Correlação entre os valores séricos de fosfatase alcalina e de desidrogenase lática e a porcentagem de necrose tumoral pós-quimioterapia no osteossarcoma / Correlation between the serum values of alkaline phosphatase and lactate deshydrogenase and the chemotherapy-induced necrosis percentage in osteossarcoma

Zumarraga Montaño, Juan Pablo

22 July 2014

INTRODUÇÃO: A resposta do osteossarcoma (OS) à quimioterapia (QT) préoperatória é atualmente o indicador mais sensível para o prognóstico de sobrevida dos pacientes diagnosticados com OS. Esta resposta é avaliada mediante a porcentagem de necrose encontrada pelo patologista após a extração da peça na cirurgia, utilizando- se o índice de necrose tumoral de Huvos, no qual a necrose é expressada percentualmente. Existem estudos correlacionando os valores da fosfatase alcalina (FA) e da desidrogenase lática (DHL) com a sobrevida do paciente. Neste trabalho foi pesquisada a relação que existe entre os valores sanguíneos, pré e pós QT, de FA e DHL, com a porcentagem de necrose tumoral encontrada na peça cirúrgica após a realização da QT pré-operatória. MÉTODOS: Foram estudados 647 prontuários de pacientes tratados pelo Grupo de Oncologia Ortopédica do Instituto de Ortopedia e Traumatologia do Hospital das Clinicas da Faculdade de Medicina da Universidade de São Paulo, no período de 1990 até o inicio de 2013, com diagnóstico anatomopatológico de OS. Destes, 510 foram excluídos por não apresentarem dados completos para a análise posterior. Foram incluídos um total de 137 prontuários. Os valores da FA e da DHL dos pacientes incluídos foram obtidos da realização do estadiamento, antes da QT pré-operatória e dos valores reportados após a finalização da QT pré-operatória. Também foi coletado o grau de necrose tumoral de cada peça extraída na cirurgia de cada paciente. Classificamos os resultados da FA e DHL obtidos em dois grupos. No grupo I os pacientes com valores normais de FA e DHL, no grupo II, os pacientes com valores acima do limite de normalidade. A classificação utilizada para agrupar os valores de sorológicos em investigação foi adaptado do trabalho realizado por Bramer et. al. Foi reportada a porcentagem de necrose tumoral descrita pelos patologistas, obtida das peças extraídas nas cirurgias realizadas pós QT. Esta porcentagem foi classificada de acordo com a classificação de Huvos. Foram calculadas as correlações da necrose da peça cirúrgica (Huvos) com as enzimas pré, pós e alteração (pós-pré) QT e também entre as enzimas, com uso de correlações de Spearman para verificar a existência de correlação entre elas. RESULTADOS: Tanto a FA como a DHL diminuíram nos pacientes estudados, quando comparados os valores pré QT e pós QT. A média da diferença da FA obtida pré QT e pós QT foi de 795,12 U/L sendo o valor pré QT maior ao valor pós QT. A diferença entre os valores da DHL pré QT e pós QT foi em média de 437,40 U/L, sendo o valor pré QT maior ao valor pós QT. Não houve correlação estatisticamente significativa entre o índice de Huvos e os valores de FA e DHL. A ausência da relação foi observada tanto com os valores pré-quimioterapia, quanto com os valores pós-quimioterapia, não obtendo correlação com a alteração das enzimas após a quimioterapia (p < 0,05). CONCLUSÃO: A medição de FA e da DHL não são fatores preditivos sobre a resposta tumoral à quimioterapia préoperatória em pacientes portadores de osteossarcoma / BACKGROUND AND AIMS: The osteosarcoma´s (OS) response to pre surgical chemotherapy (CT) is actually the most sensible predictor for life prognosis in patients diagnosed with OS. This response is evaluated by the chemotherapy-induced necrosis percentage found by the pathologist after the removal of the surgical piece, using the Huvos tumor necrosis (TN) index, in which the necrosis is expressed in percentage. There are studies that correlate the alkaline phosphatase (AP) and the lactate deshydrogenase (LDH) with the patient\'s life prognosis. In this study we researched the relationship between the serum levels of pre and post CT of AP and LDH and the percentage of TN found in the surgical piece after the pre surgical CT. METHODS: This is a retrospective study in which we studied 647 medical history files with anatomopathologic diagnosis of OS, treated by the Orthopedic oncology group of the Orthopedic and Traumatology Institute of the Hospital das Clinicas of the Medical School of the University of São Paulo between 1990 and 2013. Out of these, 510 were excluded for not having complete data for posterior analyses. We included 137 files in the study. The AP and the LDH values were obtained before and after pre surgical CT. We also obtained the degree of chemotherapy-induces TN obtained from the surgical piece. We classified the AP and the LDH into two groups. In the first group the patients with normal AP and LDH values and in the second group those with values above normal limit. This classification was adapted from the study published by Bramer et al. We classified the percentage of TN obtained from the removed surgical pieces after CT, using the Huvos index. We calculated the correlation between the TN with the pre, post and pre-post difference CT enzymes, using the Spearman correlation. RESULTS: The AP and the LDH decreased when comparing the pre CT values to the post CT values. The mean of the difference was of 795.12 U/L, the pre CT value being higher than the post CT. The difference between the LDH values pre and post CT was of 437.40 U/L, being the pre CT higher than the post CT. There was no statistically significant correlation between the Huvos index and the AP and LDH values. This was observed with the pre CT as well as with the post CT values (p < 0,05). CONCLUSIONS: The values of AP and LDH are not predictors for the tumor\'s chemotherapy-induced necrosis to pre surgical CT in patients with osteosarcoma

