ABSTRACT
Purpose: Fluorescence spectroscopy techniques have been investigated aiming to reduce the invasiveness of methods for investigation of tissue. In transplantation procedures, it may offer the possibility of a complementary technique for the monitoring of liver grafts' conditions prior to and during the transplantation procedure stages involving cold perfusion. The objective of this study was to evaluate fluorescence spectroscopy under violet light excitation (408 nm) for the monitoring of clinical hypothermic liver transplantation procedures. Methods: Organ grafts were monitored from before the removal of the donor's body to 1 h after the implant into the receptor's body. Fluorescence spectroscopy was assessed over five stages within these transplant stages. Results: The study provided evidence of a correlation between fluorescence information collected during liver grafts transplantation and the survival of patients. Conclusions: Fluorescence spectroscopy can become a tool to monitor transplantation grafts, providing objective information for the final decision of surgeons to use organs.
Subject(s)
Humans , Spectrometry, Fluorescence/methods , Ultraviolet Rays , Liver Transplantation/rehabilitationABSTRACT
The purpose of the study was to evaluate the antibacterial effect of protoporphyrin IX (PpIX) generated by the exogenous administration of 5-aminolevulinic acid or δ-ALA and activated with an argon laser over a planktonic and biofilm of Enterococcus faecalis (E. faecalis) as a pharmacological therapy alternative. A planktonic strain of E. faecalis was cultured with a solution of ∂-ALA (40 µg/mL)-thioglycolate solution for 13 min, and a biofilm of E. faecalis was cultured in a δ-ALA (80 µg/mL)-thioglycolate solution for 13 min. Then, both were irradiated with an argon laser. Finally, the antibacterial effect was evaluated by counting the CFU in planktonic form, and a LIVE/DEAD viability cell test. The production and accumulation of PpIX from exogenously administered δ-ALA on E. faecalis in planktonic and biofilm forms was confirmed by spectrofluorometry. The irradiation of PpIX with an argon laser produced an antibacterial effect on E. faecalis in planktonic and biofilm form, even without biofilm disruption, at a concentration of 40 µg/mL and 80 µg/mL of δ-ALA, respectively. The exogenous administration of δ-ALA in combination with laser irradiation on planktonic and biofilm forms of E. faecalis produces an effective antibacterial effect as complement or alternative to pharmacological therapies
Subject(s)
Protoporphyrins/adverse effects , Enterococcus faecalis/classification , Photochemotherapy/methods , Spectrometry, Fluorescence/methods , Cells , Biofilms , Drug Therapy , Aminolevulinic Acid/administration & dosageABSTRACT
Objective: To investigate the antifungal potential of A. colubrina, and its phytochemical characteristics, thermal profile and toxicity. Material and Methods: To assess potential antifungal activity, the technique of microdilution was used with the determination of the Minimum Inhibitory Concentration and Minimum Fungicidal Concentration, using standard species of Candida and recent clinical isolates of Candida albicans. Analyses of action of the extract were performed on the wall and cell morphology of C. albicans, of the interactive effect between the plant extract and nystatin on C. albicans through the checkerboard method, and of growth kinetics. The phytochemical screening was determined by spectrophotometry. The thermal profile was traced with the determination of thermogravimetric curves (TG) and differential scanning calorimetry (DSC). The toxicity was evaluated by the method of hemolysis. Results: The extract of A. colubrina showed a fungistatic potential against all bacteria tested and it acted by modifying the cellular morphology of C. albicans. There was a synergism between nystatin and the plant extract (FIC=0.375), and 53.18% of total polyphenols were determined. The TG curve showed the occurrence of three steps of thermal decomposition. None of the tested concentrations became the effective cytotoxic concentration. Conclusion: Further studies should be conducted to understand the efficacy and the mechanisms of action involved in the antifungal activity of the plant extract of A. colubrina in order to produce a new drug for the treatment of oral candidiasis.
Subject(s)
Antifungal Agents , Candida albicans/immunology , Plant Extracts , Plants, Medicinal , Anti-Infective Agents , Brazil , Spectrometry, Fluorescence/methodsABSTRACT
A obesidade e a síndrome metabólica têm aumentado em proporções preocupantes em nível mundial. Além das consequências sistêmicas, a obesidade e suas comorbidades também têm sido relacionadas com a condição bucal. O objetivo deste estudo foi identificar a progressão de lesões cariosas, presença de biofilme dentário, fluxo salivar e presença de saburra lingual em indivíduos eutróficos, sendo avaliados em dois momentos e portadores de síndrome metabólica antes e após a cirurgia bariátrica. A amostra foi constituída por 150 indivíduos, divididos em dois grupos: grupo controle (GC: 75) e grupo obeso (GO: 75), ambos avaliados em T0 e T1, sendo GC 6 meses após a primeira avaliação e GO 6 meses após a cirurgia bariátrica. A avaliação antropométrica dos indivíduos foi realizada por meio do IMC e circunferência da cintura. Os índices ICDAS II e CPOD foram utilizados para avaliar a progressão da cárie dentária. O método de fluorescência verde (QLF- Quantitative Light-induced Fluorescence) avaliou a perda mineral nas superfícies lisas dos dentes e presença de biofilme dentário. O fluxo salivar estimulado foi avaliado em mL/min. O Índice de Saburra Lingual foi utilizado para a avaliação da presença de saburra na língua. Para análise estatística, utilizou-se os testes Qui Quadrado, Exato de Fisher, Mann-Whitney, Kruskal-Wallis e Regressão Logística Múltipla, adotando nível de significância de 5%. Os resultados mostraram que houve diferença significativas entre os grupos, GC apresentou maior número de dentes hígidos (p=0,038) e dentes sem alteração no esmalte (p=0,005) quando comparado ao GO. Ao comparar GC e GO no T1, verificou-se que houve diferença significativa em relação ao CPOD (p<0,0001), dentes restaurados (p<0,0001) e área da lesão (Ws) (p=0,045), sendo as piores condições encontradas encontradas em GO. Observou-se que houve diferença significativa entre a perda mineral e quantidade de biofilme dentário por fluorescência entre os grupos, mas não entre T0 e T1. Diante dos resultados, podese concluir que indivíduos portadores de síndrome metabólica, comparado com os eutróficos, apresentam maior número de lesões cariosas antes e após a cirurgia bariátrica. No presente estudo a cirurgia bariátrica não interferiu na progressão das lesões cariosas, todavia, destaca-se a necessidade de abordagem multiprofissional e contínua, atuando na prevenção de doenças e atenção odontológica.(AU)
