Jean Torreilles

Is malonaldehyde a valuable indicator of lipid peroxidation

Malonaldehyde (MDA), a decomposition product of lipid hydroperoxides which is used as an indicator of oxidative damage to cells and tissues, reacts, in vitro, with hydrogen peroxide to form undetermined degradation products. Since human polymorphonuclear leukocytes (PMNs) release reactive oxygen species including hydrogen peroxide when stimulated with phorbol myristate acetate (PMA), we incubated specific amounts of MDA with resting PMNs and PMA-stimulated PMNs. The amount of MDA recovered after 30 min incubation with stimulated cells, as determined by MDA-thiobarbituric acid assay, was 25% lower than that recovered with resting cells. In the presence of catalase 18% of MDA disappeared and in the presence of superoxide dismutase 15% disappeared. This indicates that measurements of MDA production in living systems, in the presence of reactive oxygen species, could be underestimated.

Nitration of tyrosyl-residues from extra- and intracellular proteins in human whole blood

We measured the amounts of tyrosine and 3-nitrotyrosine (NO2-tyrosine) in proteins of plasma and polymorphonuclear leukocytes (PMN) from human whole blood before and after activation with phorbol ester (PMA) or calcium ionophore (A 23187). In unstimulated blood, no significant nitration of tyrosine was detected into PMN proteins, but a NO2-tyrosine/tyrosine ratio of 0.7% was detected in plasma proteins. When blood was activated with PMA, the NO2-tyrosine/tyrosine ratio stayed at 0.7% in plasma proteins, but it increased to 1.4% in PMN proteins, indicating a peroxynitrite production within the cells. In blood activated with calcium ionophore, the NO2-tyrosine/tyrosine ratio was 1.2% in plasma proteins and 2.1% in PMN proteins. Incubation of blood with a NO-synthase inhibitor before stimulation inhibited such a protein tyrosine nitration. To ensure that NO2-tyrosine detected in intracellular proteins did not result from the enzymatic posttranslational tyrosylation of PMN proteins, the incorporation of 14C labeled tyrosine into PMN proteins after activation with PMA or A23187 was studied. The addition of a 10 fold excess of NO2-tyrosine did not modify the course of protein tyrosylation. Because tyrosine nitration is an irreversible reaction, NO2-tyrosine could be accumulated into proteins and could act as a cumulative index of peroxynitrite production.

Des structures simples aux potentialités pharmacologiques élevées: les β carbolines. Origines, synthèses, propriétés biologiques

We reviewed the origins, the synthetic pathways and the biological properties of beta-carbolines, the condensation products of tryptophan and indole alkylamines with aldehydes. They were found in many plants, some of which have been used as hallucinogens. They also occur as minor constituents in tobacco smoke. In mammalian body, beta-carboline derivatives occur normally in plasma, platelets and urine, moreover it seems that some are formed in human body after alcohol intake. Due to interesting biological effects described in recent years (inhibition of monoamine oxidase, binding to benzodiazepine receptors, comutagenic and carcinogenic properties, 5-hydroxy tryptamine uptake inhibition), many attempts were made to prepare beta-carbolines starting from various indole derivatives. We reviewed the published methods up to 1975 and summarized the main patents related with pharmacological properties of synthetic beta-carbolines.

L-ARGININE INFUSION AFTER ISCHAEMIA-REPERFUSION OF RAT KIDNEY ENHANCES LIPID PEROXIDATION

To assess the role of superoxide (O2-) and nitric oxide (NO) in ischaemic-reperfusion-induced acute renal failure, we investigated whether an activation of the L-arginine-NO pathway contributes to ischaemia-reperfusion-induced kidney membrane peroxidation by measurement of 4-hydroxynonenal (HNE) content in anaesthetized rats submitted to acute renal ischaemia. Following ischaemia-reperfusion injury, renal blood flow (RBF) was significantly reduced, while renal vascular resistance was significantly increased. Infusion of neither L-arginine nor D-arginine led to a recovery of RBF. L-Arginine, but not D-arginine, caused a significant increase in HNE accumulation in the ischaemic kidney. L-Arginine infusion enhanced the degree of lipid peroxidation afforded by ischaemia-reperfusion injury in the kidney suggesting that products of the endogenous L-arginine-NO pathway may react with O2- to initiate lipid peroxidation.

