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In Deutschland erhalten jährlich etwa 12.500 Patienten die Diagnose Leukämie. Unter ihnen befinden sich ca. 6 % Kinder, welche mit 33,8 % den größten Anteil der kindlichen Krebsneuerkrankungen repräsentieren. Die überwiegende Form im Kindesalter ist die akute lymphatische Leukämie (ALL), deren genetische Ursache meistens in einem hyperdiploiden Karyotyp oder einer chromosomalen Translokation zu finden ist. Bei 8 % der pädiatrischen ALLs ist ein Rearrangement des MLL-Gens involviert. Unter Beteiligung des häufigsten Translokationspartnergens (TPG) AF4 entsteht die t(4;11)(q21;q23)-Translokation mit den beiden Fusionsproteinen AF4•MLL sowie MLL•AF4. Die Therapie erfolgt in der Regel gemäß Hochrisikoprotokollen aufgrund der extrem schlechten Prognose und der mit hoher Therapieresistenz assoziierten Rezidivrate. Eine Studie zur Korrelation zwischen klinischen Merkmalen und molekularen Charakteristika belegte die Abhängigkeit des Outcomes von der Verteilung des Bruchpunkts im MLL-Gen. Bei älteren Patienten treten die Bruchpunkte überwiegend in MLL Intron 9 oder 10 auf und bedeuten eine signifikant bessere Prognose im Vergleich zu den besonders bei Säuglingen präsenten Bruchpunkten im MLL Intron 11. Die damit verbundene Verkürzung der Plant Homeodomain (PHD) 1 kann neben einer modifizierten Funktion des PHD1 auch in einer veränderten Konformation der gesamten PHD-Domäne resultieren. Besondere Bedeutung hat die PHD1-3-Domäne wegen der Fähigkeit des PHD3 einerseits H3K4me-Signaturen zu erkennen und auf der anderen Seite mit CYP33 zu interagieren. Die mit transkriptionell aktivem Chromatin assoziierten H3K4me-Signaturen sowie die CYP33-vermittelte repressive Aktivität bedingen einen ambivalenten Charakter des MLL-Proteins. Daneben ist der PHD3 allein interessant wegen des Vorkommens von 4 differenten Varianten mit keinen, 3, 11 oder 14 fehlenden Aminosäuren, welche durch alternatives Spleißen an der MLL Exon 15/16-Verknüpfung entstehen (PHD3-0, PHD3-3, PHD3 11 und PHD3-14). Semiquantitative Bestimmungen in verschiedenen Zelllinien verdeutlichen die nahezu ähnliche Transkription aller 4 Varianten. Weiterführende Untersuchungen mit dem Yeast Two-Hybrid (Y2H)-System sowie folgende Koimmunpräzipitations (CoIP)-Experimente zeigten, dass der PHD3-0 die beste Dimerisierungsfähigkeit aufweist. Dagegen ist der am schlechtesten dimerisierende PHD3-3 allein in der Lage, CYP33 bzw. dessen RRM-Domäne zu binden. Die Interaktion mit inhibitorischen Proteinen und die folgende Funktion als transkriptioneller Repressor sind allein mit der PHD3-3-Variante möglich. Bei Betrachtung der gesamten PHD1-3-Domäne sowie deren verkürzter Variante (ΔPHD1-3) fällt die reduzierte Bindungsfähigkeit der ΔPHD1-3-Domäne an die CYP33 RRM-Domäne sowie deren fehlende Dimerisierung auf. Über die resultierende geringere Bindung an inhibitorische Proteine kann die transkriptionell repressive Aktivität reduziert werden, während die transkriptionell aktive Funktion an Bedeutung gewinnt. Neben der Untersuchung der PHD-Domänen des MLL-Proteins wurde das Y2H-System zur weiteren Aufklärung der AF4- und AF4•MLL-Multiproteinkomplexe (MPC) verwendet. Ähnlich den Wildtypproteinen MLL und AF4 sind auch die beiden aus der t(4;11)(q21;q23)-Translokation resultierenden Fusionsproteine an der Assemblierung von MPCs beteiligt. Besonders das reziproke AF4•MLL scheint bezüglich des Therapieerfolgs für die Leukämogenese entscheidend zu sein. Die Identifizierung und Verifizierung sowohl bekannter als auch neuer Komponenten der AF4- und AF4•MLL-MPCs gelang in verschiedenen Experimenten. Allerdings wurde meist nur die Präsenz der Proteine im MPC nachgewiesen. Die Y2H-Untersuchungen konnten