Isolamento e caracterização funcional de uma fosfolipase A2 de Bothrops jararaca: avaliação do potencial antitumoral e inflamatório / Isolation and functional characterization of a phospholipase A2 from Bothrops jararaca snake venom: evaluation of its antitumor and inflammatory potential

Araújo, Rafhaella Carolina Cedro

02 December 2014

As fosfolipases A2 (PLA2s) catalisam a hidrólise de ácidos graxos na posição sn-2 das membranas fosfolipídicas e liberam, como subprodutos, ácidos graxos livres. As PLA2s do grupo IIA são encontradas em peçonhas de serpentes da família Viperidae e desempenham diversas atividades apresentando potencial miotóxico, neurotóxico, hemolítico, edematogênico, citotóxico, hipotensivo, anticoagulante, inibição/ativação da agregação plaquetária, bactericida e pró-inflamatório. Esse trabalho teve como objetivo o isolamento e a caracterização funcional de uma PLA2 isolada da peçonha de Bothrops jararaca. Para a purificação dessa proteína, denominada BJ-PLA2-I, foram necessários três passos cromatográficos consecutivos: cromatografia de exclusão molecular em Sephacryl S-200, cromatografia de troca iônica em Source TM 15Q/50mL e cromatografia de troca iônica em MonoQ TM 5/50 GL. A BJ-PLA2-I apresentou elevado grau de pureza por SDS-PAGE e por cromatografia de fase reversa C18, em HPLC. Apresentou ainda, características ácidas, com pI em torno de 4,4 e teve a sua massa molecular determinada por dois métodos, obtendo-se valores bem próximos de 14,8 kDa (SDS-PAGE) e 14,2 kDa (MALDI-TOF). Esse fato é comum considerando que a espectrometria de massas é um método mais preciso e determina de maneira mais exata a massa molecular. O sequenciamento N-terminal da BJ-PLA2-I resultou em 60 resíduos de aminoácidos. O alinhamento múltiplo com outras fosfolipases A2 de serpentes do mesmo gênero mostrou similaridade entre elas, mostrando identidade de 100% com a BJ-PLA2, fosfolipase A2 Asp-49, também isolada da Bothrops jararaca. Esse dado levanta a hipótese de que a BJ-PLA2-I purificada neste trabalho e a BJ-PLA2 se tratam da mesma proteína, entretanto essa hipótese só poderá ser confirmada quando a sequência completa da BJ-PLA2-I for obtida. Outros dados encontrados neste trabalho reforçam essa hipótese, isso porque, avaliando a atividade fosfolipásica, o efeito sobre as plaquetas e o pI, tanto a BJ-PLA2-I quanto a BJ-PLA2 apresentaram características semelhantes. A BJ-PLA2-I, sendo uma Asp-49, mostrou alta atividade catalítica e efeito inibidor da agregação plaquetária induzida por ADP (20,5 ?g/mL inibiu 50 % da agregação plaquetária). Ela também foi capaz de induzir a migração leucocitária após a administração de diferentes concentrações (5, 10 e 20 ?g/mL) da BJ-PLA2-I. Esse dado também foi encontrado no ensaio em que a concentração de 10 ?g/mL foi fixada e variou-se o tempo de 2, 4 e 24 horas, observando-se principalmente a migração de neutrófilos. Além disso, verificou-se a liberação das citocinas IL-6 e IL-1?, de proteínas totais e de prostaglandina E2 na reação inflamatória induzida pela BJ-PLA2-I. No entanto, não foi observado a produção de TNF-?, IL-10 e leucotrieno B4. A BJ-PLA2-I caracterizou-se como uma PLA2 pró-inflamatória, produzindo inflamação local aguda. A BJ-PLA2-I foi avaliada quanto ao seu potencial antitumoral em três linhagens celulares distintas (PBMC, HL-60 e HepG2). Observou-se que a enzima em questão possui baixo potencial antitumoral para a linhagem HL-60, reduzindo o número de células tumorais em apenas cerca de 20% nas concentrações testadas. Verificou-se pequena alteração na viabilidade celular das células de PMBC, nas maiores concentrações testadas (160 e 80 ?g/mL) e, na linhagem HepG2 não foi encontrada nenhuma alteração. Concluindo, as informações adquiridas neste trabalho são de suma importância para a melhor compreensão dos mecanismos envolvidos nas atividades biológicas desempenhadas pelas PLA2s. Além disso, a BJ-PLA2-I pode servir como modelo molecular para a formulação de fármacos mais eficazes a serem utilizados no tratamento de várias doenças. / Phospholipases A2 (PLA2s) catalyze the hydrolysis of fatty acids in the sn-2 position of membrane phospholipids, releasing free fatty acids as by-products. PLA2s of group IIA are found in snake venoms of the Viperidae family and perform various activities, including myotoxic, neurotoxic, hemolytic, edematogenic, cytotoxic, hypotensive, anticoagulant, inhibition/activation of platelet aggregation, bactericidal and proinflammatory effects. This work aimed at the isolation and functional characterization of a PLA2 isolated from Bothrops jararaca venom. For the purification of this protein, called BJ-PLA2-I, three consecutive chromatographic steps were used (size exclusion chromatography on Sephacryl S-200, ion exchange chromatography on Source 15Q/50 mL, ion exchange chromatography on MonoQ 5/50 GL). Confirmation of the purity of BJ-PLA2-I was evaluated by SDS-PAGE and reverse phase HPLC using a C18 column. BJ-PLA2-I has acidic characteristics, with pI around 4.4, and its molecular mass was determined by two methods, obtaining values close to 14.8 kDa (SDS-PAGE) and 14.2 kDa (MALDI-TOF). The N-terminal sequencing of BJ-PLA2-I resulted in 60 amino acid residues. Multiple alignment with other phospholipases A2 of snakes of the same genus showed high similarity between them, showing 100% identity with BJ-PLA2, an Asp-49 phospholipase A2 previously isolated from Bothrops jararaca venom. This finding raises the possibility that the PLA2 purified in this work is the same protein previously described (BJ-PLA2), however, this assumption can only be confirmed when the complete sequence of BJ-PLA2-I is obtained. Other data obtained in this study support this hypothesis, considering that the phospholipase activity, the effect on platelets and pI of both BJ-PLA2-I and BJ-PLA2 showed to be similar. BJ-PLA2-I, being an Asp-49 PLA2, showed high catalytic activity and inhibitory effect on the platelet aggregation induced by ADP (20.5 ?g/mL inhibited 50% of the platelet aggregation). It was also able to induce leukocyte migration after the administration of different concentrations (5, 10 and 20 ?g/mL) of BJ-PLA2-I. This fact was also found when the concentration of 10 ?g/mL was fixed and response times were varied (2, 4 and 24 hours), observing especially neutrophil migration. Furthermore, there was a release of IL-6 and IL-1?, total proteins and prostaglandin E2 in the inflammatory reaction induced by BJ-PLA2-I, however, the production of TNF-?, IL-10 and leukotriene B4 was not observed. BJ-PLA2-I was characterized as a proinflammatory PLA2 producing acute local inflammation. BJ-PLA2-I was evaluated for its antitumor potential on three different cell lines (PBMC, HL-60 and HepG2). It was observed that this enzyme showed a low antitumor potential on HL-60 tumor cell line, reducing the number of tumor cells in only about 20% at the concentrations tested. There was little change in cell viability of PBMC cells in the higher concentrations tested (80 and 160 ?g/mL), but no change was found on HepG2 tumor cell line. In conclusion, the information obtained in this work are of utmost importance for better understanding the mechanisms involved in the biological activities induced by PLA2s. Furthermore, BJ-PLA2-I may serve as a molecular model for the formulation of more effective drugs to be used in the treatment of various diseases.