Alkaline phosphatase

Drug therapy

Fatores de necrose tumoral

Fosfatase alcalina

L-lactate dehydrogenase

L-lactato desidrogenase

Osteosarcoma

Osteosarcoma

Prognosis

Prognóstico

Quimioterapia

Tumor necrosis factors

Caracterização de disintegrinas de venenos viperídeos como ferramentas seletivas na detecção ou inibição da função de integrinas / Characterization of viper venom disintegrins as tools for detecting and inhibiting integrin function

Wadsworth, Diego Alberto Butera

15 December 2003

As integrinas são proteínas de membrana envolvidas em diversos processos biológicos como embriogênese, inflamação e agregação plaquetária. A alteração de seu padrão de expressão está relacionada com processos patológicos como trombose e câncer, fazendo das integrinas ótimos indicadores da progressão destas doenças. Assim, a integrina &#945;2&#946;1 pode ser considerada como indicadora de angiogênese, sendo expressa nas células endoteliais durante o crescimento de novos vasos. Já a ausência da &#945;IIb&#946;3 em plaquetas está relacionada com a doença de Glanzmann, caracterizada por uma agregação plaquetária deficiente, e sua presença em outros tipos celulares está relacionada com processos de metástase e invasão de tecidos. Estas integrinas contêm antagonistas naturais nos venenos de serpentes da família VIPERlDAE: As RGD-disintegrinas bloqueiam a integrina &#945;IIb&#946;3 e as ECD-disintegrinas bloqueiam a integrina &#945;2&#946;1. Estas últimas formam parte de metaloproteinases com múltiplos domínios de aproximadamente 50 kDa. Interessados em desenvolver marcadores moleculares para estas integrinas, direcionamos nossos objetivos para: (1) a elucidação da região mínima das ECD-disintegrinas com atividade biológica e (2) construção de biomarcadores para a integrina &#945;2&#946;1 utilizando a região elucidada, e para a integrina &#945;IIb&#946;3 utilizando uma RGD-disintegrina. Neste trabalho conseguimos determinar uma região de 49 resíduos na porção C-terminal do domínio ECD-disintegrina da jararagina que reage com um anticorpo neutralizante das atividades hemorrágica e de ligação ao colágeno da proteína. Esta região foi subclonada e expressa em fusão com a fosfatase alcalina de E. colí, mas não teve funcionalidade como marcador. No entanto, a RGD-disintegrina eristostatina em fusão com a fosfatase alcalina mostrou bifuncionalidade, apresentando tanto atividade disintegrina como atividade catalítica. Além disso, verificamos sua seletividade pela integrina &#945;IIb&#946;3 e padronizamos um ensaio direto de dot blot para a presença dessa integrina em plaquetas, com um único passo de incubação. / Integrins are membrane proteins involved in biological processes such as embriogenesis, inflammation and platelet aggregation. The alteration of their expression pattem is related to pathological disorders such as thrombosis and cancer, making integrins suitable indicators of the progression of these diseases. Thus, the &#945;2&#946;1 integrin, which is expressed in endothelial cells during capillary growth, may be an indicator of angiogenesis. The absence of &#945;IIb&#946;3 integrin in platelets is related to Glanzmann disease, characterized by defective platelet aggregation and its expression in other cellular types is related with metastasis and tissue-invasion processes. These integrins contain natural antagonists in venoms from the VIPERIDAE snake family: RGD-disintegrins, which block the &#945;IIb&#946;3 integrin and ECD-disintegrins, which block the &#945;2&#946;1 integrin. The latter forming part of multidomain metalloproteinases of approximately 50 kDa. In order to develop molecular markers for integrins, we have directed our objectives at: (1) determining the minimal region of ECD-disintegrins with biological activity and (2) engineering biomarkers for the &#945;2&#946;1 integrin using the previously determined minimal region and for the &#945;IIb&#946;3 using an RGD-disintegrin. In this work we have determined a 49-residue region located in the C-terminus of jararhagin ECD-disintegrin domain, which reacts with a neutralizing antibody of hemorrhagic and binding to collagen activities of the protein. This region was subcloned and expressed in fusion with E. coli alkaline phosphatase, but did not present a marker activity. On the other hand, the RGD-disintegrin eristostatin fused to alkaline phosphatase showed bifunctionality, presenting both, disintegrin and catalytic activities. Furthermore, we have characterized its selectivity for the &#945;IIb&#946;3 integrin and we have standardized a direct dot blot assay with one-step incubation for the presence of this integrin in platelets.

Alkaline phosphatase

Biologia molecular

Clonagem

Cloning

Desintegrinas

Disintegrinas

Disintegrins

Expressão gênica

Fosfatase alcalina.

Marcadores moleculares

Metalloproteinases

Metaloproteinases

Molecular biology

Molecular marker

Plasmídeo

Comportamento de marcadores séricos de formação e reabsorção óssea após enxerto autógeno em fissura alveolar congênita : sem e com plasma rico em plaquetas /

Marchesano, Luiz Henrique.

