Refine
Document Type
- Doctoral Thesis (3)
Has Fulltext
- yes (3)
Is part of the Bibliography
- no (3)
Institute
- Biochemie und Chemie (3) (remove)
Die 5-Lipoxygenase (5-LO) ist das Schlüsselenzym in der Biosynthese proinflammatorischer Leukotriene, die maßgeblich an der Entstehung allergischer und entzündlicher Erkrankungen wie Arthritis, Asthma und kardiovaskulären Erkrankungen beteiligt sind (23). Humane 5-LO besteht aus 673 Aminosäuren und besitzt ein Molekulargewicht von 77,8 kDa (25). Das Protein besteht aus einer größeren katalytischen Domäne, die ein zentrales Eisen(II)-Atom enthält, dass für die zweistufige LTA4-Bildung aus Arachidonsäure benötigt wird, und einer kleineren C2-ähnlichen Domäne, die Bereiche für die Membran- sowie Ca2+-Bindung enthält. Durch Stimulation von intakten Zellen kommt es zu einer Translokation der 5-LO an die Kernmembran. Die Wechselwirkung mit dem membranständigen FLAP fördert die 5-LO-Leukotrienbildung. Die vorliegende Arbeit beschäftigte sich mit niedermolekularen Modifikationen der 5-LO durch U-73122 und Glutathion sowie mit der Charakterisierung von 5-LO-Inhibitoren. U-73122 ist ein Inhibitor, der in vitro und in vivo mit einem IC50-Wert von 30 nM bzw. 2,4 µM die 5-LO-Aktivität hemmt (2). U-73122 verfügt über eine thiol-reaktive Maleinimid-Gruppe, wodurch die Substanz kovalent an einige 5-LO-Cysteine (Cys-99, -159 und weitere) binden kann. Entsprechende U-73122-5-LO-Peptide konnten nach Trypsin-Verdau der 5-LO mit MALDI-MS-Messungen nachgewiesen werden. Für diesen Zweck musste eine effiziente Aufreinigung für native 5-LO (Reinheit > 95%) entwickelt werden. Um die Veränderung der 5-LO-Aktivität nach U-73122-Zugabe zu untersuchen, wurden Cystein/Serin-5-LO-Mutanten hergestellt. Es konnte festgestellt werden, dass die Mutante C416S-5-LO nicht mehr effektiv durch U-73122 gehemmt werden konnte. Daher ist anzunehmen, dass U-73122 an Cystein-416 der 5-LO bindet und die 5-LO-Produktbildung hemmt. Auf der 5-LO-Oberfläche kann ein Bereich lokalisiert werden, der einen Zugang für das Substrat zum aktiven Zentrum der 5-LO bilden könnte (238,239). Dieser Bereich liegt in unmittelbarer Nähe zu Cystein-416. Daher besteht die Möglichkeit, dass U-73122, nachdem es an Cystein-416 gebunden hat, diesen Bereich hemmend beeinflussen kann. Es konnte nachgewiesen werden, dass Glutathion an mehrere Cysteine der 5-LO (Cystein-99, -264 und -449) kovalent binden kann. Um Veränderungen der 5-LO-Aktivität durch in vivo Glutathionylierungen zu zeigen, wurden HeLa-Zellen mit 5-LO, Cystein-/Serin-5-LO-Mutanten sowie FLAP transfiziert und mit Diamid inkubiert. Es konnte festgestellt werden, dass die native sowie FLAP-gesteigerte 5-LO-Produktbildung durch Diamid gehemmt wird. Dies konnte ebenfalls für die Mutante 3W-5-LO beobachtet werden. Zusätzlich wurden verschiedene Cystein-/Serin-5-LO-Punktmutanten sowie eine 4fach Mutante (C159S/C300S/C416S/C418S-5-LO = 2D-5-LO) untersucht. Das Verhalten dieser Mutanten konnte in drei Gruppen eingeteilt werden. Gruppe A (C159S-, C300S- und C418S-5-LO) wurde durch Diamid nicht beeinflusst. Gruppe B (C416S- und 2D-5-LO) zeigte eine sehr starke Stimulation der 5-LO±FLAP-Leukotrienbildung nach Zugabe von Diamid. Bei Gruppe C (C99S-, C264S- und C449S-5-LO) konnte eine FLAP-gesteigerte 5-HETE-Bildung beobachtet werden. Durch Diamid kommt es zu Glutathionylierungen von zellulären Proteinen, da reduziertes Glutathion (GSH) zu reaktiveren oxidierten Glutathion (GSSG) umgesetzt wird. An der 5-LO-Oberfläche können in Folge an verschiedenen Cysteinen Glutathione binden. Durch die Glutathion-Bindung wird eine stark polare Struktur auf der 5-LO-Oberfläche eingebracht. Dadurch kommt es zu einer verminderten Membranbindung und Produktbildung der nativen 5-LO. Die 5-LO-Oberfläche der 2D-5-LO-Mutante kann an verschiedenen Positionen keine Glutathione mehr binden, es kommt es zu einer stärkeren Wechselwirkung mit Membranbestandteilen und zu einer erhöhten 5-LO-Leukotrienbildung. Für Celecoxib konnte gezeigt werden, dass neben der COX2-Hemmung auch die 5-LO-Aktivität mit einem IC50-Wert von 3-10 µM gehemmt werden kann (268). Im Rahmen dieser Arbeit wurden HeLa-Zellen mit 5-LO±FLAP transfiziert, um den Einfluss von Celecoxib auf FLAP zu untersuchen. Celecoxib