Obesity and the metabolic syndrome have increased in alarming proportions at world level. Apart from systemic consequences, obesity and its comorbidities have also been related to the oral condition. The aim of this study was to identify the caries lesion progression, presence of dental biofilm, the salivary flow and tongue coating in eutrophic individuals, being evaluated in two moments and individuals with metabolic syndrome before and after undergoing bariatric surgery. The sample consisted of 150 individuals divided into two groups: Control Group (CG: 75) and Obese Group (OG): 75, both evaluated in T0 and T1; CG being evaluated six months after T0, and EG, 6 months after bariatric surgery. Anthropometric assessment of individuals was made by means of BMI and waist circumference measurement. The ICDAS II and DMFT indices were used for evaluating the progression of dental caries. The Quantitative Light-induced Fluorescence (QLF) method, for evaluating mineral loss on the smooth tooth surfaces and the presence for dental biofilm. The stimulated salivary flow was evaluated in mL/min. The Winkel tongue coating index (WTCI) was used to evaluate the presence of tongue coating. For statistical analysis, the Chi- Square, Fishers Exact, Kruskal-Wallis and Multiple Logistic Regression tests were used, adopting a significance level of 5%. The results showed statistical difference between the groups: CG presented a higher; number of healthy teeth (p=0.038) and teeth without changes in enamel (p=0.005) when compared to OG. When comparing CG and EG after the second evaluation (T1), statistically significant difference was verified in relation to DMFT (p<0.0001), restored teeth (p<0.0001) and lesion area (Ws) (p=0.045), being the worst conditions found in OG. It was observed that there was a significant difference between mineral loss and the quantity dental biofilm by fluorescence between groups, but not between T0 and T1. In view of the results, the authors concluded that patients with metabolic syndrome, compared to eutrophic, have a higher number of caries lesions before and after bariatric surgery. In the present study, bariatric surgery did not influence in caries lesion progression, however, highlights the necessity to a continuous multi professional approach to acting in the prevention of diseases and dental care.(AU)
Subject(s)
Humans , Male , Female , Adolescent , Adult , Middle Aged , Aged , Bariatric Surgery , Dental Caries/etiology , Dental Plaque/etiology , Metabolic Syndrome/complications , Obesity/complications , Obesity/surgery , Anthropometry , Biofilms , Case-Control Studies , Dental Caries/physiopathology , Dental Plaque/physiopathology , Metabolic Syndrome/physiopathology , Obesity/physiopathology , Prospective Studies , Spectrometry, Fluorescence/methods , Treatment OutcomeABSTRACT
A escala 3D-Master foi desenvolvida com a finalidade de satisfazer as maiores exigências estéticas dos pacientes, por possuir uma maior quantidade de tonalidades em relação às demais escalas. Contudo, possui uma técnica específica para a sua correta utilização, desconhecida por grande parte dos profissionais. O objetivo desse trabalho foi avaliar se, após o aprendizado da técnica correta de utilização da escala de cor VITA 3D-Master, recomendada pelo fabricante (VITA® Zahnfabrik, Alemanha), os profissionais da área de odontologia conseguem utilizá-la de forma adequada, atingindo o objetivo desejado que é a correta seleção de cor dos dentes. Para isso, foram utilizados seis elementos dentários de face vestibular hígida extraídos e doados pelos pacientes ao banco de dentes da faculdade. O terço médio da face vestibular de cada dente foi escolhido para a seleção de cor feita pelo espectrofotômetro digital VITA EasyShade programado para a escala VITA 3D-Master. Trinta e sete acadêmicos do último ano do curso de odontologia fizeram a seleção pelo método visual dos mesmos elementos dentários. Após a primeira seleção, uma palestra de 3 horas de duração foi ministrada por um técnico de prótese dental, ceramista e consultor da VITA®. Após essas orientações, os mesmos acadêmicos realizaram uma segunda seleção de cor com os mesmos elementos dentários, utilizando a técnica de seleção de cor da escala VITA 3D-Master. A técnica preconizada pela VITA® para a correta utilização da escala VITA 3D-Master impactou positivamente no resultado da segunda fase da pesquisa para a seleção de cor.
The 3D-Master shade guide was developed in order to meet higher patientsÆ aesthetic requirements as it has a greater number of shades when compared to other shade guides. However, a specific technique is needed for its correct use, which is unknown by most of professionals. The aim of this study was to evaluate if after learning the VITA 3D-Master shade guide correct technique use, recommended by the manufacturer (VITA® Zahnfabrik, Germany), dentistry professionals can use it properly, reaching the desired goal that is the correct selection of tooth color. For this, we used six extracted teeth of higid vestibular surface donated by patients to the university teeth bank. The middle third of the vestibular surface of each tooth was chosen for the color selection made by the digital spectrophotometer VITA Easyshade programmed for VITA 3D-Master shade guide. Thirty-seven students from the last year of the odontology course made the selection through the visual method in the same teeth. After the first selection, a 3 hours lecture was held by a qualified dental prosthetist, ceramist and VITA® consultant. After these guidelines, the same students performed a second color selection with the same teeth, using the VITA 3D-Master shade guide color selection technique. The technique recommended by VITA® for the correct use of VITA 3D-Master shade guide positively affected the outcome of the second phase of the research for color selection.
Subject(s)
Color Perception , Esthetics, Dental , Students, Dental , Brazil , Spectrometry, Fluorescence/methods , Cross-Sectional Studies/methodsABSTRACT
Autofluorescence exhibited by tissues often interferes with immunofluorescence. Using imaging and spectral analysis, we observed remarkable reduction of autofluorescence of formalin fixed paraffin embedded tissues irradiated with light prior to incubation with immunofluorescent dyes. The technique of photobleaching offers significant improvement in the quality and specificity of immunofluorescence. This has the potential for better techniques for disease diagnosis.