January 2005

Orientador: Iguatemy Lourenço Brunetti / Banca: Luís Carlos Spolidorio / Banca: Marília Afonso Rabelo Buzalaf / Banca: Maria Teresa Pepato / Banca: Maria Lúcia Rubo de Rezende / Resumo: O tratamento cirúrgico da fissura congênita do processo alveolar superior compreende o enxerto ósseo, um procedimento bem aceito e de grande importância na restauração da forma e da função perdidas. Associado ao enxerto ósseo tem-se utilizado um produto atóxico, não imunoreativo e de fácil obtenção, denominado plasma rico em plaquetas (PRP). Neste estudo foi analisado o comportamento dos marcadores fosfatase alcalina, fosfatase alcalina isoforma óssea, osteocalcina e fosfatase ácida tartarato resistente em 50 pacientes, com idade entre 10 e 20 anos e que foram submetidos à cirurgia de enxerto ósseo autógeno alveolar pelo serviço de Cirurgia Buco-maxilofacial do Hospital de Reabilitação de Anomalias Craniofaciais da Universidade de São Paulo. O objetivo foi acompanhar de forma sistêmica e em curto período a formação ou reabsorção óssea após a realização do enxerto ósseo alveolar, bem como avaliar a eficácia do uso do plasma rico em plaquetas no processo de formação óssea. O estudo concluiu que as propriedades restauradoras do PRP não puderam ser demonstradas por nenhum dos marcadores bioquímicos do metabolismo ósseo nos primeiros 70 dias do ato cirúrgico; a análise temporal dos marcadores de formação óssea testados demonstrou uma tendência de queda com 35 dias e retorno próximo aos níveis basais com 70 dias do ato cirúrgico nos dois grupos estudados; não houve uma correlação significativa dos marcadores com o número de plaquetas e nem com a área da fissura e o resultado do exame ao raio X foi considerado inconclusivo para a presença ou não de trabeculado ósseo organizado em fase inicial de formação. / Abstract: The surgical treatment of the congenital cleft of the upper alveolar process understands the bone graft, a well accepted procedure of great importance in the restoration of the lost form and function. Together with the bone graft it is being used a non-toxic, non imunoreactive and easily obtained product, denominated platelet-rich plasma (PRP). In this study it was analysed the behavior of the alkaline phosphatase, bone alkaline phosphatase, osteocalcin and tartrate-resistant acid phosphatase markers in 50 patients, with age between 10 and 20 years and that were undergone to alveolar autogenous bone graft performed by the Bucomaxillofacial Service of the "Hospital for Rehabilitation of Craniofacial Anomalies, University of São Paulo". The aim was follow in a sistemic and early way the bone formation or reabsorption after the accomplishment of the alveolar bone graft, as well as to evaluate the effectiveness of the use of the platelet-rich plasma in the process of bone formation. The study concluded that the restorative properties of the PRP could not be demonstrated by of the biochemistry markers of the bone metabolism in the first 70 days of the surgery; the temporal analisys of the bone formation markers tested demonstrated a fall tendency in 35 days with return near to basal levels in 70 days in the two studied groups; there was not a significant correlation between markers and the number of platelets and neither with the area of the cleft and the result of the x-ray examination was not considered conclusive for the presence or not of organized bone trabeculae in the initial phase of formation. / Doutor

Transplante ósseo.

Plasma.

Plaquetas.

Fosfatase alcalina.

Fosfatase ácida.

Alveolar bone graft. eng

Platelet-rich plasma. eng

Alkaline phosphatase. eng

Osteocalcin. eng

Tartrate-resistant acid phosphatase. eng

Influence du strontium sur la minéralisation initiée par les vésicules matricielles et sur l’activité de la phosphatase alcaline / Influence of strontium on mineralization initiated by matrix vesicles and on alkaline phosphatase activity

Bechkoff, Géraldine

11 June 2009

Les vésicules matricielles sont des organites extracellulaires impliques dans les processus de minéralisation. Nous avons détermine le mode d’action du strontium, ion contenu dans le principe actif d’un médicament antiostéoporotique sur les vésicules matricielles. Nous avons montre que le strontium agit en fonction de la concentration aussi bien sur la formation de l’hydroxyapatite que sur les activités phosphomonoéstérase et phosphodiestérase de la phosphatase alcaline tissu non spécifique. Pour des faibles concentrations (comprises entre 25 et 100^M), le strontium augmente l’activité phosphodiestérase et inhibe partiellement l’activité phosphomonoestérase. La balance entre la production de PPi, inhibiteur de la minéralisation et la production de Pi, essentiel a la formation d’hydroxyapatité pourrait être affectée par le strontium. / The matrix vesicles are extracellular organelles implicated in the process of mineralization.We determined the mode of action of strontium, ion contained in the active principle of an antiosteoporotic drug on the matrix vesicles. We showed that the action of strontium is concentration dependent on the hydroxyapatite formation and on phosphomonoesterase and phosphodiesterase activities of the tissue non specific alkaline phosphatase. At low concentration (between 25 and 100^M), strontium increased phosphodiesterase activity and inhibited partly phosphomonoesterase activity. The balance between the production of PPi, inhibitor of mineralization and the production of Pi, essential in the formation of hydroxyapatite could be affected by the strontium.

Vésicules matricielles

Strontium

Hydroxyapatite

Os

Mineralisation

Matrix vesicles

Strontium

Hydroxyapatite

Tissue non specific alkaline phosphatase

Bone

Mineralization

572

Molecular mechanisms of vascular smooth muscle cell transdifferentiation into osteochondrocyte-like cells / Mécanismes moléculaires de la trans-différenciation des cellules musculaires lisses en cellules de type ostéo-chondrocytaire

