Modulation of pharmacological, biochemical and enzymatic activities of basics sPLA2 from Bothrops jararacussu and Crotalus durissus ssp by semi purified extracts obtained from Tithonia diversifolia

Even after decades of the discovery of the anti-inflammatory inhibitors of phospholipase, there is a continuous search for new molecules which are able to provide this therapeutic effect without inducing side effects. The aim of this study was to obtain polar extract of the aerial parts of Tithonia diversifolia, enabling a quality standard for this extract from the identification of its main constituents and after this determination, to evaluate its effect on the activity of fractions A2 phospholipase basic secretory (sPLA2) obtained from Bothrops jararacussu (Bj) and Crotalus durissus ssp (Cd). The extracts were obtained by decoction and infusion and after the identification of the chromatography and LC / MS-MS. It was determined that the best yield of extract was obtained by decoction and its main constituents are cinnamic acid derivatives: caffeoyl - glycosidic, tagitinina C and quinic acid. Molecular imprint technique (MP) enabled separation of the constituents being a practical methodology. The polar extract showed anti-platelet activity at a concentration of 0.6 to 20 ?g/mL, opposite the stimulus induced by thrombin, which indicates that tea is not as inert and may promote complications in patients with coagulation disorders. Purification of Bj and Cd was performed by chromatographic techniques, with a yield of approximately 30% (p<0,05) of sPLA2. In vitro enzyme assay, which used synthetic chromogenic substrate of sPLA2 4-nitro-3-octanoyloxy benzoic acid (NOBA), it was identified that the polar extract was able to reduce by 60% (p<0,05) the enzymatic activity of sPLA2 Bj, regardless of the type of treatment applied, the reduction of the activity of sPLA2 Cd was reduced by 30% (p<0,05) when it was incubated for 30 min in presence of the extract. The modifications of the pathological effects caused by sPLA2s were evaluated by in vivo tests. The edematous action of sPLA2 Bj was reduced by 50% (p<0,05) when it was in presence of the extract, independent of incubation, since the same action for sPLA2 Cd was drastically reduced by the extract, however, after 60 min of administration of the agent inducer of inflammation, the myotoxic capacity with consequent release of creatine - kinase (CK) was modulated by the statement differently depending on the source of sPLA2, sPLA2 Bj to extract promoted a protective activity of CK release, because it reduced the release of enzyme, when applied intraperitoneally, 30 min before the offending agent, however, sPLA2 Cd showed reduced ability to release when CK was incubated with the extract for 30 min before application of the same muscle. Before the action of the extract on the sPLA2 induced inflammation was sought through the technique of polymerase chain reaction in real time (real time PCR), to determine the influence of the extract on the expression of genes involved in inflammation. We determined that Nf - Kb gene was the answer that although the presence of the extract is that the later is activated (or expressed), possibly because it was nuclear. Through these studies it was possible to determine the effect of these extracts on the acute inflammatory response induced by the action of sPLA2s from snake venoms (AU)