Subject(s)
Antibodies, Antinuclear/diagnosis , Fluorescent Antibody Technique/methods , Lung/cytology , /methods , Photobleaching , Spectrometry, Fluorescence/methodsABSTRACT
Background: Sudden cardiac death (SCD) is a sudden unexpected event, from a cardiac cause, that occurs in less than one hour after the symptoms onset, in a person without any previous condition that would seem fatal or who was seen without any symptoms 24 hours before found dead. Although it is a relatively frequent event, there are only few reliable data in underdeveloped countries. Objective: We aimed to describe the features of SCD in Ribeirão Preto, Brazil (600,000 residents) according to Coroners’ Office autopsy reports. Methods: We retrospectively reviewed 4501 autopsy reports between 2006 and 2010, to identify cases of SCD. Specific cause of death as well as demographic information, date, location and time of the event, comorbidities and whether cardiopulmonary resuscitation (CPR) was attempted were collected. Results: We identified 899 cases of SCD (20%); the rate was 30/100000 residents per year. The vast majority of cases of SCD involved a coronary artery disease (CAD) (64%) and occurred in men (67%), between the 6th and the 7th decades of life. Most events occurred during the morning in the home setting (53.3%) and CPR was attempted in almost half of victims (49.7%). The most prevalent comorbidity was systemic hypertension (57.3%). Chagas’ disease was present in 49 cases (5.5%). Conclusion: The majority of victims of SCD were men, in their sixties and seventies and the main cause of death was CAD. Chagas’ disease, an important public health problem in Latin America, was found in about 5.5% of the cases. .
Fundamento: Morte súbita cardíaca (MSC) é um evento súbito e inesperado, de causa cardiovascular, que ocorre em menos de uma hora após o início dos sintomas, em indivíduo sem qualquer condição clínica prévia potencialmente fatal ou assintomático nas últimas 24 horas antes do óbito, em caso de morte não testemunhada. Apesar de ser um evento relativamente frequente, há poucos dados confiáveis na literatura sobre países em desenvolvimento. Objetivo: Descrever as características da MSC em Ribeirão Preto (SP 600.000 habitantes) baseando-se nos relatórios de autopsias do Serviço de Verificação de Óbitos do Interior. Métodos: Foram revisados retrospectivamente 4.501 relatórios de autopsias entre 2006 e 2010, para identificar casos de MSC. Foram coletados dados como causa específica do óbito, características demográficas e comorbidades das vítimas, data, local e hora do evento, e se foram realizadas manobras de ressuscitação cardiopulmonar (RCP). Resultados: Foram identificados 899 casos de MSC (20%; razão 30/100.000 habitantes por ano). A principal causa de MSC foi doença arterial coronariana (DAC - 64%), acometendo homens (67%) entre a sexta e a sétima década de vida. A maior parte dos eventos ocorreu durante a manhã, no domicílio (53,3%), e a RCP foi realizada em quase metade das vítimas (49,7%). A comorbidade mais prevalente foi hipertensão arterial sistêmica (57,3%). Doença de Chagas foi detectada em 49 casos (5,5%). Conclusão: A maioria dos casos de MSC ocorreu por DAC em homens entre a sexta e a sétima década de vida. Doença de Chagas, um importante problema de saúde pública na América Latina, foi detectada em 5,5% dos casos. .
Subject(s)
Humans , Drug Evaluation, Preclinical/methods , Enzyme Inhibitors/pharmacology , Oligonucleotides/metabolism , Phosphoric Diester Hydrolases/metabolism , Spectrometry, Fluorescence/methods , Base Sequence , Cost-Benefit Analysis , Drug Evaluation, Preclinical/economics , High-Throughput Screening Assays , Kinetics , Mutation , Oligonucleotides/genetics , Phosphoric Diester Hydrolases/genetics , Spectrometry, Fluorescence/economicsABSTRACT
Aim: To evaluate the performance of a pen‑type laser fluorescence device (DIAGNOdent 2190; LFpen, KaVo, Germany) and bitewing radiographs (BW) for approximal caries detection in permanent and primary teeth. Materials and Methods: A total of 246 anterior approximal surfaces (102 permanent and 144 primary) were selected. Contact points were simulated using sound teeth. Two examiners assessed all approximal surfaces using LFpen and BW. The teeth were histologically assessed for the reference standard. Optimal cut‑off limits were calculated for LFpen for primary and permanent teeth. Sensitivity, specificity, accuracy and area under the receiver operating characteristic curve (Az) were calculated for D1 (enamel and dentin lesions) and D3 (dentin lesions) thresholds. The reproducibility was assessed by intraclass correlation coefficient (ICC) and Cohen’s weighted kappa values. Results: For permanent teeth, the LFpen cut‑off were 0–27 (sound), 28–33 (enamel caries) and >33 (dentin caries). For primary teeth, the LFpen cut‑off were 0–7 (sound), 8–32 (enamel caries) and >32 (dentin caries). The LFpen presented higher sensitivity values than BW for primary teeth (0.58 vs. 0.32 at D1 and 0.80 vs. 0.47 at D3) and permanent teeth (0.80 vs. 0.57 at D1 and 0.94 vs. 0.51 at D3). Specificity did not show a significant difference between the methods. Rank correlations with histology were 0.59 and 0.83 (LFpen) and 0.36 and 0.70 (BW) for primary and permanent teeth, respectively, considering all lesions. ICC values for LFpen were 0.71 (inter) and 0.86 (intra) for permanent teeth and 0.94 (inter) and 0.90/0.99 for primary teeth. Kappa values for BW were 0.69 (inter) and 0.68/0.90 (intra) for permanent teeth and 0.64 (inter) and 0.89/0.89 for primary teeth. Conclusion: LFpen presented better reproducibility for primary and permanent teeth and higher accuracy in detecting caries lesions at D1 threshold than BW for permanent teeth. LFpen should be used as an adjunct method for approximal caries detection.