Fakhry, Maya

02 December 2015

Chez les patients souffrant d'insuffisance rénale chronique, les calcifications vasculaires représentent la première cause de mortalité. Elles résultent de la trans-différenciation des cellules musculaires lisses (CMLs) en cellules de type ostéoblastique et/ou chondrocytaire, en réponse à des cytokines inflammatoires ou à une hyperphosphatémie. Les CMLs forment alors des cristaux par l'activité de la phosphatase alcaline non-spécifique du tissu (TNAP). A la lumière de résultats récents, nous avons émis l'hypothèse que la TNAP module la trans différenciation des CMLs. Nos objectifs étaient donc de déterminer l'effet de la TNAP dans la trans-différenciation des CMLs, et d'étudier les mécanismes impliqués dans son induction, avec un intérêt particulier pour les microRNAs. Nous avons observé que l'ajout de phosphatase alcaline purifiée ou la surexpression de TNAP stimule l'expression de marqueurs chondrocytaires en culture de CMLs et de cellules souches mésenchymateuses. De plus, l'inhibition de la TNAP bloque la maturation de chondrocytes primaires. Nous excluons un rôle des cristaux formés par la TNAP, puisque l'ajout de cristaux seuls ou associés à une matrice collagénique n'a pas reproduit les effets de la TNAP. Nous suspectons que la TNAP agit en hydrolysant le pyrophosphate inorganique (PPi). En effet, c'est la TNAP qui hydrolyse le PPi en culture de CMLs et de chondrocytes, et le PPi mime les effets de l'inhibition de TNAP en culture de chondrocytes. Enfin, nous rapportons le profil de microRNA des artères cultivées en conditions hyperphosphatémiques. Ces résultats pourraient être particulièrement importants dans le développement de nouvelles approches thérapeutiques / In patients with chronic kidney disease (CKD), vascular calcification represents the main cause of mortality. Vascular calcification results from the trans-differentiation of vascular smooth muscle cells (VSMCs) into cells similar to osteoblasts and/or chondrocytes, in response to inflammatory cytokines or hyperphosphatemia. Calcifying VSMCs form calcium phosphate crystals through the activity of tissue nonspecific alkaline phosphatase (TNAP). In light of recent findings, we hypothesized that TNAP also modulates VSMC trans-differentiation. Our objectives were therefore to determine the effect of TNAP activity on VSMC trans-differentiation, and secondly to investigate the molecular mechanisms involved in TNAP expression in aortas, with a particular interest in microRNAs. We first observed that addition of purified alkaline phosphatase or TNAP over-expression stimulates the expression of chondrocyte markers in culture of the mouse and rat VSMC lines, and of mesenchymal stem cells. Moreover, TNAP inhibition blocks the maturation of mouse primary chondrocytes and reduces mineralization. We exclude a role for crystals in TNAP effects, since addition of crystals alone or associated to a collagenous matrix fails to mimic TNAP effects. We rather suspect that TNAP acts through the hydrolysis of inorganic pyrophosphate (PPi). Indeed, PPi is hydrolyzed by TNAP in VSMCs and chondrocytes and addition of PPi mimics the effects of TNAP inhibition on chondrocyte maturation. Finally, we report microRNA signature of aortic explants treated under hyperphosphatemic conditions that induce vascular calcification. These results could be of particular importance in patients with CKD

Cellules musculaires lisses

Phosphatase alcaline

Trans-differentiation

Calcification vasculaire

Chondrocytes

MicroRNA

Vascular smooth muscle cells

Tissue nonspecific alkaline phosphatase

Trans-differentiation

Vascular calcification

Chondrocytes

MicroRNA

571.6

Role of Phospholipase D in Vascular Calcification / Le rôle de la phospholipase D dans la calcification vasculaire