Acidic phospholipase A2

Agregação plaquetária

Antitumor

Antitumoral

Asp-49

Asp-49

BJ-PLA2-I

BJ-PLA2-I

Bothrops jararaca

Bothrops jararaca

Fosfolipase A2 ácida

Inflamação

Inflammation

Isolamento

Isolation

Platelet aggregation

Compostos bioativos fenólicos de frutos nativos da famí­lia Myrtaceae: Avaliação da bioacessibilidade e do potencial funcional relacionado às doenças cardiovasculares / Bioactive phenolic compounds of native fruits from Myrtaceae family: Evaluation of bioaccessibility and functional potential related to cardiovascular diseases

Santiago, Gabriela de Lima

05 April 2018

As doenças cardiovasculares (DCV) são responsáveis pela maioria das mortes ocorridas em todo o mundo. Os riscos para o desenvolvimento destas patologias podem ser amenizados, em parte, por meio de uma dieta rica em alimentos de origem vegetal. Neste sentido, os frutos nativos brasileiros, como os pertencentes à família Myrtaceae, podem contribuir para melhorar a qualidade da alimentação, pois apresentam altos teores de compostos bioativos, entre eles, os fenólicos (CBF). Pouco se sabe sobre os efeitos dos polifenóis destes frutos para redução do risco de desenvolvimento das DCV. Sendo assim, este trabalho buscou avaliar a bioacessibilidade dos CBF presentes em polpas de cambuci e jabuticaba e seus efeitos in vitro sobre mecanismos de ação relacionados às DCV. Para tanto, extratos ricos em polifenóis foram obtidos a partir de extrações em fase sólida (C18 e PA) das polpas de ambos os frutos, submetidas ou não à simulação da digestão gastrointestinal. Estes extratos tiveram seus efeitos inibitórios sobre a atividade da Enzima Conversora de Angiotensina I (ECA) e a agregação plaquetária induzida por adenosina difosfato avaliados in vitro. De acordo com os resultados obtidos, a digestão in vitro foi capaz de liberar os CBF da matriz alimentar. Tal bioacessibilidade parece ter sido importante apenas para a inibição da agregação plaquetária, uma vez que a capacidade inibitória destes compostos sobre a atividade da ECA não melhorou depois da digestão in vitro. Quanto aos resultados obtidos pelos extratos provenientes das colunas PA e C18, observa-se que as maiores concentrações de taninos nestes últimos não foram suficientes para melhorar a capacidade antiagregante, mas foram importantes para aumentar a inibição da atividade da ECA. Comparando-se as respostas apresentadas pelos dois frutos, os CBF presentes no cambuci exibiram, predominantemente, potenciais anti-hipertensivo e antiagregantedo maiores do que os da jabuticaba. Neste contexto, o consumo de cambuci e jabuticaba, bem como a utilização de seus polifenóis purificados, podem ser adjuvantes para a redução dos riscos relacionados ao desenvolvimento das DCV. / The cardiovascular diseases (CVD) are the leading cause of death worldwide. The risk of development of these disorders can be reduced, partially, by a vegetal-based diet. In this way, the Brazilian native fruits from Myrtaceae family may contribute to improve the diet quality, once they have high quantity of bioactive compounds, such as the phenolic (PC). The knowledge about the cardioprotective effects of consuming these fruit polyphenols is limited, so this study aimed to evaluate the bioaccessibility of the cambuci and jaboticaba PC and their in vitro potential on CVD-related mechanisms. First, gastrointestinal digestion simulation of each fruit pulp was done, and then the polyphenols rich extracts were obtained by solid phase extractions, before and after the pulps digestion. The polyphenols rich extracts had their phenolic concentrations determined and were used to evaluate the capacity of PC in inhibit the Angiotensin Converting Enzyme (ACE) activity and the platelet aggregation induced by ADP. The results were expressed as IC50, considering the total phenolic content per milliliter of reaction. According to the results, the in vitro digestion process was able to release the polyphenols from the food matrix. Therefore, the bioaccessibility had no significant effect on ACE activity, but decreased the IC50 values of platelet aggregation. In relation to the extracts from PA and C18 columns, the higher tannin concentration In comparison to the IC50 values presented by PA extracts, the higher concentrations of tannins in the last one were not enough to improve the antiaggregant effect, but were important to increase the inhibition of ACE activity. Cambuci polyphenols presented higher antihypertensive and antiaggregant potentials than the jaboticaba compounds. In this respect, the ingestion of cambuci and jaboticaba and the use of their purified polyphenols can be of particular importance in reducing the risk for the CVD development.

Agregação plaquetária

Angiotensin converting enzyme

Cambuci (Campomanesia phaea O. Berg.)

Cambuci (Campomanesia phaea O. Berg.)

Compostos fenólicos

Enzima conversora de angiotensina I

Phenolic compounds

Platelet aggregation

Caractérisation de métabolites oxygénés issus de l’acide alpha-linolénique : Effets anti-agrégants et anti-inflammatoires / Characterization of oxygen metabolites from alpha-linolenic acid : Effect of anti-aggregatory and anti-inflammatory