führt zu einer direkten Hemmung der 5-LO. ML3000 (Licofelon) wurde als dualer COX/5-LO-Inhibitor entwickelt und hemmt die 5-LO-Aktivität in intakten Zellen, aber nicht im Homogenat. Daher wurden Versuche mit 5-LO±FLAP-tranfizierten HeLa-Zellen durchgeführt, um den Einfluss von ML3000 auf die FLAP-gesteigerte 5-LO-Leukotrienbildung zu zeigen. Aus diesen und weiteren Ergebnissen unserer Arbeitsgruppe konnte gefolgert werden, dass ML3000 ein FLAP-Inhibitor ist (277). Garsubellin A ist strukturverwandt zu Hyperforin, einem dualen COX/5-LO-Inhibitor (204). Garsubellin A hemmt die 5-LO-Aktivität im Homogenat von PMNL und am gereinigten Enzym mit einer IC50 von 10-30 µM. Verbindungen, die den Bicyclo[3.3.1]nonan-Grundkörper des Garsubellin A und Hyperforin enthalten, wurden auf ihr inhibitorisches Potential getestet. Es konnte gezeigt werden, dass der Bicyclo[3.3.1]nonan-Grundkörper alleine nicht für eine 5-LO-Hemmung ausreicht, sondern eine freie Carbonsäure sowie eine bis zwei Prenylierungen vorliegen müssen, um eine 5-LO-Hemmung zu erzielen. Sind diese Voraussetzungen vorhanden, wird die 5-LO-Aktivität in intakten PMNL mit einer IC50 von 10 µM und an gereinigter 5-LO mit 0,3-1 µM gehemmt.
During the last years, chemopreventive activity of NSAIDs against a great variety of tumors was highly investigated. COX-2 seemingly plays a major part in tumorigensis and tumor development, underlined by several studies in animals and humans. At first, NSAIDs were thought to accomplish chemoprevention by inhibition of COX-2 as their so far known mode of action comprises unselective inhbition of COX-enzymes. However, further studies revealed COX-independent mechanisms. Sulindac is known as a well established drug used to treat inflammation and pain exerting the most prominent chemopreventive action, mainly in colorectal cancer or FAP and can be classified into the group of NSAIDs inhibting both COX-isoformes. As interference with the AA metabolism is evident, it was speculated whether Ssi has targets other than COX-enzymes providing evidence and explanation of its beneficial side effect profile and its ability to reduce tumor growth. 5-LO is another master enzyme in the AA cascade which produces inflammatory lipid mediators (LTs) upon stimulation in inflamed tissues. The present work should answer the question if Ssi targets the 5-LO pathway and should examine the molecular mechanisms behind Ssi-mediated 5-LO inhibiton. As COX-2 is upregulated during carcinogenesis and is inhibited by Ssi, further investigations should show regulatory effects of Ssi on 5-LO gene expression in MM6-cells and whether Sp1 as a common transcriptional factor is involved in such a regulation. As the use of NO-NSAIDs seem to be a promising strategy concerning their chemopreventive and gastroprotective effects compared to the parent NSAIDs, a possible interaction with the 5-LO pathway as a second, potent target should additionally be elucidated. In the first section it was demonstrated that the pharmacologically active metabolite of sulindac, Ssi, targets 5-LO. Ssi inhibited 5-LO in ionophore A23187- and LPS/fMLP-stimulated human PMNL (IC50 ≈ 8 -10 μM). Importantly, Ssi efficiently suppressed 5-LO in human whole blood at clinically relevant plasma levels (IC50 = 18.7 μM). Ssi was 5-LO-selective as no inhibition of related lipoxygenases (12-LO, 15-LO) was observed. The sulindac prodrug and the other metabolite, sulindac sulfone, failed to inhibit 5-LO. Mechanistic analysis demonstrated that Ssi directly suppresses 5-LO with an IC50 of 20 μM. Together, these findings may provide a novel molecular basis to explain the COX-independent pharmacological effects of sulindac under therapy. In the second part of the work dealing with the analysis of Ssi’s inhibitory mechanism on 5-LO it was presented that Ssi shows a lack of potency in cellular systems where membrane constituents are existent. The addition of microsomal fractions of PMNLto crude 5-LO enzyme were able to recover enzyme activity to ~ 100 %. Selectively 5-LO activity stimulating lipids like PC, participating in 5-LO membrane interactions within the regulatory C2-like domain of 5-LO, counteracted the Ssimediated inhibition on 5-LO-wt in a concentration-dependent manner. Lastly, a