Skafi, Najwa

20 December 2017

La calcification vasculaire est l’accumulation de cristaux de calcium dans les vaisseaux sanguins à travers un processus pathologique qui ressemble à la formation de l’os ou du cartilage. Elle apparaît notamment chez les patients diabétiques ou atteints d’une insuffisance rénale chronique. La conséquence principale de la calcification vasculaire est la perte de l’élasticité qui est indispensable pour la fonction des larges artères, elle est de plus associée à la mortalité des patients hémodialysés. Les traitements contre la calcification vasculaire sont généralement limités à ceux qui corrigent les facteurs causatifs des problèmes de santé mais aucune intervention efficace, spécifique et ciblée n’est disponible. Par conséquence, une compréhension profonde des mécanismes moléculaires impliqués dans la calcification vasculaire est nécessaire dans le but de trouver de nouvelles cibles thérapeutiques. La phospholipase D catalyse l’hydrolyse des phospholipides en acide phosphatidique et une tête polaire, elle est aussi impliquée dans différentes fonctions cellulaires et maladies. Il a été démontré qu’elle peut être activée par des facteurs impliqués dans l’ostéogenèse et par d’autres impliqués dans la calcification vasculaire. Ainsi, nous avons étudié le rôle de la phospholipase D dans la calcification vasculaire dans 3 modèles différents. Le premier est un modèle in-vitro de cellules musculaires lisses murines (lignée cellulaire MOVAS), elles sont cultivées en présence d’acide ascorbique et de β-glycérophosphate. Le deuxième est un modèle ex-vivo d’explants d’aortes cultivés en présence de fortes concentrations de phosphate et le troisième est un modèle in-vivo d’insuffisance rénale chronique produite chez des rats. Dans ce dernier modèle, la calcification vasculaire est induite par un régime riche en phosphore et en calcium et par des injections de vitamine D active. La calcification dans ces trois modèles a été suivie par l’analyse de la minéralisation en dosant les dépôts de calcium, de l’activité phosphatase alcaline, et de l’expression de différents marqueurs ostéo-chondrocytaires. Une augmentation de l’expression génique de Pld1 a été observée dans les trois modèles, en particulier au cours des premières étapes de la calcification, et a été accompagnée d'une activité accrue de la phospholipase D dans les modèles in vitro et ex-vivo. L’inhibition de l’activité phospholipase D dans ces deux modèles ou de la phospholipase D1 dans le modèle MOVAS a bloqué complètement la calcification. Par contre, l’inhibition spécifique de la phospholipase D2 n’a pas montré des effets significatifs. Deux voies par lesquelles la phospholipase D peut être activée ont été testées, la voie de la protéine kinase C et la voie de la sphingosine-1-phosphate. Ces deux voies métaboliques se sont révélées être impliquées dans le processus de calcification mais pas forcément dans l’activation de la phospholipase D au cours de ce processus. Des résultats préliminaires ont montré que la phospholipase D pourrait agir après activation de la sphingosine kinase 2 dont l’activité s’est avérée nécessaire pour la calcification dans le modèle MOVAS. Des études supplémentaires sont nécessaires pour comprendre par quels mécanismes la phospholipase D est activée et comment elle agit. La phospholipase D pourrait être une nouvelle cible thérapeutique pour le traitement de la calcification vasculaire vu que son inhibition ne semble pas avoir des effets secondaires chez les patients / Vascular calcification is the accumulation of calcium phosphate crystals in blood vessels via a pathological process that resembles physiological bone or cartilage formation. Calcification in the medial layer is mainly seen in diabetic and chronic kidney disease patients. Its main consequence is the loss of elasticity which is indispensable for the function of large arteries. Accordingly, vascular medial calcification was significantly associated with mortality in hemodialysis patients. Vascular calcification treatments are limited to those that correct its causative health problems, but no efficient, specific and targeted interventions are available. Therefore, a deep understanding of its molecular mechanisms is needed to find novel therapeutic targets. Phospholipase D catalyses the hydrolysis of phospholipids into phosphatidic acid and a head group. It is implicated in different cellular functions and diseases. It was found to be activated by factors involved in osteogenesis and others involved in vascular calcification. Thus, we investigated its role in vascular calcification in 3 models: an in-vitro model of murine smooth muscle cell line MOVAS cultured with ascorbic acid and β-glycerophosphate, an ex-vivo model of rat aortas cultured in high phosphate medium, and an in-vivo model of adenine-induced kidney disease in rats in which vascular calcification is induced by further administration of high phosphorus/calcium diet and active vitamin D injections. Calcification was detected in these models using different approaches including alkaline phosphatase activity, calcium dosage, and/or evaluation of osteo-chondrocytic markers expression. Pld1 expression was seen upregulated in all the three models, especially during early stages of calcification, and was accompanied with increased phospholipase D activity in the in-vitro and ex-vivo model. The inhibition of total phospholipase D activity in these two models, or that of phospholipase D1 in case of MOVAS model, abolished calcification. Phospholipase D2-specific inhibition did not induce significant effects. Two pathways by which phospholipase D can be activated were tested, protein kinase C and sphingosine 1-phosphate pathways, but they were found to be involved in calcification but not necessary for phospholipase D activation during this process. Alternatively, the preliminary results showed that PLD may be acting by activation of sphingosine kinase 2 whose activity was found necessary for calcification in the MOVAS model. Further investigations are needed to understand the mechanisms by which phospholipase D is activated and by which it is acting. Phospholipase D could be a novel target for vascular calcification especially that its inhibition in patients did not induce adverse health effects

Phospholipase D

Calcification vasculaire

Phosphatase alcaline

Cellules musculaires lisses

Insuffisance rénale chronique

Aorte

Phospholipase D

Vascular calcification

Alkaline phosphatase

Smooth muscle cells

Chronic kidney disease

Aorta

571.6

Specific recognitioin and enzymatic inhibition : chemical and biochemical aspects of mineralization mechanisms / Reconnaissance spécifique et inhibition enzymatique : aspects chimiques et biochimiques des mécanismes de minéralisation

Li, Lina

14 December 2008

Trois dérivés d’amino acides sont reconnus d’une manière stéréo sélective par l’albumine du sérum bovin. Cette propriété a été observée dans le cas de la phosphatase alcaline de tissu non spécifique, (TNAP). Des inhibiteurs agissant à trois niveaux distincts sur les processus de minéralisation ont été cherchés: 1) TNAP ; 2) Formation de l’hydroxyapatite (HA); 3) Vésicules maticielles (VMs). Nous avons trouvé que des dérivés de benzothiophènes et de tétramisoles, solubles dans l’eau, sont des inhibiteurs spécifiques de TNAP. Un modèle qui permet de produire du HA, a été développé et a confirmé que les nucléotides sont des inhibiteurs de formation de HA. Nous avons montré que le médicament anti-rhumatisme sinomenine, n’ayant aucun effet sur le TNAP, ainsi que la théophylline ralentissaient tous les deux la formation de HA induits par les VMs. Ces modèles de minéralisation présentent un grand potentiel lors du criblage de médicaments pour le traitement de l’ostéoarthrose / Three amino acid derivatives were stereoselectively recognized by bovine serum albumin. Such property was also observed in the case of tissue non-specific alkaline phosphatase (TNAP), a marker in mineral formation. Inhibitors acting at three distinct levels on mineral formation were searched: 1) TNAP; 2) Hydroxyapatite (HA) formation; 3) Matrix vesicle (MV). We found that benzothiophene derivative of tetramisole are water soluble inhibitors of TNAP. A model producing HA as MVs was developed and served to screen HA inhibitors, confirming that several nucleotides inhibited HA formation. We demonstrated that the anti-rheumatic Chinese medicine sinomenine, having no effect on TNAP and theophylline, slowed down HA induced by MVs. The mineralization models presented a great potential to screen putative drugs to cure ostoarthritis.