Liu, Miao

10 July 2013

Les acides gras de la série n-3 et notamment l’acide docosahexaénoïque (DHA) jouent un rôle important dans la prévention des maladies cardiovasculaires. Un de ses métabolites, la protectine DX (PDX), qui est un isomère de la protectine D1 (PD1), inhibe l’agrégation des plaquettes sanguines. D’autres composés similaires appelés "poxytrins", qui possèdent aussi un triène conjugué avec une géométrie E,Z,E, ont également été synthétisés à partir d'autres acides gras polyinsaturés (AGPI) via la lipoxygénase de soja. Ces composés présentent des propriétés anti-agrégantes en inhibant la cyclo-oxygénase plaquettaire et le récepteur du thromboxane A2. Dans cette thèse, nous décrivons de nouveaux composés dihydroxylés synthétisés par la 15-lipoxygénase de soja à partir de l’acide alpha-linolénique (18:3n-3), un acide gras polyinsaturé indispensable consommé au niveau du gramme chez l’Homme adulte. Il est converti en acides gras monohydroxylés et dihydroxylés. Ces composés ont été séparés par HPLC en phase inverse et caractérisés par GC-MS après dérivation adéquate. Un acide gras monohydroxylé, majoritaire, l’acide 13(S)-octadécatriénoïque et quatre acides gras dihydroxylés ont été détectés. Ces derniers présentent tous un spectre UV caractéristique avec une absorption maximale à 270 nm et deux épaulements à 260 et 280 nm. Les spectres UV de deux d'entre eux sont superposables à celui de la PDX, ce qui suggère une géométrie E,Z,E des doubles liaisons de leur triène. La caractérisation complète de ces composés a été réalisée par RMN à haut champ et par GC-MS. Ce sont les acides 9(R),16(S)-dihydroxy-octadéca-10E,12E,14E-triénoïque, 9(S),16(S)-dihydroxy-octadéca-10E,12E,14E-triénoïque, 9(S),16(S)-dihydroxy-octadéca-10E,12Z,14E-triénoïque et 9(R),16(S)-dihydroxy-octadéca-10E,12Z,14E-triénoïque. Ils sont également synthétisés par la 15 lipoxygénase recombinante humaine de type 2. Ces composés dihydroxylés 9,16-diHOTEs ont été testés sur les plaquettes isolées à partir du sang humain. Nous avons observé que seules les molécules ayant la géométrie E,Z,E du triène conjugué inhibent l'agrégation plaquettaire induite par le collagène et inhibent la cyclooxygénase-1 (COX-1) de mouton. Les propriétés anti-inflammatoires de ces produits ont également été étudiés. Tous les isomères 9,16-diHOTEs, possédant un triène conjugué avec une géométrie E,Z,E, inhibent la COX-2 recombinante humaine et seul l’acide 9(R),16(S)-dihydroxy-octadéca-10E,12Z,14E-triénoïques inhibe la 5-lipoxygénase des leucocytes, siège de la synthèse des leucotriènes issus de l’acide arachidonique. En conclusion, les composés dihydroxlés possédant un triène conjugué E,Z,E, issus du 18:3n-3, ainsi que la PDX, inhibent l’activité des COX-1 et 2, et seraient anti-agrégants et anti-inflammatoires. Ces résultats donnent des perspectives pharmacologiques aux recommandations nutritionnelles promouvant la consommation d’acide alpha linolénique. / N-3 fatty acids, especially docosahexaenoic acid (DHA), play an important role in the prevention of cardiovascular diseases. One metabolite of DHA, protectin DX (PDX), an isomer of protectin D1 (PD1) (Chen P et al., 2009),possesses inhibits blood platelet aggregation. Similar compounds called "poxytrins", which have a conjugated triene with a E,Z,E geometry have also been synthesized from other polyunsaturated fatty acids (PUFA) by soybean lipoxygenase. They have anti-aggregating properties by inhibiting platelet cyclooxygenase and thromboxane A2 receptor (Chen P et al., 2011). In this thesis, we describe new dihydroxy compounds synthesized by the soybean 15-lipoxygenase from alpha-linolenic acid (18:3n-3), an essential PUFA that is consumed in the gram range in human adults . It is converted into monohydroxylated and dihydroxylated derivatives. These compounds were separated by reverse phase high performance liquid chromatography (HPLC) and characterized by gas chromatography-mass spectrometry (GC-MS) after appropriate derivatization. A main monohydroxylated fatty acid, 13(S)-octadecatrienoic acid (13(S)-OH-18:3) and four dihydroxylated fatty acids were detected. The last ones have all a characteristic UV spectrum with a maximum absorbance at 270 nm with two shoulder peaks at 260 and 280 nm. The UV spectra from two of them are superimposable to that of PDX, suggesting a E,Z,E geometry for their conjugated triene. The complete characterization of these compounds was performed by high field nuclear magnetic resonance (NMR) and by GC-MS. These are the 9(R),16(S)-dihydroxy-octadeca-10E,12E,14E-trienoic, 9(S),16(S)-dihydroxy-octadeca-10E,12E,14E-trienoic, 9(S),16(S)-dihydroxy-octadeca-10E,12Z,14E-trienoic and 9(R),16(S)-dihydroxy-octadeca-10E,12Z,14E-trienoic acids. They can also be synthesized by the (type 2) 15 human recombinant lipoxygenase. These dihydroxylated compounds (9,16-diHOTEs)were tested on isolated human blood platelets. We observed that only molecules containing a conjugated triene with a E,Z,E geometry are able to inhibit platelet aggregation induced by collagen, and inhibit sheep cyclooxygenase-1 (COX-1). The anti-inflammatory properties of these products were also studied. All 9,16-diHOTEs isomers having a conjugated triene with a E,Z,E geometry, inhibit human recombinant cyclooxygenase-2 (COX-2) and only 9(R),16(S)-dihydroxy-octadeca-10E,12Z,14E-trienoic acid inhibits polymorphonuclear leukocytes (PMN) 5-lipoxygenase which is involved in the leukotriene synthesis from arachidonic acid. In conclusion, the E,Z,E dihydroxlated compounds from 18:3n-3, as well as PDX, inhibiting the COX-1 and 2 activities appear to be anti-aggregatory and anti-inflammatory agents. These results provide pharmacological perspectives to nutritional recommendations promoting the intake of alpha-linolenic acid.

Biosciences

Acide gras

Acide docosahéxaénoïque

Spectrométrue de masse

Résonance magnétique nucléaire

Agrégation plaquettaire

Leucocytes humains

Biosciences

Fatty acid

Docosahexaenoic acid

High performance liquid chromatography

Mass spectrometry

Nuclear magnetic resonance

Platelet aggregation

Human leukocytes

572.507 2

Rôle des lipides oxydés dans la régulation de l'activation plaquettaire par les lipoprotéines de haute densité (HDL) plasmatiques et implication dans le diabète de type 2 / Role of oxidized lipids in the regulation of platelet activation by plasma highdensity lipoproteins (HDL) and involvement in type 2 diabetes

Lê, Quang Huy

20 October 2015

Le diabète de type 2 (DT2) est associé à un risque athéro-thrombotique élevé, en partie dû à l'hyperactivation plaquettaire et aux dyslipoprotéinémies. Les lipoprotéines de haute densité (HDL) possèdent des propriétés anti-athérogènes et subissent des modifications glycoxydatives lors du DT2. Notre objectif a été de déterminer les effets d'HDL glycoxydées in vitro ou de DT2 sur les plaquettes sanguines humaines et de déterminer leur contenu en lipides oxydés. Les HDL glycoxydées possèdent des proportions moindres d'acides linoléique et arachidonique dans les phospholipides (PL) et esters de cholestérol, des concentrations plus élevées de dialdéhyde malonique et des principaux acides gras hydroxylés (AGOH) dont les 9-HODE, 13- HODE et 15-HETE dans toutes les classes lipidiques, en particulier dans les PL ainsi que des concentrations très faibles de vitamine E comparativement aux HDL contrôles. Les HDL glycoxydées in vitro et de patients DT2 inhibent de façon dose-dépendante l'agrégation plaquettaire induite par le collagène via le récepteur SR-BI. Ces HDL glycoxydées diminuent la phosphorylation des p38 MAPK et cPLA2 plaquettaires. D'autre part, des HDL contrôles enrichies avec le PC(16:0/13-HODE) inhibent fortement l'agrégation comparativement aux HDL contrôles. De plus, les effets des sous-classes d'HDL, HDL 2 & 3, de DT2 et de témoins ont été testés sur l'agrégation plaquettaire. Les HDL2 de DT2 possèdent des concentrations d'AGOH plus élevées que les HDL3 de DT2 et tendent à inhiber plus l'agrégation plaquettaire. En conclusion, nos résultats montrent que les HDL glycoxydées de patients diabétiques ne perdent pas leurs propriétés anti-agrégantes, qui pourraient être médiées par certaines PL oxydés / Type 2 diabetes (T2D) is associated with a high athero-thrombotic risk, partly due to platelet hyperactivation and dyslipoproteinemia. High-density lipoproteins (HDL) possess antiatherogenic properties and undergo glycoxidation changes in T2D. Our objective was to determine the effects of glycoxidized HDL in vitro or from T2D patients on human blood platelets and to identify their oxidized lipid species. Compared to control HDL, glycoxidized HDL have lower proportions of linoleic and arachidonic acids in phospholipids (PL) and cholesteryl esters, higher concentrations of malondialdehyde and main hydroxylated fatty acid (HOFA) including 9-HODE, 13-HODE and 15-HETE in all lipid classes, especially in PL, and very low concentrations of vitamin E. In vitro glycoxidized and T2D HDL dose-dependently inhibit platelet aggregation induced by collagen via the SR-BI receptor. Glycoxidized HDL decrease the phosphorylation of platelet p38 MAPK and cPLA2. On the other hand, control HDL enriched with oxidized phospholipids i.e. PC(16:0/13-HODE) strongly inhibit platelet aggregation compared to controls. Moreover, the effects of HDL subclasses, HDL 2 & 3, from T2D patients and healthy controls were tested on platelet aggregation. T2D HDL2 have higher concentrations of HOFA than T2D HDL3 and tend to inhibit platelet aggregation to a greater extent. In conclusion, our results show that T2D glycoxidized HDL do not lose their anti-aggregatingproperties and are even more effective than control HDL. These anti-aggregatory effects could be partly due to some oxidized PL species