Interaktionen zwischen den verschiedenen Proteinen der Komplex identifizieren und damit die Kenntnis über die Zusammensetzung der MPCs wesentlich erweitern und vertiefen. Aufgrund der Beteiligung viraler Proteine an der Krebsentstehung sowie der Rekrutierung von Transkriptionsfaktoren der Wirtszelle für die virale Replikation erscheint auch die Nutzung der Superelongationskomplexe (SEC) durch virale Proteine plausibel. Die Funktion des AF4-Proteins als Kofaktor von viralen Proteinen, besonders der HCMV und EBV immediate early (IE)-Proteine, wurde bereits gezeigt. Außerdem konnte der Einfluss des HCMV IE1 auf AF4-abhängige Effekte sowie dessen Beteiligung am AF4-MPC nachgewiesen werden. Mithilfe der Y2H-Experimente konnten nicht nur Interaktionen des HCMV IE1 sondern auch Wechselwirkungen der Onkoproteine E6/E7 des HPV mit den Proteinen der AF4- und AF4•MLL-MPCs identifiziert werden.
Changes in vitamin D serum levels have been associated with inflammatory diseases, such as inflammatory bowel disease (IBD), rheumatoid arthritis, systemic lupus erythematosus, multiple sclerosis (MS), atherosclerosis, or asthma. Genome- and transcriptome-wide studies indicate that vitamin D signaling modulates many inflammatory responses on several levels. This includes (i) the regulation of the expression of genes which generate pro-inflammatory mediators, such as cyclooxygenases or 5-lipoxygenase, (ii) the interference with transcription factors, such as NF-κB, which regulate the expression of inflammatory genes and (iii) the activation of signaling cascades, such as MAP kinases which mediate inflammatory responses. Vitamin D targets various tissues and cell types, a number of which belong to the immune system, such as monocytes/macrophages, dendritic cells (DCs) as well as B- and T cells, leading to individual responses of each cell type. One hallmark of these specific vitamin D effects is the cell-type specific regulation of genes involved in the regulation of inflammatory processes and the interplay between vitamin D signaling and other signaling cascades involved in inflammation. An important task in the near future will be the elucidation of the regulatory mechanisms that are involved in the regulation of inflammatory responses by vitamin D on the molecular level by the use of techniques such as chromatin immunoprecipitation (ChIP), ChIP-seq, and FAIRE-seq.
Our focus is the identification, characterisation and functional analysis of different MLL fusions. In general, MLL fusion proteins are encoded by large cDNA cassettes that are difficult to transduce into haematopoietic stem cells. This is due to the size limitations of the packaging process of those vector-encoded RNAs into retro- or lentiviral particles. Here, we present our efforts in establishing a universal vector system to analyse different MLL fusions. The universal cloning system was embedded into the backbone of the Sleeping Beauty transposable element. This transposon has no size limitation and displays no integration preference, thereby avoiding the integration into active genes or their promoter regions. We utilised this novel system to test different MLL fusion alleles (MLL-NEBL, NEBL-MLL, MLL-LASP1, LASP1-MLL, MLL-MAML2, MAML2-MLL, MLL-SMAP1 and SMAP1-MLL) in appropriate cell lines. Stable cell lines were analysed for their growth behaviour, focus formation and colony formation capacity and ectopic Hoxa gene transcription. Our results show that only 1/4 tested direct MLL fusions, but 3/4 tested reciprocal MLL fusions exhibit oncogenic functions. From these pilot experiments, we conclude that a systematic analysis of more MLL fusions will result in a more differentiated picture about the oncogenic capacity of distinct MLL fusions.