Alcaline phosphatase

Sinomenine

Reconnaissance

Vésicules matricielles

Ostéoarthrose

Minéralisation

Theophylline

Inhibiteurs

Calcification pathologique

Benzothiophene

Anti-rhumatisme

Alkaline phosphatase

Benzothiophene

Inhibitors

Matrix vesicles

Anti rheumatic

Osteoarthritis

Theophylline

Pathological calcification

Mineralization

Comportamento de marcadores séricos de formação e reabsorção óssea após enxerto autógeno em fissura alveolar congênita: sem e com plasma rico em plaquetas

Marchesano, Luiz Henrique [UNESP]

06 December 2005

Made available in DSpace on 2014-06-11T19:30:28Z (GMT). No. of bitstreams: 0 Previous issue date: 2005-12-06Bitstream added on 2014-06-13T18:40:39Z : No. of bitstreams: 1 marchesano_lh_dr_arafcf.pdf: 336354 bytes, checksum: 54de5ce8ee681faefedf0567be191430 (MD5) / Universidade Estadual Paulista (UNESP) / O tratamento cirúrgico da fissura congênita do processo alveolar superior compreende o enxerto ósseo, um procedimento bem aceito e de grande importância na restauração da forma e da função perdidas. Associado ao enxerto ósseo tem-se utilizado um produto atóxico, não imunoreativo e de fácil obtenção, denominado plasma rico em plaquetas (PRP). Neste estudo foi analisado o comportamento dos marcadores fosfatase alcalina, fosfatase alcalina isoforma óssea, osteocalcina e fosfatase ácida tartarato resistente em 50 pacientes, com idade entre 10 e 20 anos e que foram submetidos à cirurgia de enxerto ósseo autógeno alveolar pelo serviço de Cirurgia Buco-maxilofacial do Hospital de Reabilitação de Anomalias Craniofaciais da Universidade de São Paulo. O objetivo foi acompanhar de forma sistêmica e em curto período a formação ou reabsorção óssea após a realização do enxerto ósseo alveolar, bem como avaliar a eficácia do uso do plasma rico em plaquetas no processo de formação óssea. O estudo concluiu que as propriedades restauradoras do PRP não puderam ser demonstradas por nenhum dos marcadores bioquímicos do metabolismo ósseo nos primeiros 70 dias do ato cirúrgico; a análise temporal dos marcadores de formação óssea testados demonstrou uma tendência de queda com 35 dias e retorno próximo aos níveis basais com 70 dias do ato cirúrgico nos dois grupos estudados; não houve uma correlação significativa dos marcadores com o número de plaquetas e nem com a área da fissura e o resultado do exame ao raio X foi considerado inconclusivo para a presença ou não de trabeculado ósseo organizado em fase inicial de formação. / The surgical treatment of the congenital cleft of the upper alveolar process understands the bone graft, a well accepted procedure of great importance in the restoration of the lost form and function. Together with the bone graft it is being used a non-toxic, non imunoreactive and easily obtained product, denominated platelet-rich plasma (PRP). In this study it was analysed the behavior of the alkaline phosphatase, bone alkaline phosphatase, osteocalcin and tartrate-resistant acid phosphatase markers in 50 patients, with age between 10 and 20 years and that were undergone to alveolar autogenous bone graft performed by the Bucomaxillofacial Service of the Hospital for Rehabilitation of Craniofacial Anomalies, University of São Paulo. The aim was follow in a sistemic and early way the bone formation or reabsorption after the accomplishment of the alveolar bone graft, as well as to evaluate the effectiveness of the use of the platelet-rich plasma in the process of bone formation. The study concluded that the restorative properties of the PRP could not be demonstrated by of the biochemistry markers of the bone metabolism in the first 70 days of the surgery; the temporal analisys of the bone formation markers tested demonstrated a fall tendency in 35 days with return near to basal levels in 70 days in the two studied groups; there was not a significant correlation between markers and the number of platelets and neither with the area of the cleft and the result of the x-ray examination was not considered conclusive for the presence or not of organized bone trabeculae in the initial phase of formation.

Ossos - Enxerto

Enxerto ósseo alveolar

Plasma sanguineo

Plaquetas (Sangue)

Fosfatase alcalina

Fosfatase acida

Osteocalcina

Alveolar bone graft

Platelet-rich plasma

Alkaline phosphatase

Osteocalcin

Tartrate-resistant acid phosphatase

Interação da toxina Cry1ac de Bacillus thuringiensis às microvilosidades apicais das células colunares do intestino médio de Helicoverpa armigera Hübner, 1805 (Lepidoptera: Noctuidae) em diferentes ínstares larvais / Interaction of Cry1ac toxin from Bacillus thuringiensis to brush border membrane of Helicoverpa armigera Hübner, 1805 (Lepidoptera: Noctuidae) midgut in different larval instars

Silva, Igor Henrique Sena da [UNESP]