Diabète de type 2

HDL glycoxydées

Agrégation plaquettaire

Acides gras hydroxylés

Phospholipides oxydés

Sous-classes d’HDL

Type 2 diabetes

Glycoxidized HDL

Platelet aggregation

Hydroxylated fatty acids

Oxidized phospholipids

HDL subclasses

572

Efeitos do veneno da serpente Bothrops jararaca sobre a agregação e secreção plaquetária de plaquetas humanas e de camundongos / Effects of Bothrops jararaca venom (BjV) on the aggregation and secretion of washed mouse and human platelets

Rosa, Jaqueline Gomes

14 November 2018

Trombocitopenia e diminuição da função plaquetária são achados comuns em pacientes picados por serpentes do gênero Bothrops. Sabe-se que o veneno de Bothrops jararaca (VBj) apresenta compostos com características pró e anti-agregantes plaquetárias, porém existem poucos estudos sobre a influência do veneno total assim como das principais famílias de proteínas que o compõem sobre as funções plaquetárias. A utilização de modelos experimentais é essencial para entender as desordens plaquetárias em humanos que culminam em sangramentos diversos. Portanto, o objetivo deste estudo foi (i) comparar as respostas ex vivo de plaquetas lavadas de humanos e de camundongos frente ao VBj, assim como entender a participação de serinaproteinases (SVSP) e metaloproteinases (SVMP) presentes no veneno sobre a agregação dessas plaquetas; e (ii) delimitar dentro do complexo proteico do veneno os compostos que induzem a trombocitopenia em camundongos após 3 horas do início do envenenamento botrópico. As plaquetas lavadas de humanos e camundongos BALB/c, C57BL/6 e do mutante natural pérola (Ap3b1-/-) apresentaram respostas de agregação máxima ao VBj na concentração de 24,4 ?g/mL, porém esta concentração provocou uma agregação menos intensa em plaquetas humanas quando comparada àquela observada nas linhagens BALB/c e C57BL/6. Mesmo em plaquetas de camundongos pérolas, deficientes em corpos densos plaquetários, o VBj se mostrou um potente agonista, promovendo a agregação plaquetária sem a necessidade da secreção do conteúdo granular. A ação agonista do veneno promoveu a secreção de ATP presente nos corpos densos plaquetários de humanos e das linhagens BALB/c e C57BL/6 de forma tão intensa quanto à provocada pela trombina, assim como a secreção de PF4 presente nos grânulos ? de plaquetas humanas e de camundongos BALB/c. Já em relação à secreção lisossomal, observou-se que as plaquetas humanas secretam níveis mais baixos de ?-hexosaminidase quando estimuladas com VBj do que pela trombina, enquanto que em plaquetas de camundongos BALB/c a secreção lisossomal ao VBj foi superior à constatada com a trombina. Os baixos níveis de lactato desidrogenase (LDH) no sobrenadante das plaquetas estudadas mostraram ausência de atividade direta citotóxica pelo VBj. Para verificar se as principais classes de famílias de enzimas do VBj, SVMP e SVSP, estavam envolvidas na ativação plaquetária ex vivo, elas foram inibidas com Na2EDTA (13 mM) e AEBSF (8 mM), respectivamente. Observou-se que em plaquetas humanas as serinaproteases são importantes para a agregação ex vivo, enquanto a agregação das plaquetas de camundongos BALB/c foi independente dessa classe de toxinas. Os resultados dos ensaios in vivo demonstraram que as proteínas do VBj com peso molecular inferior a 50 kDa (UF < 50 kDa) são importantes para o estabelecimento da trombocitopenia em camundongos BALB/c que receberam essa fração por via subcutânea e que esse quadro é independente de manifestações hemorrágicas e do desenvolvimento de coagulopatia durante o envenenamento botrópico. A caracterização dos compostos presentes no UF < 50 kDa foi realizada por espectrometria de massas e foi observada a presença predominante de metaloproteinases (37%) e proteínas similares às lectinas do tipo-C (33%), enquanto serinaproteases (17%), fosfolipases A2 (10%) e outros compostos (3%) somaram 30% da fração UF < 50 kDa. Em conclusão, o veneno é um potente agonista plaquetário que promove agregação, aglutinação e secreção de plaquetas humanas e de camundongos, independente da secreção de corpos densos plaquetários, e a fração do veneno responsável pela trombocitopenia em camundongos BALB/c tem peso molecular menor que 50 kDa / Thrombocytopenia and platelet dysfunction are common findings in patients bitten by Bothrops jararaca snakes. Pro- and anti-aggregating toxins have been isolated from Bothrops jararaca venom (BjV), but only few studies have been carried out about the effects of crude BjV and its main families of enzymes on platelet function ex vivo, as well as to understand their relevance to the pathophysiological events that occur during B. jararaca envenomation. Animal models have been used to understand platelet disorders in humans that culminate in bleeding manifestations. Thus, the aim of this study was to investigate (i) the effects of BjV, and snake venom serine proteinases (SVSP) and snake venom metalloproteinases (SVMP) contained therein, on aggregation and secretion in suspensions of washed human and mouse platelets, and (ii) to determine the BjV fractions, obtained by ultrafiltration, that induce thrombocytopenia in BALB/c mice after 3 h of administration of Bothrops envenomation. Washed platelets from humans and BALB/c, C57BL/6 and pearl (Ap3b1-/-) mice showed maximal aggregation responses to BjV at the concentration of 24.4 ?g/mL. However, this concentration aggregated less intensely platelets from humans than BALB/c or C57BL/6 mice. Even in pearl mouse platelets, which are deficient in dense bodies, BjV proved to be a potent agonist, promoting platelet aggregation without the requirement of granule content secretion. Nonetheless, BjV induced secretion of ATP, present in dense bodies, and PF4, present in ? granules, in the same extent as thrombin, from platelets of humans and mice. In regard to lysosomal secretion, it was observed that human platelets secreted low ?-hexosaminidase levels when stimulated by BjV than thrombin, whereas in BALB/c platelets higher secretion was induced by BjV than by thrombin. Release of lactate dehydrogenase (LDH) was similar between BjV and thrombin, evidencing the absence of cytotoxic activity by BjV on platelets. Inhibition of SVMP and SVSP, using Na2EDTA (13 mM) and AEBSF (8 mM), respectively, demonstrated that SVSP are important for ex vivo aggregation only in human platelets, whilst BALB/c platelet aggregation was independent of both of them. In in vivo studies, only BjV toxins with molecular weight less than 50 kDa (UF50) caused thrombocytopenia when administered s.c. to BALB/c mice, and it was independent of hemorrhagic manifestations and consumptive coagulopathy. Characterization by mass spectrometry of these toxins present in UF50 showed the predominant presence of SVMP (37%) and type-C lectin proteins (33%) were observed, while SVSP (17%), phospholipases A2 (10%) and other proteins (3%) accounted for the remaining toxins in UF50. In conclusion, BjV is a potent platelet activating agent that promotes aggregation, agglutination and secretion of human and mouse platelets, independent of secretion of dense platelet bodies, and the fraction of venom responsible for thrombocytopenia in BALB / c mice has a molecular weight less than 50 kDa

Agregação plaquetária

Blood platelets

Bothrops

Bothrops jararaca

Camundongos

Espectrometria de massas

Hermansky-Pudlak syndrome

Humans

Mass spectrometry

Mice

Plaquetas

Platelet aggregation

Platelet secretion

Secreção plaquetária

Seres humanos

Síndrome de Hermansky-Pudlak

Snake venoms

Thrombocytopenia

Trombocitopenia

Venenos de serpentes

Caracterização do precursor e da atividade de inibição da agregação plaquetária da BnP1 e de disintegrinas do veneno de Bothrops neuwiedi. / Characterization of the precursor and the inhibitory activity on platelet aggregation of BnP1 and disintegrins from Bothrops neuwiedi venom.