Caspase-2 represents the most conserved member of the caspase family, which exhibits features of both initiator and effector caspases. Using ribonucleoprotein (RNP)-immunoprecipitation assay, we identified the proapoptotic caspase-2L encoding mRNA as a novel target of the ubiquitous RNA-binding protein HuR in DLD-1 colon carcinoma cells. Unexpectedly, crosslinking-RNP and RNA probe pull-down experiments revealed that HuR binds exclusively to the caspase-2-5' untranslated region (UTR) despite that the 3' UTR of the mRNA bears several adenylate- and uridylate-rich elements representing the prototypical HuR binding sites. By using RNAi-mediated loss-of-function approach, we observed that HuR regulates the mRNA and in turn the protein levels of caspase-2 in a negative manner. Silencing of HuR did not affect the stability of caspase-2 mRNA but resulted in an increased redistribution of caspase-2 transcripts from RNP particles to translational active polysomes implicating that HuR exerts a direct repressive effect on caspase-2 translation. Consistently, in vitro translation of a luciferase reporter gene under the control of an upstream caspase-2-5'UTR was strongly impaired after the addition of recombinant HuR, whereas translation of caspase-2 coding region without the 5'UTR is not affected by HuR confirming the functional role of the caspase-2-5'UTR. Functionally, an elevation in caspase-2 level by HuR knockdown correlated with an increased sensitivity of cells to apoptosis induced by staurosporine- and pore-forming toxins as implicated by their significant accumulation in the sub G1 phase and an increase in caspase-2, -3 and poly ADP-ribose polymerase cleavage, respectively. Importantly, HuR knockdown cells remained insensitive toward STS-induced apoptosis if cells were additionally transfected with caspase-2-specific siRNAs. Collectively, our findings support the hypothesis that HuR by acting as an endogenous inhibitor of caspase-2-driven apoptosis may essentially contribute to the antiapoptotic program of adenocarcinoma cells by HuR.
Die akute myeloische Leukämie (AML) ist eine klonale Erkrankung einer myeloischen Vorläuferzelle, welche nicht zur geregelten Selbsterneuerung und terminalen Differenzierung in der Lage ist. Es kommt zur Anhäufung von unreifen Zellen im Knochenmark und peripheren Blut. Häufig werden in AML-Patienten reziproke Chromosomentranslokationen wie t(6;9), t(8;21) und t(15;17) detektiert. Diese Translokationen führen zu Genfusionen und bilden die Fusionsproteine DEK/CAN, AML1/ETO und PML/RARα. In dieser Arbeit wurde DEK/CAN untersucht, das Fusionsprodukt der Translokation t(6;9).
Die t(6;9)-positive Leukämie zeichnet sich durch eine äußerst schlechte Prognose aus sowie einem Eintritt der Krankheit bereits im jungen Erwachsenenalter. Aus diesen Gründen wird die t(6;9)-positive Leukämie nach der neuen WHO-Klassifikation als eigene Entität geführt. Das leukämogene Potential des Fusionsproteins DEK/CAN wurde bereits nachgewiesen, der Mechanismus der Leukämieinduktion ist jedoch völlig ungeklärt.
Von den Leukämie-assoziierten Fusionsproteinen AML1/ETO und PML/RARα ist bekannt, dass sie mutierte Transkriptionsfaktoren sind und die lokale Zusammen-setzung chromatin-assoziierter Proteine beeinflussen. Durch die aberrante Rekrutierung von chromatin-modifizierenden Faktoren kommt es zur Deregulierung von differenzierungsrelevanten Genen. Ziel dieser Arbeit war es daher zu ermitteln, ob es sich bei DEK/CAN ebenso um einen aberranten Transkriptionsfaktor mit Einfluss auf das Chromatin handelt.
