue, a atividade da CAT foi alta nos grupos D e DInsCur (P<0,05). A atividade da SOD no sangue estava reduzida nos grupos D e DInsCur e aumentada nos grupos DIns e DCur (P<0,05), já no fígado, a atividade da SOD estava aumentada nos grupos D e DInsCur. A atividade da enzima delta-aminolevulinato desidratase (δ-ALA-D) estava reduzida no fígado e rins do grupo D e o tratamento com insulina e/ou curcumina preveniu a redução da sua atividade no tecido hepático dos grupos DIns, DInsCur e DCur e no tecido renal dos grupos DCur e DInsCur. Dessa forma, observa-se que o tratamento com curcumina ou insulina preveniu o estresse oxidativo no sangue dos ratos diabéticos, através da modulação das defesa antioxidantes enzimáticas. Em relação à peroxidação lipídica, ambas substâncias apresentaram efeito benéfico no soro, fígado e rins, com exceção do soro do grupo DInsCur, revelando um efeito negativo quando a curcumina e a insulina foram associadas. Com esta investigação, foi possível demonstrar a importância do uso da insulina como tratamento de eleição do DM, visto que este fármaco foi capaz de prevenir danos celulares nos órgãos avaliados histologicamente. Além disso, este estudo contribuiu para a compreensão de que antioxidantes provenientes de plantas medicinais, como a curcumina, podem ser utilizados como adjuvantes no tratamento desta endocrinopatia e não como terapia isolada.

Diabetes mellitus

Catalase

Superóxido dismutase

Peroxidação lipídica

Insulina

Curcumina

δ-ALA-D

Diabetes mellitus

Catalase

Superoxide dismutase

Lipid peroxidation

Insulin

Curcumin