Furlan, Maria Stella

24 June 2010

Neste trabalho visamos otimizar o isolamento da BnP1, uma SVMP presente no veneno de B. neuwiedi, e isolar disintegrinas desse veneno, ambas originadas de precursores tipo P-II, analisando as seqüências de cDNA e a ação sobre plaquetas. A purificação da BnP1 foi por exclusão molecular e troca iônica; duas novas disintegrinas, D2 e D4, foram isoladas por cromatografia em fase reversa; e outra disintegrina, MS, foi caracterizada a partir do SDS-PAGE. As proteínas foram parcialmente seqüenciadas por espectrometria de massas. Diferentes cDNAs foram clonados a partir da glândula de veneno de B. neuwiedi e os precursores da BnP1 e MS se localizaram em um cluster que inclui SVMPs classe P-I e P-II. O precursor de D4 correspondeu a uma SVMP tipicamente P-II. A BnP1, ao contrário das disintegrinas, não inibiu a agregação plaquetária induzida por diferentes agonistas. Este trabalho indica ainda que a biossíntese de SVMPs da classe P-II pode envolver processamento de mRNA, um novo mecanismo de geração de diversidade das SVMPs. / The aim of this study was to optimize the isolation of BnP1, a SVMP from B. neuwiedi venom, and isolate new disintegrins from this venom, both originated from P-II class precursors, and analyze the sequence of their precursors and their action on platelets. BnP1 was isolated by size exclusion and anion-exchange chromatography; the disintegrins D2 and D4 by reverse-phase chromatography and MS was isolated from SDS-PAGE. These proteins were partially sequenced by mass spectrometry. Several SVMPs cDNAs were cloned from B. neuwiedi venom gland, and BnP1 and MS precursors localized in a cluster enclosing P-I and P-II SVMPs. MS cDNA was tipical of P-II class of SVMPs. BnP1, unlike the disintegrins, was not able to inhibit platelet aggregation induced by different agonists. This work suggested that the biosynthesis of class P-II SVMPs include mRNA processing as a further step to generate venom diversity.

Agregação plaquetária

Biossíntese

Biosynthesis

cDNA

cDNA

Disintegrinas

Disintegrins

Enzimas proteolíticas

Metalloproteinases

Metaloproteínases

Platelet aggregation

Poisons of animal origin

Proteolytic enzymes

Serpentes

Snakes

Toxinas em animal

Toxins in animal

Venenos de origem animal

Design, synthesis and pharmacological evaluation of original nitrobenzenesulfonylureas and sulfonylcyanoguanidines as thromboxane A2 receptor antagonists/Conception, synthèse et évaluation pharmacologique de nitrobenzènesulfonylurées et sulfonylcyanoguanidines en tant qu'antagonistes des récepteurs au thromboxane A2

Hanson, Julien

23 May 2007

Thromboxane A2 (TXA2) is an important mediator metabolized from arachidonic acid through the cyclooxygenase pathway, mainly in platelets and macrophages. It is a potent inducer of platelet aggregation and smooth muscle contraction. Its overproduction has been detected in pathologies such as stroke, asthma, myocardial infarction or atherosclerosis. The action of TXA2 is mediated by a specific G-protein coupled receptor (TP) of which two alternative spliced isoforms, TPalpha and TPbeta, have been described. The exact role of these two isoforms is not clearly understood. However, recent studies have described their implications in vascular physiology and pathology. The inhibition of the action of TXA2 on platelets and blood vessels would be interesting as original therapies against cardiovascular diseases. Consequently, the design of TP receptor antagonists remains of great interest in cardiovascular medicine. In the laboratory of medicinal chemistry (University of Liège, Belgium), several nitrobenzenesulfonylureas, derived from torasemide (a loop diuretic), have been previously described as TP receptor antagonists. Two compounds, BM573 and BM613 were among the most interesting molecules identified in that previous work. The present project is divided in two parts. First, we have determined the pharmacological properties of BM573 and BM613 as thromboxane synthase inhibitors and TP receptor antagonists, in vitro and in vivo. In our assays, these two compounds were proved to have high affinity for both TPalpha and TPbeta, to be potent antiplatelet agents, to inhibit thromboxane synthase and TP-mediated smooth muscle contraction. Additionally, they significantly reduced the size of the thrombus in a rat model of ferric chloride-induced arterial thrombosis. Consequently, we demonstrated that the TP receptor antagonists BM573 and BM613, belonging to the chemical family of nitrobenzenesulfonylureas, could be regarded as antiplatelet and antithrombotic agents potentially useful in thromboxane-related diseases such as stroke or myocardial infarction. Secondly, given the interesting pharmacological profile of BM573 and BM613, we have designed and synthesized several series of compounds derived from these two agents. We have evaluated the binding properties (affinity) of the first generation (+/- 35 original derivatives) of compounds on either TPalpha or TPbeta, transiently expressed in COS-7 cell lines. Additionally, we have measured the ability of our drugs to inhibit the intracellular calcium mobilization upon TPalpha or TPbeta stimulation. To confirm our results, we also assessed the antiplatelet properties of our drugs by means of determination of inhibition of human platelet aggregation. On the basis of the results obtained with these in vitro assays, we have synthesized and evaluated a second generation of derivatives (+/- 35 original compounds) and improved the selectivity of several original compounds for TP receptor isoforms. The originality of this work was to evaluate a large library of synthetic compounds on both TP receptor isoforms, using specific pharmacological tests. By means of structure-activity relationship studies, we were able to identify chemical groups implicated in selectivity and to propose lead compounds for development of highly specific TPalpha or TPbeta antagonists. Besides, we have identified an in vivo drug candidates for prevention of thrombosis and pathological platelet aggregation./Le thromboxane A2 (TXA2) est un métabolite de la cascade de lacide arachidonique (AA) par la voie des cyclooxygénases et de la thromboxane synthase, principalement formé dans les plaquettes et les macrophages. Le TXA2 est un puissant inducteur de lagrégation plaquettaire et de la contraction des muscles lisses vasculaires et bronchiques. Par ailleurs, une augmentation des taux en TXA2 a été constatée dans différentes pathologies : l'infarctus du myocarde, l'atherosclérose, les accidents vasculaires cérébraux, ou encore l'asthme. Laction du TXA2 sur les tissus résulte de la stimulation dun récepteur appartenant à la famille des récepteurs couplés aux protéines G. Ce récepteur au TXA2 (TP) présente deux isoformes générées par épissage alternatif, TPalpha et TPbeta. Le rôle physiologique exact de ces deux isoformes n'est pas encore connu. Cependant, de récents travaux ont mis en évidence leur importance, notamment dans la physiologie vasculaire et dans certaines pathologies. Linhibition de laction du TXA2 au niveau des plaquettes et des vaisseaux sanguins pourrait donc être une stratégie thérapeutique innovante pour traiter et prévenir les maladies cardiovasculaires. En conséquence, le développement dantagonistes des récepteurs TP reste dun grand intérêt en médecine cardiovasculaire. Des études de pharmacomodulation avaient permis au Laboratoire de Chimie Pharmaceutique (Université de Liège, Belgique) d'identifier des nitrobenzènesulfonylurées, dérivées du torasémide (un diurétique de lanse), présentant un puissant antagonisme des récepteurs TP. Parmi ceux-ci, deux composés, le BM573 et le BM613, faisaient parties des molécules les plus intéressantes identifiées au cours de ces précédentes recherches. Ce projet est divisé en deux parties. Premièrement, nous avons déterminé les propriétés pharmacologiques du BM573 et du BM613 en tant quinhibiteurs de la thromboxane synthase et antagonistes des récepteurs TP, in vitro et in vivo. Au cours de nos expériences, ces deux composés se sont révélés posséder une grande affinité pour TPalpha et TPbeta, être de puissants agents antiplaquettaires, des inhibiteurs de la thromboxane synthase et de la contraction des muscles lisses induite par le TXA2. En outre, lutilisation de ces produits dans un modèle de thrombose artérielle induite par le chlorure ferrique chez le rat a provoqué une réduction significative du thrombus formé. En conséquence, nous avons démontré que le BM573 et le BM613, appartenant à la famille chimique des nitrobenzenesulfonylurées, pouvaient être considérés comme des agents antiplaquettaires et antithrombotiques, potentiellement utiles en tant quagents thérapeutiques dans des pathologies associées au TXA2 telles que linfarctus du myocarde ou laccident vasculaire cérébral. Ensuite, nous nous sommes concentrés sur l'activité de cette famille de composés (les nitrobenzènesulfonylurées) vis-à-vis des deux isoformes du récepteur au thromboxane. Pour ce faire, nous avons conçu et synthétisé de nombreuses séries de composés dérivés du BM573 et du BM613. Nous avons tout dabord évalué laffinité de la première génération de composés (+/- 35 dérivés) sur des lignées cellulaires (COS-7) exprimant sélectivement soit TPalpha soit TPbeta. De plus, nous avons mesuré la capacité de ces composés à inhiber la mobilisation de calcium intracellulaire ([Ca2+]i) induite par la stimulation des deux isoformes TPalpha et TPbeta séparément. Nos résultats ont été confirmés sur agrégation plaquettaire humaine. Sur la base des résultats obtenus avec cette première génération de produits, nous avons synthétisé une seconde génération (+/- 35 dérivés) de composés, et avons réussi à augmenter la sélectivité en faveur de TPbeta pour certains produits. Loriginalité de ce travail réside dans le fait que nous avons évalué un nombre de produits importants sur TPalpha et TPbeta, au moyen de tests pharmacologiques spécifiques. Grâce à des études de relation structure-activité, nous avons identifié des groupements chimiques impliqués dans la sélectivité entre les deux isoformes. Nous pouvons donc proposer des structures "chef de file" pouvant être utiles pour le développement de composés hautement sélectifs, soit pour TPalpha, soit pour TPbeta. Par ailleurs, nous avons identifié in vivo des candidats pour le développement dagents thérapeutiques pour la prévention des thromboses et des autres pathologies provoquées par une activation plaquettaires excessive.