Dazu wurden zunächst folgende Grundeigenschaften eines Transkriptionsfaktors untersucht: nukleäre Lokalisation und Chromatinassoziation. Immunfluoreszenz-untersuchungen bestätigten eine nukleäre Lokalisation von DEK/CAN. Es zeigte sich dabei, dass die Fusion mit CAN eine Umverteilung von DEK zur Folge hat. Während DEK diffus im Zellkern verteilt ist, zeigt das Fusionsprotein ein punktiertes Muster. Anschließend wurde die Assoziation von DEK/CAN zum Chromatin mit Hilfe von Zellfraktionierungsexperimenten nachgewiesen. Dabei konnte DEK/CAN aus der gleichen nukleären Fraktion eluiert werden wie andere chromatin-assoziierte Proteine.
Es stellte sich daraufhin die Frage, ob DEK/CAN die epigenetische Maschinerie beeinflussen und möglicherweise Veränderungen von Chromatinmodifikationen verursachen kann. Hierfür wurde die globale Verteilung der Histonmethylierungen H3K9me3, H3K27me3, H3K4me2 und H4R3me2 in An- und Abwesenheit von DEK/CAN untersucht. Es stellte sich heraus, dass DEK/CAN die Verbreitung von H4R3me2 maßgeblich beeinflusst. Histonmethylierungen regulieren das Expressionsniveau der gebundenen DNA, weshalb DEK/CAN durch seine Wirkung auf H4R3me2 die Deregulierung tumorrelevanter Gene verursachen könnte.
AML-assoziierte Fusionsproteine verändern die lokale Zusammensetzung von chromatin-modifizierenden Faktoren, indem sie oligomerisieren und so mehr Inter-aktionsmöglichkeiten für chromatin-modifizierende Proteine schaffen. Eine Gemein-samkeit aller AML-assoziierten Fusionsproteine ist der Besitz einer Oligomeri-sierungsoberfläche. Die putative Coiled coil (CC)-Domäne von CAN wurde hinsichtlich ihres Einflusses auf das leukämogene Potential und der Fähigkeit zur Bildung von Oligomeren untersucht, denn auch beim APL-spezifischen Fusionsprotein PML/RARα ist eine CC-Domäne für die Akkumulation verantwortlich. Die Deletion einzelner Helices aus der putativen CC-Domäne von DEK/CAN führte im CFU-S12 Assay zur Reduktion der Kolonienbildung. Damit konnte gezeigt werden, dass die Integrität der putativen CC-Domäne für den proliferationsstimulierenden Effekt von DEK/CAN auf das Kompartiment der Stammzellen notwendig ist. Eine Funktion als Oligomerisierungsoberfläche wurde für die CC-Domäne jedoch ausgeschlossen.
DEK ist ein nukleäres Phosphoprotein mit vielfältigen Funktionen, die unter anderem durch seinen Phosphorylierungsstatus gesteuert werden. Um die Relevanz der Phosphorylierungsstellen für das leukämogene Potential von DEK/CAN zu ermitteln, wurden DEK- und DEK/CAN-Mutanten erstellt, die nur partiell phosphorylierbar sind. Tatsächlich zeigte ein CFU-S12 Assay, dass die Mutation dieser Phosphorylierungsstellen zur Reduktion der Milzkolonienzahl und damit zur Aufhebung des leukämogenen Potentials führt. Außerdem hebt die Mutation der Phosphorylierungsstellen den DEK-vermittelten Effekt der Apoptoseresistenz auf.
Mit dieser Arbeit wurde durch Chromatinuntersuchungen und Struktur-Funktions-analysen ein Beitrag zur Entschlüsselung des leukämogenen Mechanismus von DEK/CAN geleistet.