Nickel (II) Complexes of Histidyl-Peptides as Fenton-Reaction Catalysts

Addition of histidyl-peptides containing the glycyl-glycyl-L-histidyl sequence stimulated the catalysis of Ni(II) hydrogen peroxide reduction. Maximum bleaching of murexide or nitrosodimethylaniline was obtained with glycyl-glycyl-L-histidine. A decrease in the bleaching rates was observed upon addition of SOD or hydroxyl radical scavengers, showing that the hydrogen peroxide/Ni(II)/glycyl-glycyl-L-histidine system generated superoxide anions as well as hydroxyl radicals. In contrast, addition of glycyl-glycyl-L-histidine inhibited the Cu(II) hydrogen peroxide reduction. When peptides or proteins were exposed to oxygen radicals produced by Ni(II)/glycyl-glycyl-L-histidine catalysis of hydrogen peroxide reduction, the observed effects were similar to those produced by oxygen radicals generated by water radiolysis or by Fe(II) or Cu(II) mediated Fenton-reactions: hydroxylation of phenylalanine, interchange of disulfides, destruction of tryptophans and dityrosine formation.

Specific sulfonation of tyrosine, tryptophan and hydroxy-amino acids in peptides

1. ClSO3H in trifluoroacetic acid rapidly converts serine and threonine into O-sulfate ester derivatives while tyrosine and tryptophan are converted into arylsulfonic acids. 2. H2SO4 in trifluoroacetic acid reacts more slowly with serine, threonine and tyrosine while is not able to modify tryptophan. 3. All other amino acids are perfectly stable under the above reaction conditions. 4. Peptides containing susceptible amino acid residues are specifically converted into the corresponding sulfonated derivatives in high or quantitative yield.

Boomerangg effecgt between [Met]-enkephalin derivatives and human polymorphonuclear leukocytes

[Met]-enkephalin or its precursor, pre-[Met]-enkephalin, were exposed to activated oxygen species produced by human phorbol myristate acetate (PMA)-stimulated polymorphonuclear leukocytes (PMNs) and then analyzed by high-pressure liquid chromatography (HPLC). The chromatograms recorded at the tyrosine maximum wavelength (lambda em 300 nm and lambda ex 280 nm) showed the formation of new peptides by oxidation of methionyl residue in position 5 and ortho, meta, or para hydroxylation of phenylalanyl residue in position 4. The chromatograms recorded at the dityrosine maximum wavelength (lambda em 400 nm and lambda ex 325 nm) showed the formation of new dimeric peptides which contained two [Met]-enkephalin-derivatives linked by a dityrosyl group. These new peptides were tested for chemiluminescence response to PMA-stimulated PMNs. [Met]-enkephalin, pre-[Met]-enkephalin, and the methionyl-oxidized derivatives suppressed the PMA-induced respiratory burst of PMNs. Conversely, after hydroxylation by activated oxygen species released by stimulated PMNs, these peptides enhanced the PMA-induced respiratory burst of PMNs. In the same conditions, dimeric peptides had no effect.

Phosphorus-31 and proton fourier transform NMR. Metal ion-ribose interaction in the Cu2+-adenine nucleotide system

Abstract Using the 31 P and 1 H NMR techniques, the binding site of Cu 2+ to adenine nucleotide is clearly speci-field as a function of the pH values. When the pH is strongly basic, neither the N(7) of the base, nor the phosphate groups are still bound. The ribose moiety is then the coordination site of the metallic cation.

POTENTIAL ROLE OF THE PEROXIDASE-DEPENDENT METABOLISM OF SEROTONIN IN LOWERING THE POLYMORPHONUCLEAR LEUKOCYTE BACTERICIDAL FUNCTION

Serotonin (5-hydroxytryptamine, 5-HT) significantly and dose-dependently suppressed the luminol-enhanced chemiluminescence (CL) signal generated by polymorphonuclear leukocytes (PMN) activated with phorbol myristate acetate (PMA), but did not modify either lucigenin-enhanced CL or the reduction of superoxide dismutase-inhibitable cytochrome c. Moreover, stimulation of PMNs previously incubated with 5-HT resulted in a threefold increase in 5-HT equivalents bound to the proteins of PMN. The addition of catalase or sodium azide substantially reduced this binding. The present results suggest that 5-HT metabolism is mediated by H2O2 and myeloperoxidase (MPO) released by activated PMNs. Hence 5-HT could lower the bactericidal function of these cells by competition with hypochlorite formation from halides and MPO/H2O2.

Neutrophil-Catalysed Dimerisation of Tyrosyl Peptides

Evidence is given that tyrosyl-peptides are dimerised by polymorphonuclear leukocytes leading to a new family of compounds. The products formed are homo- and hetero-dimeric peptides with linkage between the tyrosyl residues. This corresponds to a dityrosine structure as determined by analytic and spectroscopic data.