thromboxane

TP receptor antagonist/Antagoniste TP

GPCR/RCPG

Efeitos do exercício físico sobre a atividade de enzimas dos sistemas purinérgico e colinérgico em sangue de ratos hipertensos / Effects of physical training on purinergic and cholinergic system enzymes activities in blood of hipertensive rats

Cardoso, Andréia Machado

29 August 2014

Coordenação de Aperfeiçoamento de Pessoal de Nível Superior / Hypertension is a multifactor clinical condition, which is accompanied by a low-grade inflammation and alterations in platelet function. These modifications may be related to an imbalance in the regulation of adenine nucleotides (ATP, ADP and AMP), adenosine and acetylcholine (ACh) levels. This regulation is performed by purinergic [NTPDases, ecto-5 - nucleotidase and adenosine deaminase (ADA)] and cholinergic [Acetylcholinesterase (AChE) and Butyrylcholinesterase (BuChE)] system enzymes, present in blood, respectively. These enzymes can be modulated by regular practice of physical exercise, which has been recommended for the treatment of hypertension. Thus, the aim of this study was to investigate the effect of six swimming training weeks on blood pressure, on purinergic and cholinergic systems enzymes activities in blood as well as on platelet aggregation and classic inflammatory markers in rats with hypertension induced by methyl Nω-nitro-L-arginine ester hydrochloride (L-NAME) administration. In order to better understand chronic changes, we also evaluated the effect of a single acute bout of exercise on the activity of the enzymes already mentioned. The animals were divided into four groups (n = 10): control, exercise, LNAME and exercise L-NAME. After 60 days of treatment, animals were euthanized and platelets, lymphocytes, whole blood and serum were used for experimental determinations. The results showed that swimming training was able to reduce blood pressure in hypertensive rats, and to prevent the increase in NTPDase, ecto-5'-nucleotidase and ADA activities in lymphocytes and platelets. This probably contributed in preventing platelet aggregation. Chronically, swimming was also effective in preventing the increase in AChE (in lymphocytes and whole blood) and BuChE (in serum) activities. Regarding to the expression of NPTDase1, exercise per se triggered a reduction in the expression of this enzyme, but had no significant effects in hypertensive rats. The prevention of the increase in cholesterol, triglycerides, C-reactive protein levels and myeloperoxidase activity generated by swimming practice reinforces the fact that exercise reduced inflammation in hypertensive rats. In response to a single acute bout of exercise, was observed an increase in the activity of cholinergic system enzymes in whole blood, lymphocytes and serum, and purinergic system enzymes in platelets. However, there was a decrease in the activity of NTPDase and ADA in lymphocytes. It can be concluded that this study allowed us to unveil, in part, the mechanisms related to the protective processes arising from regular physical exercise on hypertension related to inflammation and platelet aggregation. The results also reinforce the importance of measuring the purinergic and cholinergic systems enzymes as parameters of inflammatory response. Also, it is concluded that regular physical exercise has antithrombotic and anti-inflammatory effects by modulating the activity purinergic and cholinergic systems enzymes in hypertension. It is suggested that these responses have been derived from the adaptations that occur in the body due to each acute stimulus that promotes enough impact to break homeostasis and promote beneficial adaptations. Thus, moderate aerobic exercise has a key role in acting as an adjuvant in the treatment of hypertension. / A hipertensão é uma condição clínica multifatorial que, na maioria dos casos, está acompanhada de um quadro inflamatório de baixo grau e alterações nas funções plaquetárias. Essas modificações podem estar relacionadas a um desequilíbrio na regulação dos níveis de nucleotídeos de adenina (ADP, ADP e AMP), da adenosina e da molécula acetilcolinesterase (ACh), que é realizada pelas enzimas do sistemas purinérgico [NTPDases, ecto-5 -nucleotidase e adenosina desaminase (ADA)] e colinérgico [Acetilcolinesterase (AChE) e Butirilcolinesterase (BuChE)] presentes no sangue, respectivamente. A atividade dessas enzimas pode ser modulada pela prática regular de exercícios físicos, a qual tem sido recomendada para o tratamento da hipertensão. Sendo assim, o objetivo deste estudo foi verificar o efeito de seis semanas de natação sobre a pressão arterial, a atividade de enzimas dos sistemas purinérgico e colinérgico em sangue, bem como sobre a agregação plaquetária e marcadores inflamatórios clássicos em ratos com hipertensão induzida através de administração de metila Nω-Nitro-L-arginina cloridrato de éster (L-NAME). Com o objetivo de melhor compreender as alterações crônicas, avaliouse, também, o efeito de uma única sessão aguda de exercício sobre a atividade das enzimas já mencionadas. Os animais foram divididos em quatro grupos (n = 10): Controle, Exercício, L-NAME e L-NAME Exercício. Após 60 dias de tratamento, os animais foram submetidos à eutanásia e as plaquetas, os linfócitos, o sangue total e o soro foram usados para as determinações experimentais. Os resultados obtidos mostraram que o treinamento com natação foi capaz de reduzir a pressão sanguínea em ratos hipertensos, além de prevenir o aumento da atividade das enzimas NTPDase, ecto-5 -nucleotidase e ADA em linfócitos e plaquetas, o que provavelmente contribuiu para prevenir a agregação plaquetária. Cronicamente, a natação também foi eficaz na prevenção do aumento da atividade das enzimas AChE em linfócitos e sangue total e BuChE em soro. Com relação à expressão da NPTDase1, o exercício per se gerou a redução da expressão desta enzima, mas não apresentou efeitos significativos nos ratos hipertensos. A prevenção do aumento dos níveis de colesterol, triglicerídeos, proteína C-reativa e mieloperoxidase gerada pela prática da natação reforça o fato de que o exercício reduziu a inflamação em ratos hipertensos. Como resposta a uma única sessão aguda de exercício, verificou-se o aumento da atividade das enzimas dos sistemas colinérgico em sangue total, linfócitos e soro e do sistema purinérgico em plaquetas. Entretanto, ocorreu a diminuição da atividade da NTPDase e da ADA em linfócitos. Pode-se concluir que este estudo permitiu desvendar em parte os mecanismos relacionados aos processos protetores advindos da prática regular de exercício físicos na hipertensão relativos aos processos inflamatórios e à agregação plaquetária. Os resultados ainda reforçam a importância da dosagem das enzimas dos sistemas purinérgico e colinérgico como parâmetros da resposta inflamatória. Conclui-se, também, que a prática regular de exercício físico possui efeitos antitrombóticos e antiinflamatórios através da modulação da atividade das enzimas dos sistemas purinérgico e colinérgico na hipertensão. Sugere-se que estas respostas tenham sido provenientes das adaptações ocorridas no organismo decorrentes de cada estímulo agudo, que gerou estímulos suficientes para quebrar a homeostase do organismo e promover adaptações benéficas. Desta forma, o exercício físico aeróbico moderado possui um papel fundamental na atuação como coadjuvante no tratamento da hipertensão.