Subject(s)
Dental Caries/diagnosis , Dental Caries/diagnostic imaging , Lasers/methods , Radiography, Dental, Digital/methods , Spectrometry, Fluorescence/methodsABSTRACT
Introducción: la proteasa aspártica secretada (Sap) es considerada un factor de virulencia en el proceso de infección por Candida albicans. La frecuencia de candidiasis a nivel mundial aumenta cada día, razón por la cual se hace necesario encontrar nuevos medicamentos que combatan esta enfermedad, al mismo tiempo desarrollar métodos que evalúen en forma rápida compuestos inhibidores de Sap. Objetivo: estandarizar un método fluorescente para identificar la inhibición de actividad de Sap. Métodos: se indujo la producción de Sap en cultivos de C. albicans según la metodología descrita por Capobiancoy se evaluaron sus niveles por electroforesis en geles SDS-PAGE en diferentes lapsos de tiempos. La actividad de Sap fue verificada por espectrofluorometría, para lo cual se determinaron las condiciones de reacción, variando las concentraciones de cobre y fluorexon, y los resultados de inhibición, se expresaron como disminución en la señal de fluorescencia. Como control de inhibición de Sap se utilizó Pepstatin A y como control positivo de actividad proteasa se utilizó pancreatina. Resultados: se establecieron concentraciones de 5,5 y 5,0 µM para fluorexon y cobre respectivamente; el tiempo óptimo de acoplamiento de estos fue de 120 min y la mayor actividad de Sap se alcanzó a las 22 h de incubación. Conclusiones: las condiciones estandarizadas para el método espectrofluorométrico, permiten confirmar la inhibición de Sap por Pepstatin A y demostrar que es un método viable para evaluar inhibidores de esta proteasa(AU)
Introduction: the Secreted Aspartyl Protease (Sap) is considered a virulence factor in the infection process caused by Candida albicans. The frequency of candidiasis worldwide is increasing, hence the need for finding new drugs to fight this illness and also a quick and economic evaluation and screening methods to identify some Sap inhibition agents. Objective: to standardize fluorescent method for identifying the Sap activity inhibition. Methods: Sap production was induced in C. albicans cultures following the methodology described by Capobianco, their levels were evaluated by electrophoresis on SDS-PAGE gels at different periods of time. Sap activity was checked by spectrofluorometry, for which the reaction conditions were determined, varying the concentrations of copper and fluorexon, and the inhibition results were expressed as decreased fluorescence signal. Pepstatin A served as Sap inhibition control whereas pancreatin was the positive control of the protease activity. Results: the concentration rates of 5.5 µM and 5.0 µM were found for fluorexon and copper, respectively; their optimal coupling times was 120 min and the maximum Sap activity was observed after 22 h of incubation. Conclusions: the standardized conditions for the spectrofluorometric method allowed confirming the inhibition of Sap by Pepstatin A and showing that this is a viable method to evaluate inhibitors of this protease(AU)
Subject(s)
Spectrometry, Fluorescence/methods , Candida albicans , Fluorescence , ColombiaABSTRACT
The dissolution process is considered an important in vitro tool to evaluate product quality and drug release behavior. Single dissolution methods for the analysis of combined dosage forms are preferred to simplify quality control testing. The objective of the present work was to develop and validate a single dissolution test for a telmisartan (TEL) and amlodipine besylate (AML) combined tablet dosage form. The sink conditions, stability and specificity of both drugs in different dissolution media were tested to choose a discriminatory dissolution method, which uses an USP type-II apparatus with a paddle rotating at 75 rpm, with 900 mL of simulated gastric fluid (SGF without enzymes) as the dissolution medium. This dissolution methodology provided good dissolution profiles for both TEL and AML and was able to discriminate changes in the composition and manufacturing process. To quantify both drugs simultaneously, a synchronous first derivative spectrofluorimetric method was developed and validated. Drug release was analyzed by a fluorimetric method at 458 nm and 675 nm for AML and TEL, respectively. The dissolution method was validated as per ICH guidance.
O processo de dissolução é considerado como uma importante ferramenta in vitro para avaliar a qualidade do produto e o comportamento de liberação do fármaco. Prefere-se um ensaio único de dissolução para formas farmacêuticas contendo associação de fármacos pela simplificação dos testes de controle de qualidade. O objetivo do presente trabalho foi desenvolver e validar um teste de dissolução único para forma farmacêutica comprimidos contendo telmisartana (TEL) e besilato de anlodipino (AML) associados. Condições "sink", estabilidade e especificidade de ambos os fármacos nos diferentes meios de dissolução foram avaliadas para selecionar um método de dissolução discriminatório, que utiliza um aparato do tipo II da USP, com pás girando a 75 rpm e 900 mL de fluido gástrico simulado (SGF sem enzima) como o meio de dissolução. Estas condições proporcionaram bons perfis de dissolução para ambos, TEL e AML, sendo capaz de discriminar as mudanças na composição e processo de fabricação. Para quantificar os dois fármacos simultaneamente, um método de fluorescência derivada sincronizado foi desenvolvido e validado. A quantidade de fármaco liberado foi analisada pelo método fluorimétrico em 458 e 675 nm para a AML e TEL, respectivamente. O método de dissolução foi validado de acordo com a orientação da ICH.
Subject(s)
Spectrometry, Fluorescence/methods , Antihypertensive Agents , Quality Control , Dosage Forms , Dissolution/classificationABSTRACT
Here, a spectrofluorimetric method for the determination of potassium losartan (PL) in pharmaceutical products is described. The effects of critical parameters, pH, acid molarity, and temperature, on the fluorescence intensity of PL were analyzed, and these parameters were optimized using a central composite design (CCD). The highest fluorescent intensity at excitation (λex) and emission (λem) wavelengths of 248 nm and 410 nm, respectively, was achieved using 0.01 M sulfurous acid (pH 2) at 21.6 °C. Under optimum conditions, the method was linear from 0.025-0.5 µg/mL, with a reasonably high correlation coefficient (0.9993). Furthermore, the method was very sensitive (LOQ, 0.006), accurate (RE, ≤7.06), and precise (%RSD, ≤6.51). After development and validation of the method, samples containing PL were analyzed with this method, and the obtained data were statistically compared with those obtained with a previously published reference method using a two one-sided equivalence test (TOST). According to the data, the results from the proposed and reference assays were equivalent.