protein mutant lacking three trp resudies essential for linking the enzyme to nuclear membranes and deploying catalytic activity was not influenced by Ssi and shows enzyme activity in a cell-free assay. Ssi displays the first 5-LO inhibitor on the market interacting with the C2-like domain of the enzyme and therfore can stand for a novel lead structure of 5-LO inhibitors. An influence on 5-LO gene expression by Ssi could be detected in differentiated MM6-cells, described in the results chapter 3 (4.3). Ssi downregulated the 5-LO mRNA level after 72 hrs of incubation in differentiated MM6-cells to ~ 20 % of output control at concentrations of 10 μM. Concomitantly, mRNA levels of Sp1 were suppressed. Reporter gene studies revealed Sp1 most probably as a regulating agent involved in the Ssi-mediated 5-LO mRNA downregulation as co-transfection of increasing amounts of Sp1 could abrogate the effect. A ChIP assay could identify Sp1 as a critical transcriptional factor as Sp1 binding to the 5-LO promoter decreased in presence of Ssi. Lastly, three NO-NSADIs (NO-sulindac, NOnaproxen, NO-aspirin) were tested for the ability of 5-LO product inhibition. In intact PMNL, all compounds showed effective inhibition of 5-LO activity and NO-sulindac was most potent with an IC50 value of ~ 3 μM. NO-ASA inhibited 5-LO with IC50 values of ~ 30 μM and showed a non-competitive mode of action in cell-based assays. On human recombinant 5-LO all compounds again showed inhibitory potency whereas NO-sulindac again suppressed LT biosynthesis with an IC50 vaue comparable to intact cellular systems. Unfortunately, all inhibitors showed a loss of potency when tested for inhibition of 5-LO product synthesis in human whole blood as higher concentrations up to 100 μM were needed to reach at least 55 % enzyme inhibition. However, this strategy of 5-LO inhibition seems promising and needs further experimental approaches to gain more insight into the mechanism of 5-LO inhibition by NONSAIDs.
On the molecular basis of novel anti-inflammatory compounds and functional leukocyte responses
(2006)
Inflammation is a complex pathophysiological event that can be triggered by activation of a number of distinct activation pathways eventually leading to the release of pro-inflammatory molecules and enzymes. Among all cells involved in inflammatory processes, neutrophils, monocytes and platelets are of major relevance. Activation of leukocytes occurs via binding of agonists to distinct GPCRs leading to activation of G proteins and proximate signaling cascades. In short, GPCR activation by pro-inflammatory agonists such as fMLP, PAF or LTB4 leads to activation of G proteins that are associated with the receptor at the cytosolic side of the plasma membrane. G proteins consist of a Gα- and a Gβγ-subunit which are associated in the inactive state. In this state, G proteins bind GDP. Upon activation, GDP is replaced by GTP that results in the dissociation of the Gα- from the Gβγ-subunit. Both subunits are capable of activating distinct PLC-β isoenzymes that catalyze the turnover of PtdIns(4,5)P2 into the second messengers Ins(1,4,5)P3 and DAG. Every GPCR holds a distinct pattern of associated G proteins which preferentially activate distinct PLC-β isoenzymes. Ca2+ channels within the SR/ER-membrane function as specific receptors for Ins(1,4,5)P3. Ligation of Ins(1,4,5)P3 to this receptor causes a release of Ca2+ from intracellular stores into the cytosol that is subsequently followed by the influx of Ca2+ e through channels in the plasma membrane. Ca2+ represents an important signaling molecule, involved in the regulation of cellular processes and enzymes that mediate inflammatory events such as ROS formation and the release of degradative enzymes. 