Hipertensão

Ectonucleotidases

Colinesterases

Ratos

Sangue

L-NAME

Pressão arterial

Resposta inflamatória

Agregação plaquetária

Hypertension

Ectonucleotidases

Cholinesterases

Rats

Blood

L-NAME

Blood pressure

Inflammatory response

Platelet aggregation

CNPQ::CIENCIAS BIOLOGICAS::BIOQUIMICA

Cardiovascular protective effects of Lindera obtusiloba / Les effets de "Lindera obtusiloba" pour la protection cardiovasculaire

Lee, Jung-Ok

06 March 2013

La dysfonction endothéliale est un problème majeur au niveau mondial du fait de son implication dans de nombreuses pathologies. Ainsi, la dysfonction endothéliale est considérée comme un facteur pronostique défavorable dans les maladies cardiovasculaires. Les principaux mécanismes impliqués dans la dysfonction endothéliale sont la réduction de la formation et/ou de la biodisponibilité du monoxyde d’azote (NO), et la présence d’un stress oxydant. Le but de ce travail était d’évaluer des traitements phytothérapeutiques pouvant prévenir et/ou améliorer la dysfonction endothéliale. Le criblage de plus de trois cent plantes en fonction de leur capacité à induire une relaxation vasculaire et une inhibition de la NADPH oxydase (données confidentielles) a conduit à s’intéresser à Lindera obtusiloba. Ensuite, la capacité d’un extrait alcoolique de Lindera obtusiloba (LOE) à améliorer in vitro et in vivo la dysfonction endothéliale en activant la eNOS et en réduisant le stress oxydant a été testée. En conclusion, ces travaux indiquent que LOE possède des effets vasoprotecteurs in vitro et in vivo dans plusieurs modèles expérimentaux comme l’hypertension artérielle induite par l’angiotensine II, le diabète de type 2, l’athérosclérose et la thrombose pulmonaire. Ces effets bénéfiques impliquent, au moins en partie, la stimulation de la formation endothéliale du NO, la réduction du stress oxydant vasculaire via l’inhibition de la NADPH oxydase et l’inhibition de l’agrégation plaquettaire. Ainsi, LOE pourrait être un excellent candidat pour la prévention et/ou le traitement phytothérapeutique des maladies cardiovasculaires associées à une dysfonction endothéliale. / Endothelial dysfunction is a major worldwide topic because it is an important component and risk factor of a number of common human diseases. Therefore, endothelial dysfunction is considered a hallmark for vascular diseases, and has also been shown to be predictive of future adverse cardiovascular events. The main characteristic is a reduced NO production and bioavailability, and an increased vascular oxidative stress. The goal of the present research was to find a candidate for cardiovascular protective herbal medicine for the treatment of endothelial dysfunction. Through measurement of changes in isometric tension of porcine coronary artery rings, Lindera obtusiloba was selected amongst three hundred plants. Thereafter, the aim of our research was to determine whether an ethanolic extract of L. obtusiloba stems (LOE) improves endothelial dysfunction via activation of endothelial nitric oxide synthase and reduction of oxidative stress oxidase in vitro and in several animal models of cardiovascular diseases, and, if so, to elucidate the underlying mechanism. Altogether, the present findings indicate that LOE has vasoprotective effects both in vitro and in vivo including the Ang II-induced hypertention in rats, a type 2 diabetic mice model, and an atherosclerotic mice model, and a thromboembolism mice model, which involve its ability to stimulate the formation of NO, to reduce oxidative stress in the arterial wall, and to inhibit platelet aggregation. In conclusion, our studies reveal that LOE might be an interesting candidate as a cardiovascular protective herbal medicine in pathologies with endothelial dysfunction.