Descreve-se método espectrofluorométrico para a determinação de losartana potássica (PL) em produtos farmacêuticos. Os efeitos de parâmetros críticos (pH, molaridade ácida e temperatura) na intensidade da fluorecência foram otimizados usando o planejamento de componente central (DCC). A mais alta intensidade fluorescente com λex=248 nm e λem= 410 nm foi obtida usando ácido sulfúrico 0.01 M (pH 2) e 21.6 ºC. Nas condições ideais, a linearidade do método foi estabelecida na faixa de concentração de 0.025-0.5 µg/mL com coeficiente de correlação bastante elevado (0.9993). Além disso, o método foi muito sensível com valor de LOQ 0.006, exato (RE≤7.06) e preciso (RSD%≤6.51). Depois do desenvolvimento e validação do método, amostras de medicamentos contendo PL foram analisadas com este método e os resultados obtidos foram comparados estatisticamente com método de referência, publicado anteriormente, usando o Teste de equivalência TOST (Teste de Equivalência Unilateral). De acordo com os dados estatísticos, os resultados do ensaio de referência e do método proposto foram equivalentes.
Subject(s)
Spectrometry, Fluorescence/methods , Chemistry, Pharmaceutical/methods , Losartan/classification , Composite ResinsABSTRACT
A adesão celular está ligada à formação e disseminação de metástases, a principal causa de óbito de pacientes diagnosticados com câncer. O objetivo deste trabalho foi investigar in vitro o efeito de fotossensibilizadores na adesão celular. Foram utilizadas porfirinas comerciais (PpIX, CPpI, TSPP, TMPyP e Zn(II)TMPyP) e um fotossensibilizador sintetizado através da ligação de poli-L-lisina à protoporfirina IX (PLLPpIX). A adesão celular foi estudada por RICM, técnica que permite quantificar a área de contato entre uma célula e um substrato por binarização das imagens digitais utilizando limiares apropriados. A técnica foi padronizada e revelou dois regimes de adesão celular: um limitado e outro não limitado pela quantidade de proteína de adesão adsorvida na superfície. Neste último foi observada lise celular. Todos os fotossensibilizadores estudados foram capazes de aumentar a adesão celular na ausência de irradiação comparados ao controle sem fotossensibilizador, o que não havia sido observado nos ensaios de resistência à tripsinização normalmente utilizados para estudar o efeito de fotossensibilizadores na adesão celular. Quanto maior a anfifilicidade do fotossensibilizador, maior foi o efeito na adesão, o que é explicado pela capacidade das moléculas em se intercalarem na membrana, mudando a sua rigidez. Este aumento da adesão no escuro correlaciona com a diminuição da migração segundo ensaios de ferida. A análise do padrão de expressão de integrinas na superfície celular revela que o aumento da adesão correlaciona com o aumento na expressão de αV. Quando os fotossensibilizadores estão concentrados na região perimembranar (1 minuto de incubação) e as células são irradiadas, há um aumento da adesão em relação ao controle sem fotossensibilizador, mas uma diminuição em relação ao controle tratado com o fotossensibilizador e não irradiado, o que implica que a PDT leva a uma diminuição da adesão celular e não a um aumento como reportado na literatura. Com 3h de incubação, PLLPpIX impede a adesão celular, enquanto PpIX praticamente não muda a adesão comparado ao controle não irradiado. Esta ausência do efeito da irradiação sugere que a PpIX afeta a adesão celular principalmente devido a sua intercalação na membrana e não devido à formação de espécies reativas. Com 3h de incubação os fotossensibilizadores não se encontram na membrana e, portanto, o efeito na adesão celular é indireto e também não está relacionado à diferenças na eficiência de internalização. O comportamento observado deve ter relação com diferenças de citolocalização. Outro processo que pode alterar a adesão celular é a oxidação das proteínas do soro fetal bovino. Como observado nos estudos de fotossensibilização de células, PLLPpIX foi capaz de impedir a adesão celular, diferentemente da PpIX. A maior eficiência da PLLPpIX foi associada a presença do polímero, o qual força por questões estéricas que a interação da PLLPpIX com a albumina, o componente majoritário do soro, fique restrita à superfície da proteína, deixando o fotossensibilizador disponível para interagir com o oxigênio molecular e gerar oxigênio singlete. Assim, a funcionalização com um polímero tornou a PpIX capaz de modular a adesão celular tanto agindo dentro da célula quanto na matriz extracelular
Cell adhesion is associated to the formation and spread of metastasis, the leading cause of death in cancer patients. The aim of this study was to investigate, in vitro, the effect of photosensitizers in cell adhesion. Five commercial porphyrins (PpIX, CPpI, TSPP, TMPyP e Zn(II)TMPyP) and Protoporphyrin IX covalently tethered to poli-L-lysine (PLLPpIX) were used. Cell adhesion was mainly studied by RICM, a technique that allows quantifying the contact area between a cell and a substrate for binarization of digital images using appropriate thresholds. The technique was standardized and disclosed two systems for cell adhesion: a system limited by the amount of adhesion proteina adsorbed on the surface and another one no limited, in which cell lysis was observed. All photosensitizers were able to enhance cell adhesion in the absence of irradiation compared to control without photosensitizer, which had not been observed in the trypsinization resistance tests usually used to study the effect of photosensitizers in cell adhesion. The greater the amphiphilicity of the photosensitizer, the greater was the effect on cell adhesion. This is explained by the ability of molecules to fit in the membrane, changing its tension. This increased adhesion correlates with the decrease in migration according to wound healing assays. Analysis of the integrin expression pattern on cell surface reveals that increased adhesion correlates with