Immune cells are key players in several physiological and pathophysiological events such as acute and chronic inflammation, atherosclerosis and cancer. Especially in acute inflammation, macrophages are indispensable for the switch from the acute inflammatory phase to the resolution phase. Not only the phagocytosis of apoptotic cells, but especially the surrounding cytokines and mediators are able to switch macrophage polarization from inflammatory- to anti-inflammatory phenotypes. Within this cytokine environment, sphingosine-1-phosphate (S1P) plays an important role for immune cell activation, polarization and migration.
BACKGROUND: Micro-RNAs (miRNA) are attributed to the systems biological role of a regulatory mechanism of the expression of protein coding genes. Research has identified miRNAs dysregulations in several but distinct pathophysiological processes, which hints at distinct systems-biology functions of miRNAs. The present analysis approached the role of miRNAs from a genomics perspective and assessed the biological roles of 2954 genes and 788 human miRNAs, which can be considered to interact, based on empirical evidence and computational predictions of miRNA versus gene interactions.
RESULTS: From a genomics perspective, the biological processes in which the genes that are influenced by miRNAs are involved comprise of six major topics comprising biological regulation, cellular metabolism, information processing, development, gene expression and tissue homeostasis. The usage of this knowledge as a guidance for further research is sketched for two genetically defined functional areas: cell death and gene expression. Results suggest that the latter points to a fundamental role of miRNAs consisting of hyper-regulation of gene expression, i.e., the control of the expression of such genes which control specifically the expression of genes.
CONCLUSIONS: Laboratory research identified contributions of miRNA regulation to several distinct biological processes. The present analysis transferred this knowledge to a systems-biology level. A comprehensible and precise description of the biological processes in which the genes that are influenced by miRNAs are notably involved could be made. This knowledge can be employed to guide future research concerning the biological role of miRNA (dys-) regulations. The analysis also suggests that miRNAs especially control the expression of genes that control the expression of genes.
Epicutanoeus immunotherapy as a novel prophylactic and therapeutic strategy for birch pollen allergy
(2014)
The development of a convenient, effective and safe allergen-specific immunotherapy (SIT) for birch pollen allergy, one of the most prevalent allergic diseases in Northern Europe, North America and Northern Japan, is of crucial importance. Epicutaneous immunotherapy (EPIT) has gained attention as a safe and non-invasive alternative for subcutaneous immunotherapy, a conventional SIT. However, clinical studies showed a limited effcacy of EPIT, indicating the necessity of improvement of the treatment regime. In this study, we hypothesized that a combination of a hypoallergen with an appropriate adjuvant could be a strategy to improve EPIT. To verify this hypothesis, we aimed at investigating the efficacy of epicutaneous treatment with rBet v 1, the major birch pollen allergen, plus Toll-like receptor (TLR) agonists for prophylaxis and therapy of birch pollen allergy using a murine model of birch pollen-induced allergic asthma. Furthermore, the efficacy of rBet v 1B2, a hypoallergenic variant of Bet v 1, as a therapeutic allergen in EPI was pre-clinically investigated. TLRs recognize conserved microbial molecules (like PAMPs), and are known to promote the counter-regulation of TH2 responses by the induction of TH1-type and/or regulatory cytokines by immune cells. The hypoallergen Bet v 1B2 is a folding-variant of the wild-type allergen rBet v 1 with reduced allergenicity, but retained T-cell immunogenicity. The low allergenicity, could allow the application of hypoallergens in higher doses, and therefore provide a safer and more effective treatment to regulate T-cell immune responses. First, the expression and purification of recombinant