26 July 2017

Submitted by IGOR HENRIQUE SENA DA SILVA null (igor.sena@outlook.com.br) on 2017-09-05T13:59:07Z No. of bitstreams: 1 DISSERTAÇÃO_Igor_Henrique_Sena_Silva.pdf: 1536012 bytes, checksum: da24e2e008037696caee4c8842fc8f05 (MD5) / Approved for entry into archive by Luiz Galeffi (luizgaleffi@gmail.com) on 2017-09-06T13:13:51Z (GMT) No. of bitstreams: 1 silva_ihs_me_jabo.pdf: 1536012 bytes, checksum: da24e2e008037696caee4c8842fc8f05 (MD5) / Made available in DSpace on 2017-09-06T13:13:51Z (GMT). No. of bitstreams: 1 silva_ihs_me_jabo.pdf: 1536012 bytes, checksum: da24e2e008037696caee4c8842fc8f05 (MD5) Previous issue date: 2017-07-26 / Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP) / Helicoverpa armigera é uma praga altamente polífaga e ataca culturas de grande importância agrícola em diversos países do mundo. O controle desta praga é realizado primariamente por inseticidas químicos. Porém, o uso indiscriminado do controle químico levou a resistência de populações desta praga a maioria dos inseticidas químicos usados para seu controle, dificultando o seu manejo no campo. Além do controle químico, o controle de H. armigera tem sido realizado com uso de plantas transgênicas que expressam a proteína Cry1Ac de Bacillus thuringiensis (Bt) ou por bioinseticidas que contem esta e outras proteínas. No entanto, estudos têm demonstrado uma diminuição significativa na susceptibilidade de H. armigera às proteínas Cry com o aumento de seu desenvolvimento larval. O mecanismo de resistência mais comum dos insetos às proteínas Cry é a redução de ligação da proteína aos receptores presentes na membrana, levando a uma menor afinidade de ligação da proteína aos receptores intestinais. Desta forma, o objetivo deste trabalho foi avaliar a susceptibilidade de lagartas de diferentes ínstares de H. armigera à Cry1Ac e correlacionar com a capacidade de ligação da proteína Cry1Ac às microvilosidades apicais das células colunares do intestino médio (BBMVs) isoladas de todos ínstares larvais. Além disso, por meio de ensaios de imunoprecipitação e análise por cromatografia líquida acoplada a espectrofotometria de massa, identificar as proteínas envolvidas na interação com a proteína Cry1Ac no segundo e quinto ínstares de H. armigera. Foi observada uma redução significativa na susceptibilidade dos últimos ínstares larvais de H. armigera à proteína Cry1Ac comparado aos ínstares iniciais. Os valores estimados de CL50 variaram de 31,1 a 2525,7 ng de proteína/cm² de dieta, em lagartas de primeiro e sexto ínstar, respectivamente. Estes resultados evidenciam uma diferença de 80 vezes na susceptibilidade à proteína Cry1Ac do último para o primeiro ínstar. Nos testes de ligação de ELISA da proteína Cry1Ac às BBMVs dos diferentes ínstares, foi constatada uma diminuição total na capacidade de ligação da proteína Cry1Ac as BBMVs dos estádios mais tardios comparados aos iniciais, com afinidade de ligação aparente de 3,88 vezes menor no último ínstar comparado ao primeiro. Assim, uma clara correlação direta entre toxicidade de Cry1Ac e a afinidade de ligação da proteína às BBMVs de H. armigera foi demonstrada. Os resultados dos ensaios de imunoprecipitação demonstraram um padrão diferenciado de interação com a proteína Cry1Ac no segundo e quinto ínstar. A proteína fosfatase alcalina (ALP) foi identificada apenas no segundo ínstar, bem como, outras proteínas de membrana, como proibitina e uma proteína de canal iônico, que podem estar envolvidas para a alta toxicidade de Cry1Ac em ínstares iniciais de H. armigera. A identificação e o papel funcional das proteínas de ligação nos diferentes estádios de desenvolvimento de H. armigera, facilitará a elucidação do mecanismo de ação da proteína Cry1Ac e poderá ajudar a propor estratégias que retardem a evolução da resistência dos insetos às cultivares transgênicas que expressam esta proteína. / Helicoverpa armigera is a highly polyphagous pest and attacks important crops worldwide. The control of this pest is carried out primarily by chemical insecticides. However, the indiscriminate use of chemical control, led to pest populations to develop resistance to most of the chemical insecticides used for their control, making it difficult to management in the field. In addition to chemical control, H. armigera has been done by transgenic crops expressing Cry1Ac toxin from Bacillus thuringiensis (Bt) or by biopesticides that contains Cry1Ac or other toxins. However, studies have demonstrated a susceptibility decrease of H. armigera to Cry toxins with their larval development increase. The most common mechanism of resistance used by insects against Cry toxins is the reduced toxin binding to receptors present on the membrane, leading to a lower binding affinity of the toxin to intestinal receptors. Thus, the objective of this work was to evaluate the susceptibility of different instar larvae of H. armigera to Cry1Ac toxin and to correlate with the Cry1Ac toxin binding capacity to BBMV isolated from all larval instar. Furthermore, by pull-down techniques and liquid chromatography coupled to mass spectrometry analysis, to identify the proteins involved in the Cry1Ac toxin interaction in the second and fifth instars of H. armigera. A significant reduction in the susceptibility of the late instars of H. armigera to Cry1Ac toxin was observed compared to early instars. LC50 estimated values ranged from 31.1 to 2525.7 ng of toxin/cm2 of diet in first and sixth instar larvae, respectively. These results point a difference of 80-fold in the susceptibility to Cry1Ac toxin from late to first larval instar. In the ELISA binding assays results to BBMV of the different instars was found a total decrease in the binding capacity of Cry1Ac toxin to BBMVs from late instars compared to BBMV from early instars, presenting an apparent binding affinity of 3.88 times lower in the last instars than the first. Thus, a clearly correlation between Cry1Ac toxicity and binding toxin affinity to H. armigera BBMV has been demonstrated. The pull-down assays demonstrated a different pattern of the interaction between Cry1Ac toxin with the second and fifth instars. The protein phosphatase alkaline (ALP) was identified only in the second instar, as well as, other membrane proteins, as prohibitin and an ion channel protein, which may be involved for higher toxicity of Cry1Ac in early instars of H. armigera. The identification and functional role of binding proteins in the different stages of development of H. armigera will facilitate the elucidation of the Cry1Ac toxin mechanism of action and will may help to propose strategies that delay the insect resistance evolution to transgenic crops that express this protein. / FAPESP: 2015/24330-5