Maladies cardiovasculaires

Dysfonction endothéliale

Lindera obtusiloba

Hypertension

Diabètes

Athérosclérose

Thrombotiques

Agrégation plaquettaire

Endothelial dysfunction

Vascular diseases

Lindera obtusiloba

Hypertention

Type 2 diabetic mice model

Atherosclerotic mice model

Thromboembolism mice model

Platelet aggregation

615.7

Isolamento e caracterização funcional de uma fosfolipase A2 de Bothrops jararaca: avaliação do potencial antitumoral e inflamatório / Isolation and functional characterization of a phospholipase A2 from Bothrops jararaca snake venom: evaluation of its antitumor and inflammatory potential

Rafhaella Carolina Cedro Araújo

02 December 2014

As fosfolipases A2 (PLA2s) catalisam a hidrólise de ácidos graxos na posição sn-2 das membranas fosfolipídicas e liberam, como subprodutos, ácidos graxos livres. As PLA2s do grupo IIA são encontradas em peçonhas de serpentes da família Viperidae e desempenham diversas atividades apresentando potencial miotóxico, neurotóxico, hemolítico, edematogênico, citotóxico, hipotensivo, anticoagulante, inibição/ativação da agregação plaquetária, bactericida e pró-inflamatório. Esse trabalho teve como objetivo o isolamento e a caracterização funcional de uma PLA2 isolada da peçonha de Bothrops jararaca. Para a purificação dessa proteína, denominada BJ-PLA2-I, foram necessários três passos cromatográficos consecutivos: cromatografia de exclusão molecular em Sephacryl S-200, cromatografia de troca iônica em Source TM 15Q/50mL e cromatografia de troca iônica em MonoQ TM 5/50 GL. A BJ-PLA2-I apresentou elevado grau de pureza por SDS-PAGE e por cromatografia de fase reversa C18, em HPLC. Apresentou ainda, características ácidas, com pI em torno de 4,4 e teve a sua massa molecular determinada por dois métodos, obtendo-se valores bem próximos de 14,8 kDa (SDS-PAGE) e 14,2 kDa (MALDI-TOF). Esse fato é comum considerando que a espectrometria de massas é um método mais preciso e determina de maneira mais exata a massa molecular. O sequenciamento N-terminal da BJ-PLA2-I resultou em 60 resíduos de aminoácidos. O alinhamento múltiplo com outras fosfolipases A2 de serpentes do mesmo gênero mostrou similaridade entre elas, mostrando identidade de 100% com a BJ-PLA2, fosfolipase A2 Asp-49, também isolada da Bothrops jararaca. Esse dado levanta a hipótese de que a BJ-PLA2-I purificada neste trabalho e a BJ-PLA2 se tratam da mesma proteína, entretanto essa hipótese só poderá ser confirmada quando a sequência completa da BJ-PLA2-I for obtida. Outros dados encontrados neste trabalho reforçam essa hipótese, isso porque, avaliando a atividade fosfolipásica, o efeito sobre as plaquetas e o pI, tanto a BJ-PLA2-I quanto a BJ-PLA2 apresentaram características semelhantes. A BJ-PLA2-I, sendo uma Asp-49, mostrou alta atividade catalítica e efeito inibidor da agregação plaquetária induzida por ADP (20,5 ?g/mL inibiu 50 % da agregação plaquetária). Ela também foi capaz de induzir a migração leucocitária após a administração de diferentes concentrações (5, 10 e 20 ?g/mL) da BJ-PLA2-I. Esse dado também foi encontrado no ensaio em que a concentração de 10 ?g/mL foi fixada e variou-se o tempo de 2, 4 e 24 horas, observando-se principalmente a migração de neutrófilos. Além disso, verificou-se a liberação das citocinas IL-6 e IL-1?, de proteínas totais e de prostaglandina E2 na reação inflamatória induzida pela BJ-PLA2-I. No entanto, não foi observado a produção de TNF-?, IL-10 e leucotrieno B4. A BJ-PLA2-I caracterizou-se como uma PLA2 pró-inflamatória, produzindo inflamação local aguda. A BJ-PLA2-I foi avaliada quanto ao seu potencial antitumoral em três linhagens celulares distintas (PBMC, HL-60 e HepG2). Observou-se que a enzima em questão possui baixo potencial antitumoral para a linhagem HL-60, reduzindo o número de células tumorais em apenas cerca de 20% nas concentrações testadas. Verificou-se pequena alteração na viabilidade celular das células de PMBC, nas maiores concentrações testadas (160 e 80 ?g/mL) e, na linhagem HepG2 não foi encontrada nenhuma alteração. Concluindo, as informações adquiridas neste trabalho são de suma importância para a melhor compreensão dos mecanismos envolvidos nas atividades biológicas desempenhadas pelas PLA2s. Além disso, a BJ-PLA2-I pode servir como modelo molecular para a formulação de fármacos mais eficazes a serem utilizados no tratamento de várias doenças. / Phospholipases A2 (PLA2s) catalyze the hydrolysis of fatty acids in the sn-2 position of membrane phospholipids, releasing free fatty acids as by-products. PLA2s of group IIA are found in snake venoms of the Viperidae family and perform various activities, including myotoxic, neurotoxic, hemolytic, edematogenic, cytotoxic, hypotensive, anticoagulant, inhibition/activation of platelet aggregation, bactericidal and proinflammatory effects. This work aimed at the isolation and functional characterization of a PLA2 isolated from Bothrops jararaca venom. For the purification of this protein, called BJ-PLA2-I, three consecutive chromatographic steps were used (size exclusion chromatography on Sephacryl S-200, ion exchange chromatography on Source 15Q/50 mL, ion exchange chromatography on MonoQ 5/50 GL). Confirmation of the purity of BJ-PLA2-I was evaluated by SDS-PAGE and reverse phase HPLC using a C18 column. BJ-PLA2-I has acidic characteristics, with pI around 4.4, and its molecular mass was determined by two methods, obtaining values close to 14.8 kDa (SDS-PAGE) and 14.2 kDa (MALDI-TOF). The N-terminal sequencing of BJ-PLA2-I resulted in 60 amino acid residues. Multiple alignment with other phospholipases A2 of snakes of the same genus showed high similarity between them, showing 100% identity with BJ-PLA2, an Asp-49 phospholipase A2 previously isolated from Bothrops jararaca venom. This finding raises the possibility that the PLA2 purified in this work is the same protein previously described (BJ-PLA2), however, this assumption can only be confirmed when the complete sequence of BJ-PLA2-I is obtained. Other data obtained in this study support this hypothesis, considering that the phospholipase activity, the effect on platelets and pI of both BJ-PLA2-I and BJ-PLA2 showed to be similar. BJ-PLA2-I, being an Asp-49 PLA2, showed high catalytic activity and inhibitory effect on the platelet aggregation induced by ADP (20.5 ?g/mL inhibited 50% of the platelet aggregation). It was also able to induce leukocyte migration after the administration of different concentrations (5, 10 and 20 ?g/mL) of BJ-PLA2-I. This fact was also found when the concentration of 10 ?g/mL was fixed and response times were varied (2, 4 and 24 hours), observing especially neutrophil migration. Furthermore, there was a release of IL-6 and IL-1?, total proteins and prostaglandin E2 in the inflammatory reaction induced by BJ-PLA2-I, however, the production of TNF-?, IL-10 and leukotriene B4 was not observed. BJ-PLA2-I was characterized as a proinflammatory PLA2 producing acute local inflammation. BJ-PLA2-I was evaluated for its antitumor potential on three different cell lines (PBMC, HL-60 and HepG2). It was observed that this enzyme showed a low antitumor potential on HL-60 tumor cell line, reducing the number of tumor cells in only about 20% at the concentrations tested. There was little change in cell viability of PBMC cells in the higher concentrations tested (80 and 160 ?g/mL), but no change was found on HepG2 tumor cell line. In conclusion, the information obtained in this work are of utmost importance for better understanding the mechanisms involved in the biological activities induced by PLA2s. Furthermore, BJ-PLA2-I may serve as a molecular model for the formulation of more effective drugs to be used in the treatment of various diseases.

Agregação plaquetária

Antitumoral

Asp-49

BJ-PLA2-I

Bothrops jararaca

Fosfolipase A2 ácida

Inflamação

Isolamento

Acidic phospholipase A2

Antitumor

Asp-49

BJ-PLA2-I

Bothrops jararaca

Inflammation

Isolation

Platelet aggregation