Bet v 1 and Bet v 1B2 was optimized. Compared to natural proteins, recombinant proteins offer the possibility to use well-defined molecules with a consistent pharmaceutical quality. Using optimal Escherichia coli expression strains in combination with immobilized metal chelate affinity chromatography (IMAC) and size exclusion chromatography (SEC), we successfully prepared a large amount of rBet v 1 and rBet v 1B2 with a high purity. The allergenic potency of rBet v 1 and the hypoallergenic characteristics of rBet v 1B2 were confirmed by measurement of IgE reactivity and mediator release capacity using ELISA and basophil activation tests, respectively. In a second part, a murine model of birch pollen-induced allergic asthma was established. It was shown that intraperetoneal sensitization with an optimal dose of rBet v 1 and intranasal challenge with birch pollen extract induced elevated IgE levels, airway eosinophilia and pulmonary inflammation in BALB/c mice. The clinical features are comparable to those in patients with allergic asthma, indicating that sensitized and challenged mice could be used for a pre-clinical study to assess the efficacy of the treatment for birch pollen allergy. Next, we investigated the adjuvant effects of Polyadenylic:polyuridylic acid (Poly(A:U)), a TLR3 agonist, and R848 (resiquimod), a TLR7 agonist, in prophylactic EPI with rBet v 1 to intervene with birch pollen allergy. Here, we hypothesized that TLR3 and TLR7 could be possible target receptors to induce adjuvant effects in EPI, since these receptors are expressed in Langerhans cells and dermal dendritic cells, persistent antigen presenting cells in the cutaneous tissues. BALB/c mice received EPI with rBet v 1 alone, or plus Poly(A:U), or R848 on their depilated back using patches. Mice treated epicutaneously were then sensitized with rBet v 1 plus ALUM and intranasally challenged with birch pollen extract. We found that prophylactic EPI with rBet v 1 plus R848 inhibited the production of Bet v 1-specific IgE antibodies in sensitization, suppressed pulmonary inflammation and airway hyperreactivity upon challenge. In contrast to R848, no adjuvant effect of Poly(A:U) on suppression of asthmatic features was observed. Our results indicated that R848, but not Poly(A:U), could be a potential adjuvant for prophylactic EPI of birch pollen induced allergic asthma. Finally, the therapeutic potency of EPI with rBet v 1, or rBet v 1B2 alone, or plus R848 was assessed. After sensitization and challenge, mice received therapeutic EPI with rBet v 1 alone, or plus R848, and re-challenge with birch pollen extract. We found that therapeutic treatment with Bet v 1B2 reduced established Bet v 1-specific IgE antibodies, pulmonary inflammation and airway hyperreactivity upon re-challenge. Therapeutic treatment with the recombinant wild-type allergen does not influence these key characteristics of allergic asthma. In contrast to the findings in the prophylactic treatment with rBet v 1 plus R848,no therapeutic benefit was found upon combination with R848. This could be due to the high number of treatment days. Reduction of this number may lead to a beneficial effect. However, these findings indicate that Bet v 1B2 could be a potential therapeutic agent for the treatment of established birch pollen induced allergic asthma. In conclusion, this study demonstrates for the first time that prophylactic EPI with the recombinant form of Bet v 1 in combination with R848 could prevent and suppress asthmatic features in an established birch pollen allergy. Not only therapeutic, but also prophylactic applications of EPI could be of importance to prevent allergic sensitization, considering the high prevalence of allergic diseases. R848 could be a potential adjuvant for enhancing the prophylactic potential of EPI for the treatment of birch pollen allergy. Furthermore, the beneficial use of the hypoallergen Bet v 1B2 in therapeutic EPI was demonstrated by intervention of established asthmatic features. In the future, a combination of hypoallergens alone or together with adjuvants in EPIT could lead to a more convenient and effective therapeutic treatment of established birch pollen induced allergic asthma.