increased expression of alpha V. When photosensitizers are concentrated in the perimembranar region (1 minute of incubation) and cells are irradiated, there is an increase in adhesion when compared to control without photosensitizer, but a decrease relative to controls treated with the photosensitizer without irradiation, implying that PDT leads to a reduction of cell adhesion and not to an increase as reported in the literature. With 3h of incubation PLLPpIX prevents cell adhesion, while PpIX practically does not change the adhesion compared to dark control. This lack of effect of irradiation suggests that PpIX affects cell adhesion primarily because of its intercalation into the membrane and not due to the formation of reactive species. With 3h of incubation the photosensitizers are not on the membrane and therefore the effect on cell adhesion is indirect and it is not also related to differences in uptake efficiency. The observed behavior must be related to differences in subcellular localization arising from differences in molecular structure. Another process that can alter the cell adhesion is serum protein oxidation. As noted in the studies with cells, photosensitization of serum with PLLPpIX (but not with PpIX) was capable of preventing cell adhesion. The greater efficiency of PLLPpIX was associated with the presence of the polymer, which, by the steric hindrance, forces that interaction of PLLPpIX with albumin, the major serum component, is restricted to the protein surface, leaving the photosensitizer available to interact with molecular oxygen and generate singlet oxygen. Thus, the functionalization of a polymer has turned PpIX capable of modulating cell adhesion by acting both within and outside (in extracellular matrix) the cell
Subject(s)
Cell Adhesion/genetics , Porphyrins/analysis , Cell Culture Techniques/methods , L-Lysine 6-Transaminase , Neoplasms/genetics , Oxidative Stress/genetics , Photochemotherapy/adverse effects , Photosensitizing Agents/adverse effects , Spectrometry, Fluorescence/methodsABSTRACT
Os antipsicóticos são drogas utilizadas no tratamento de muitos transtornos psiquiátricos, sendo classificados em dois grupos: típicos e atípicos. Os típicos formam o grupo de drogas que bloqueiam especialmente os receptores de dopamina e, por isto, causam efeitos colaterais característicos, que se manifestam através de sintomas extrapiramidais e podem terminar em discinesia tardia. Os atípicos apresentam eficácia antipsicótica similar à dos antipsicóticos típicos, mas produzem menos efeitos colaterais extrapiramidais e não causam discinesia tardia. Os antipsicóticos se ligam às proteínas plasmáticas, principalmente a albumina, a qual representa cerca de 60% do total das proteínas no soro humano. Neste trabalho estudamos os processos de interação de duas drogas antipsicóticas atípicas, risperidona e sulpirida, com as albuminas séricas humana (HSA) e bovina (BSA), através da técnica de supressão da fluorescência intrínseca do triptofano. A partir dos espectros de fluorescência, a análise dos dados foi feita obtendo-se os gráficos e as constantes de Stern-Volmer. A análise da supressão da fluorescência foi feita a partir da média aritmética dos dados oriundos dos experimentos realizados em cada condição adotada. Como a molécula da sulpirida é fluorescente desenvolvemos uma modelagem matemática do processo de interação, que nos permitiu então obter os dados referentes à supressão da fluorescência da proteína. Os resultados mostraram que a risperidona e a sulpirida suprimem a fluorescência de ambas albuminas por um processo de quenching estático, formando complexos droga-albumina. A risperidona tem uma afinidade com a HSA cerca de 6,5 vezes maior do que a sulpirida, a 37 oC. As constantes de associação calculadas para a interação risperidona-HSA, através da Teoria de Stern-Volmer, foram 1,43 (± 0,05) x 105 M-1, a 37 °C, e 2,56 (± 0,09) x 105 M-1, a 25 ºC1; e para a sulpirida, 2,20 (± 0,08) x 104 M-1, a 37 ºC, e 5,46 (± 0,20) x 104 M-1, a 25 ºC...
Antipsychotics are drugs used to treat many psychiatric disorders. They are classified into two groups: typical and atypical. The typical group act blocking dopamine receptors in particular and it causes characteristic side effects with extrapyramidal symptoms, and can lead to tardive dyskinesia. The atypical group presents similar efficacy to typical group, but they produce less extrapyramidal side effects and does not cause tardive dyskinesia. Antipsychotics bind to plasmatic proteins, mainly to albumin, which represents about 60% of total human serum proteins. In this study we studied the interactions of two atypical antipsychotic drugs, risperidone and sulpiride, with human serum albumin (HSA) and bovine (BSA) through the technique of intrinsic tryptophan fluorescence quenching. From the fluorescence spectra, a data analysis was made to obtain Stern-Volmer plots and constants. Quenching analysis was performed used from using arithmetic means of data from experiments for each adopted condition. As sulpiride molecule is fluorescent, a mathematical modeling for interaction process was made. It allows us then to obtain the data referents to fluorescence quenching of protein. Results showed that risperidone and sulpiride quench the fluorescence for both albumins by static quenching process, forming complexes drug-albumin. The risperidone affinity to HSA is about 6.5 higher than supiride, at 37 oC. Stern-Volmer constants for interaction risperidone-HSA were 1.43 (± 0.05) x 105 M-1, at 37oC, and 2.56 (± 0.09) x 105 M-1, at 25 oC; and for sulpiride were 2.20 (± 0.08) x 104 M-1, at 37 oC, and 5.46 (± 0.20) x 104 M-1, at 25 oC. As the quenching ratio for BSA was higher than HAS, we suggested that the primary site for risperidone on albumin is closer of the domain of trypthophan 134 of BSA than the domain of trypthophan 212 of HAS. The same is suggested for the primary site of supiride at 37oC.