5-LO and COXs are involved in the biosynthesis of pro-inflammatory eicosanoids and catalyze the turnover of AA into LTs and PGs, respectively. Both enzymes play pivotal roles in the initiation and maintenance of allergic diseases and inflammatory processes. LTB4 is regarded as a potent chemotactic and chemokinetic substance, whereas the cysteinyl-LTs cause smooth muscle contraction and increased vascular permeability. Therefore, 5-LO inhibitors are assumed to possess therapeutic potential for the treatment of diseases related to inflammation. Besides the intervention with 5-LO activity, inhibition of COX-activity is an effective way to suppress inflammatory reactions. The two COX isoenzymes, namely COX-1 and COX-2 show different patterns in terms of tissue expression and sensitivity towards inhibitors. COX-1 is supposed to be constantly expressed whereas COX-2 expression is upregulated at sites of inflammation. The extract of H. perforatum is commonly used for the treatment of mild to moderate depressive disorders, accompanied by a moderate profile of side effects. The extract´s efficacy as an antidepressant can be traced back to the content of the phloroglucinol hyperforin which represents the most abundant lipophilic constituent. However, in folk medicine hypericum extracts are additionally used for the treatment of inflammatory disorders such as rheumatoid arthritis or inflammatory skin diseases. In fact, it was shown that hypericum extracts and hyperforin possess anti-inflammatory potential. Hyperforin was described as a dual inhibitor of 5-LO and COX-1. The phloroglucinols MC and S-MC from M. communis significantly differ from the molecular structure of hyperforin. Hyperforin represents a monomeric prenylated derivative whereas MS and S-MC are non-prenylated oligomeric compounds. To date, the anti-inflammatory potential of SM and S-MC has not been investigated in detail. So far, solely antioxidant activity was attributed to MC and S-MC that indeed might qualify them as anti-inflammatory drugs. The phloroglucinols MC, S-MC and hyperforin are potent inhibitors of ROS formation and HLE release. However, any inhibitory potential of these compounds was only observed when cells were activated by GPCR agonists such as fMLP or PAF. In contrast, when cells were stimulated under circumvention of G protein-associated signaling cascades, the abovementioned inhibitors were not effective at all. In leukocytes, [Ca2+]i plays a pivotal role in signal transduction and regulation of the indicated pro-inflammatory cellular functions. We were able to show that MC, S-MC and hyperforin inhibited GPCR-mediated Ca2+ mobilization with approximately the same potency as the above-mentioned leukocyte responses. However, all of the indicated phloroglucinols were ineffective when cells were stimulated with ionomycin. Since ionomycin as well as GPCR agonists exert their effects by mobilizing Ca2+ i, it seems conceivable that MC, S-MC and hyperforin somehow interfere with G protein-associated signaling pathways. In order to investigate PLC as a potential target of hyperforin, the effects of hyperforin were compared to those of the broad spectrum PLC inhibitor U-73122. We found that both inhibitors acted in a comparable manner in terms of agonist-induced Ca2+ mobilization and in regard of the manipulation of basal Ca2+ levels in unstimulated cells. In this respect, significant differences between hyperforin and U-73122 were obvious for inhibition of total PLC activity in vitro. Thus, U-73122 blocked PLC activity whereas hyperforin was ineffective in this respect. This might indicate that only certain PLC isoenzymes are affected by hyperforin. Alternatively, other components within G protein-associated signaling pathways such as G proteins itself or the Ins(1,4,5)P3 receptor must be taken into account as putative targets of hyperforin. We were able to introduce MC and S-MC as novel dual inhibitors of 5-LO and COX-1. Interestingly, such a pattern was also described for hyperforin. MC and S-MC turned out to be direct inhibitors of 5-LO, based on the fact that they inhibit 5-LO not only in intact cells but also as purified enzyme in vitro. For MC and S-MC, great discrepancies were observed between the IC50 values concerning 5-LO inhibition and the concentrations that exert the antioxidative effects. It seems probable that 5-LO inhibition is not related to reduction of the active site iron as a result of the antioxidant activity of MC and S-MC but rather to direct interference with the 5-LO enzyme. The capability of MC and S-MC to suppress COX-1 activity seems not to be a unique effect of these phloroglucinols because for COX-1, the IBPC, present in both MC and S-MC, turned out to be the most active compound. ....