Aminopeptidase N

Fosfatase alcalina

Controle biológico

Ensaios de ligação

Espectrofotometria de massa

Cromatografia líquida

Imunoprecipitação

Biological control

Binding assay

Alkaline phosphatase

Mass spectrometry analysis

Liquid chromatography

Pull-down

Prospecção bioquímica da biomassa global da cianobactéria tóxica Microcystis aeruginosa BB005

Copelli, Thalita da Silva

12 February 2015

Cianobactérias são microrganismos capazes de produzir substâncias com potencial biológico e biotecnológico. Tais substâncias podem acarretar em malefícios, causados pelas toxinas, ou ter em sua composição substâncias benéficas como carotenoides, lipídeos e enzimas, de interesse biotecnológico. Assim, esse trabalho teve como objetivo avaliar a toxicidade e prospectar componentes presentes na biomassa global da cianobactéria Microcystis aeruginosa BB005. A toxicidade foi avaliada através de bioensaios com Daphnia magna, e a biomassa seca foi caracterizada por análises dos ésteres metílicos de ácidos graxos (EMAGs), determinação de carotenoides, obtenção do perfil proteico por eletroforese e hidrólise ácida de carboidratos. Também foi empregada uma metodologia de separação adsortiva por bolhas a fim de separar o pigmento ficocianina e enzimas de interesse biotecnológico (e.g. fosfatase alcalina e lipase) utilizando o sobrenadante de um cultivo. Apesar de ter sido possível quantificar a produção de toxinas pela cepa BB005, os ensaios ecotoxicológicos não permitiram estabelecer uma correlação entre a concentração de toxina e a imobilidade dos organismos. O perfil de EMAGs apresentou preponderância de PUFAs (ω-ácidos graxos) sendo que os linolenatos corresponderam a 25% do total. O teor de carotenoides encontrado durante a purificação dos lipídeos transesterificados e expresso como β-caroteno foi de 6,66 mg/g de biomassa seca. A eletroforese mostrou pelo menos 15 bandas distintas de proteínas e o perfil cromatográfico dos hidrolisados de carboidratos mostrou maior concentração do monossacarídeo glucose e de um dissacarídeo de glucose, possivelmente maltose. A separação de proteínas por espumação apresentou uma correlação direta entre fluxo de nitrogênio e a fração de espuma coletada. O fator de enriquecimento para a ficocianina foi de 41,69 utilizando fluxo de 20 mL/min de N2. Para a enzima fosfatase alcalina, os melhores resultados foram obtidos para o fluxo de 120 mL/min de N2, que apresentou fator de enriquecimento e de purificação de 5,25 e 2,85, respectivamente. Portanto, este trabalho demonstrou a importância de investigações sobre os componentes oriundos de M. aeruginosa, sobretudo dos EMAGs incomuns, a quantidade expressiva de carotenos e ainda da separação da ficobilina e de enzimas chave nos processos bioquímicos utilizando o processo por espumação. / Cyanobacteria are microorganisms able to produce substances with high biological and biotechnological potential. These substances may cause disorders because of the toxins or may be composed by beneficial substances such as carotenoids, lipids and enzymes of technological interest. Hence, the scope of the current research was centered in the toxicity evaluation or prospect the substances from the Microcystis aeruginosa cyanobacterium biomass – BB 005. Daphnia magna was used in the toxicity bioassays and the cyanobacterium dry biomass was characterized by the transesterified lipids analysis, carotenoid determination, electrophoretic profile for proteins and acid hydrolysis of polysaccharides. The foam fractionation methodology was performed to separate the phycocyanin pigment and enzymes (e.g. alkaline phosphatase and lipase), using the supernatant from a liquid culture of the cyanobacterium. Although it was possible to quantify the production of toxins by BB005 strain, the ecotoxicological tests have no establish a correlation between toxin concentration and the immobility of organism bodies.The methyl esters profile in which there was a large amount of PUFAs (ω-fatty acids) with 25% of linolenates. The carotenoid content found during the lipids transesterificaction, expressed as β – carotene, was 6.6 mg/g of dry mass. The electrophoresis indicated at least 15 distinct bands of proteins and the chromatographic profile from the native polymeric carbohydrates indicated higher concentration of monosaccharide glucose and a glucose disaccharide, possible maltose. Proteins separation through foaming showed a direct correlation between the nitrogen flow and the collected foam. The phycocianin enrichment factor was high, 41.69, at a 20 mL/min N 2 flow. While in the case of alkaline phosphatase the best result was attained in the 120 mL/min of N2 flow which lead to enrichment and purification factors equal to 5.25 and 2.85 respectively. Therefore, this research has demonstrated the importance of the investigation on compounds from the M. aeruginosa entire biomass, especially the methyl esters from less common and highly insaturated fatty acids, an expressive content of carotenoids and, furthermore, the separation of phycobillin and key- enzymes for biochemical processes, that were feasibly and primarily demonstrated in this experiment by the use of foaming procedure. / 5000

Ácidos graxos

Esteres

Carotenóides

Fosfatase alcalina

Flotação

Separação (Tecnologia)

Toxicologia ambiental

Tecnologia ambiental

Fatty acids

Esters

Carotenoids

Alkaline phosphatase

Flotation

Separation (Technology)

Environmental toxicology

Green technology