Subject(s)
Antipsychotic Agents/pharmacology , /methods , Serum Albumin , Drug Interactions , Spectrometry, Fluorescence/methods , Mathematical Computing , Risperidone , Sulpiride , Serum Albumin, Bovine/chemistry , Tryptophan/chemistryABSTRACT
Grau de Conversão (GC) em dentística restauradora se define como o método para medir da taxa de conversão de resinas compostas. Devido aos diferentes tipos de polimerização bem como de composições das resinas esta propriedade é imperceptível ao profissional clínico e somente torna-se perceptível através de instrumentos laboratoriais. Foi medido o Grau de Conversão para este estudo de 3 marcas comerciais de resinas compostas (Filtek Z250, Fill Magic e Opallis) para a restauração direta, através do Infravermelho por Transformadas de Fourier (FTIR) BXll Perkin Elmer com absorbância nos números de onda 1297 ± 10 cm-1, 1319 ± 10 cm-1 e 1637 ± 10 cm-1 em função da potência dos aparelhos fotoativadores Bisco (300 mW/cm2 e 600 mW/cm2) e DMC Ultra Blue IS (350 mW/cm2). Uma amostra de 10 mg ± 2 mg foi colocada no ZnSe ATR ( Miracle ATR, Perkin Elmer) e medido antes da polimerização (T0) com os parâmetros : 600 4000 cm-1 e 32 scans. Após esta leitura inicial a amostra foi polimerizada por 20s, 40s, 60s e 80s com o aparelho fotoativador na intensidade pretendida e ajustada. As resinas Filtek Z250, FillMagic e Opallis apresentaram um grau de conversão semelhantes entre si e satisfatório com o fotoativador Bisco na duas potências (300 e 600 mW) testadas. Com a fotoativador DMC as resinas Opallis e Fill Magic não atingiram o objetivo de 52 % de conversão. A combinação Fotoativador, Resina e Tempo de Polimerização ideal é de imensa importância para o sucesso da restauração
The Degree of Conversion (DC) in restorative dentistry is defined as a method to measure the rate of conversion of composites. Due to the different types of compositions and polymerization of the resins this property is imperceptible to the clinician and only becomes visible through laboratory instruments. In this study was measured the degree of conversion of three brands of resin composites (Filtek Z250, Fill Magic and Opallis) for direct the restoration, by Fourier Transformed Infrared (FTIR) BXll - Perkin Elmer with absorbance in the wave numbers 1297 ± 10 cm-1 1319 ± 10 cm-1 and 1637 ± 10 cm-1 in function of the power of light curing units Bisco (300 mW/cm2 and 600 mW/cm2) and DMC IS Ultra Blue (350 mW/cm2) .A sample of 10 mg ± 2 mg was placed on the ZnSe ATR (ATR Miracle, Perkin Elmer) and measured before the polymerization (T0) with the parameters: 600 - 4000 cm-1 and 32 scans. After this initial reading of the sample was polymerized for 20s, 40s, 60s and 80s with the light-curing unit and desired intensity. The resins Filtek Z250, FillMagic and Opallis showed a similar and satisfactory degree of conversion with the two intensities of the curing unit Bisco (300 and 600 mW) tested. With the DMC curing unit the resins Opallis and Fill Magic failed to reach the goal of 52% conversion. The ideal combination of Light-Curing Unit, resin and polymerization time is of immense importance to the success of the restoration
Subject(s)
Light-Curing of Dental Adhesives , Spectrometry, Fluorescence/methods , Light , Chemical Phenomena , Polymerization , Composite Resins , Dental Restoration, Permanent , Materials Testing/methods , Data Interpretation, StatisticalABSTRACT
A fluorometric analytical method was developed for quantification of protoporphyrin IX (PpIX) in skin samples and receptor phase solution after in vitro cutaneous penetration/permeation studies. Analytical conditions used were: excitation and emission wavelengths: 400 nm and 632 nm; bandwidth: 0.5 nm; excitation and emission slits: 10/10. PpIX was recovered from two different layers of skin, the stratum corneum (SC) and the epidermis plus dermis ([E+D]), by vortex homogenization, probe and bath sonication, using DMSO as an extraction solvent. The detection and quantification limits were 0.002 and 0.005 μg/mL, respectively. The assay was linear from 0.005 - 0.5 μg/mL. The within-day and between-day assay precision and accuracy in DMSO and receptor phase solution were each studied at the two concentration levels 0.04 and 0.2 μg/mL, and 0.01 and 0.08 μg/mL, respectively. The coefficients of variation and deviation from the theoretical values were lower than 5%. The skin recovery of PpIX from SC and [E+D] layers using two different concentrations (0.5 and 1.0 μg/mL) were all above 90.0%. The method described has potential application to in vitro penetration/permeation studies of PpIX using porcine skin as a biological membrane model.
Um método analítico por espectrofluorimetria foi desenvolvido para quantificar a protoporfirina IX (Pp IX) em amostras de pele e fase receptora após a realização de testes in vitro de penetração/permeação cutâneas. As condições analíticas utilizadas foram: comprimentos de onda de excitação e emissão: 400 nm e 632 nm; largura de banda: 0,5 nm; fendas de excitação e emissão: 10/10. A PpIX foi extraída de amostras de estrato córneo (EC) e da epiderme sem estrato córneo + derme ([E+D]) através da agitação em vórtex e sonicação por haste e banho, utilizando-se o DMSO como solvente extrator. O limite de detecção e quantificação foram, respectivamente, de 0,002 e 0,005 μg/mL. O método mostrou-se linear da faixa de 0,005 - 0,5 μg/mL. A precisão e exatidão intra e inter-ensaio em DMSO e na fase receptora foram validadas utilizando-se duas concentrações distintas, respectivamente, de 0,004 e 0,2 μg/mL, e 0,01 e 0,08 μg/mL. Os valores de coeficiente de variação e o desvio do valor teórico foram inferiores a 5%. A recuperação da PpIX das camadas da pele (EC e [E+D]) utilizando-se duas concentrações distintas (0,5 e 1,0 μg/mL) foram todas acima de 90,0%. O método descrito pode ser utilizado para determinação da PpIX após estudos de penetração/permeação cutânea in vitro utilizando pele de porco como modelo de membrana.