Conjugated vaccines consisting of flagellin and antigen activate TLR5 and induce strong innate and adaptive immune responses. Objective of the present study was to gain further insight into the mechanisms by which flagellin fusion proteins mediate their immune modulating effects. In a mouse model of Ova-induced intestinal allergy a fusion protein of flagellin and Ova (rflaA:Ova) was used for intranasal and intraperitoneal vaccination. Aggregation status of flaA, Ova and flaA:Ova were compared by light scattering, uptake of fluorescence labeled proteins into mDC was analyzed, processing was investigated by microsomal digestion experiments. Mechanism of DC-activation was investigated using proteasome and inflammasome inhibitors. Immune responses of wildtype, IL-10−/−, TLR5−/− mDCs and Ova-transgenic T cells were investigated. Mucosal and i.p.-application of rflaA:Ova were able to prevent allergic sensitization, suppress disease-related symptoms, prevent body weight loss and reduction in food uptake. Intranasal vaccination resulted in strongest suppression of Ova-specific IgE production. These protective effects were associated with increased aggregation of rflaA:Ova and accompanied by tenfold higher uptake rates into mDC compared to the mixture of both proteins. Microsomal digestion showed that stimulation with rflaA:Ova resulted in faster degradation and the generation of different peptides compared to rOva. rflaA:Ova-mediated activation of mDC could be suppressed in a dose-dependent manner by the application of both inflammasome and proteasome inhibitors. Using TLR5−/− mDC the rflaA:Ova induced IL-10 secretion was shown to be TLR5 dependent. In co-cultures of IL-10−/− mDC with DO11.10 T cells the lack of rflaA:Ova-mediated IL-10 secretion resulted in enhanced levels of both TH2 (IL-4, IL-5) and TH1 (IL-2 and IFN-y) cytokines. In summary, mucosal vaccination with flaA:Ova showed strongest preventive effect. Stimulation with rflaA:Ova results in strong immune modulation mediated by enhanced uptake of the aggregated fusion protein, likely resulting in a different processing by DC as well as stronger TLR5 mediated cell activation.
To overcome poor treatment response of pediatric high-risk acute lymphoblastic leukemia (ALL), novel treatment strategies are required to reactivate programmed cell death in this malignancy. Therefore, we take advantage of using small-molecule antagonists of Inhibitor of apoptosis (IAP) proteins, so called Smac mimetics such as BV6, which are described to overcome apoptosis resistance and thereby sensitize tumor cells for several apoptotic stimuli. To address the question whether redox alterations can sensitize leukemic cells for Smac mimetic-mediated cell death, we interfered with the cellular redox status in different ALL cell lines. Here, we show for the first time that redox alterations, mediated by the glutathione depleting agent Buthioninesulfoximine (BSO), prime ALL cells for BV6-induced apoptosis. Besides ALL cell lines, BV6/BSO cotreatment similarly synergizes in cell death induction in patient-derived primary leukemic samples. In contrast, the combination treatment does not exert any cytotoxicity against peripheral blood lymphocytes (PBLs) or mesenchymal stroma cells (MSCs) from healthy donors, suggesting some tumor selectivity of this treatment. We also identify the underlying molecular mechanism of the novel synergistic drug interaction of BSO and BV6. We demonstrate that both agents act in concert to increase reactive oxygen species (ROS) production, lipid peroxidation and finally apoptotic cell death. Enhanced ROS levels in the combination treatment account for cell death induction, since several ROS scavengers, like NAC, MnTBAP and Trolox attenuate BSO/BV6-induced apoptosis. BSO/BV6-induced ROS can be mainly classified as lipid peroxides, since the vitamin E derivate α-Tocopherol as well as Glutathione peroxidase 4 (GPX4), which both specifically reduce lipid-membrane peroxides, prevent lipid peroxidation, caspase activation and cell death induction. Vice versa, GPX4 knockdown and pharmacological inhibition of GPX4 by RSL3 or Erastin enhance BV6-induced cell death. Importantly, cell death induction critically depends on the formation of a complex consisting of RIP1/FADD/Caspase-8, since all complex components are required for ROS production, lipid peroxidation and cell death induction. Taken together, we demonstrate that BSO and BV6 cooperate to induce ROS production and lipid peroxidation which are eventually required for caspase activation and cell death execution. Collectively, findings of this study indicate that BV6-induced apoptosis is mediated via redox alterations offering promising new treatment strategy to overcome apoptosis resistance in ALL.