Subject(s)
Skin Absorption , Spectrometry, Fluorescence/methods , In Vitro Techniques , Protoporphyrins/biosynthesis , Protoporphyrins/chemistry , Biological Assay/methods , SkinABSTRACT
Simple and sensitive spectrophotometric and spectrofluorimetric methods have been developed for determination of 1, 4-dihydropyridine [1, 4-DHP] drugs based on the oxidation of the investigated 1, 4-DHP drugs with acidic KMnO4 [method I] or Ce [IV] [method II]. The first method is based on the decrease in the colour of the permanganate solution due to the presence of the studied drug was measured at 525 nm. And the second method is based on monitoring the fluorescence of the produced cerium [III] at emission 355 nm [excitation at 255 nm]. All variables that affect the performance of the proposed methods were carefully studied and optimized. The analytical performance of the methods was validated according to International Conference of Harmonization guidelines. The proposed methods were applied successfully to the determination of the drugs in commercial tablets and capsules. The results of the proposed procedures were statistically and compared with those obtained by the reference methods
Subject(s)
Spectrophotometry/methods , Spectrometry, Fluorescence/methods , Potassium Permanganate , Cerium , Ammonium SulfateABSTRACT
O uso de interação da luz com a matéria não é um conceito novo em biologia para a detecção de processos físico-químicos, embora ainda seja utilizado de uma forma rudimentar. Já é sabido que imagens de refletância e fluorescência podem revelar informações importantes sobre tais processos em amostras biológicas. Apesar deste potencial, os sistemas experimentais disponíveis para a obtenção de tais imagens costumam serem complexos e de difícil implementação. Neste trabalho é descrita a construção e a caracterização de uma montagem experimental para produção de imagens hiperespectrais entre 400 e 1.000 nm. O sistema é composto de um espectrômetro, um conjunto de lentes para formação da imagem e uma câmera CCD para capturá-la. São descritos em detalhes o procedimento de calibração do sistema, o qual envolve os parâmetros largura da imagem, campo de visão, resolução espectral e espacial. O sistema de iluminação utiliza diodos emissores de luz de alta potência, tanto de luz branca quanto em 470 e 405 nm. Demonstramos que o sistema construído é capaz de obter imagens de fluorescência e/ou refletância de amostras biológicas. Como exemplos de aplicações, o instrumento aqui desenvolvido foi utilizado em dois campos distintos, a agricultura e a odontologia. Foram obtidas imagens de fluorescência de folhas de citros contaminadas com cancro cítrico, e de processos de desmineralização em dentes. Os resultados demonstram que o sistema construído está operando como projetado.
The use of light-mater interaction for the detection of chemicalphysical processes is not a new concept in biology, though it is still used in a rudimentary form. It is already known that reflectance as well as fluorescence images can reveal important information on such processes in biological samples. In spite of this potential, the experimental available image systems usually are complexes and of difficult implementation. In this work, we describe the construction and characterization of an experimental device to produce hyperspectral images between 400 and 1,000 nm. The system is composed of a spectrometer, a set of lenses for image formation and a CCD camera to capture it. We describe in details also the calibration procedure of the system, which involves parameters as image width, field of view, spectral and space resolution. The illumination system uses high power light emitting diodes, either at white light or at 470 and 405 nm. We demonstrate that our system is able to obtain reflectance as well as fluorescence images of biological samples. As examples of applications, we use it into two different fields, agriculture and dentistry. We obtained fluorescence images of citrus leaves contaminated with citrus canker and demineralization processes in teeth. Our results demonstrate that our system isoperating as designed.
Subject(s)
Spectrometry, Fluorescence/instrumentation , Spectrometry, Fluorescence/methods , Spectrometry, Fluorescence , Spectrum Analysis/instrumentation , Spectrum Analysis/methods , Diagnostic Imaging/instrumentation , Molecular Imaging/instrumentation , Image Interpretation, Computer-Assisted/instrumentation , Risk Measurement EquipmentABSTRACT
The interaction of erythrosine B (ErB), a commonly used dye for coloring foods and drinks, with bovine serum albumin (BSA) was investigated both in the absence and presence of bilirubin (BR) using absorption and absorption difference spectroscopy. ErB binding to BSA was reflected from a significant red shift of 11 nm in the absorption maximum of ErB (527 nm) with the change in absorbance at λmax. Analysis of absorption difference spectroscopic titration results of BSA with increasing concentrations of ErB using Benesi-Hildebrand equation gave the association constant, K as 6.9 104 M-1. BR displacing action of ErB was revealed by a significant blue shift in the absorption maximum, accompanied by a decrease in absorbance difference at λmax in the difference spectrum of BR-BSA complex upon addition of increasing concentrations of ErB. This was further substantiated by fluorescence spectroscopy, as addition of increasing concentrations of ErB to BR-BSA complex caused a significant decrease in fluorescence at 510 nm. The results suggest that ErB binds to a site in the vicinity of BR binding site on BSA. Therefore, intake of ErB may increase the risk of hyperbilirubinemia in the healthy subjects.
Subject(s)
Animals , Bilirubin/chemistry , Binding Sites , Cattle , Erythrosine/chemistry , Erythrosine/metabolism , Kinetics , Protein Binding , Serum Albumin/chemistry , Serum Albumin, Bovine/chemistry , Spectrometry, Fluorescence/methods , TemperatureABSTRACT
A serine residue Ser463, required for proper function of E. coli -glutamyltranspeptidase (EcGGT) was identified by site-directed mutagenesis on the basis of sequence alignment of human, pig, rat, and three bacterial enzymes. Thr-, Asp-, and Lys-substituted variants were overexpressed in E. coli M15 cells and the recombinant proteins were purified to near homogeneity by nickel-chelate chromatography. With the exception of S463T, the other two variants completely lost GGT activity, implying the importance of this residue in EcGGT. Moreover, substitution of Ser463 with either Lys or Asp impaired the capability of autocatalytic processing of the precursor into - and -subunit. Computer modeling showed that the critical bonding distance of Gln390 C-Thr391 OG1 was significantly increased in S463D and S463K, indicating that these distance changes might be responsible for the lack of enzyme maturation. Measurements of intrinsic tryptophan fluorescence revealed alteration of the microenvironment of aromatic amino acid residues in S463D and S463K, while circular dichroism (CD) spectra were nearly identical for wild-type and all mutant enzymes. The temperature-dependent signal in the far-UV region for S463T was consistent with that of wild-type enzyme, but S463D and S463K showed a different sensitivity towards temperature-induced denaturation. These results implied that a significant conformational change occurred as a result of Asp- and Lys-substitution.