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Transkription und DNA-Reparatur in den Bruchpunktsregionen des MLL-Gens und seiner fünf häufigsten Translokationspartnergene AF4, AF9, AF10, ELL und ENL
(2008)
- In der Vergangenheit wurden verschiedene Fusionstranskripte, welche normalerweise bei Leukämie-assoziierten chromosomalen Translokationen auftreten, in hämatopoetischen Zellen gesunder Personen gefunden. Da diese Personen keine entsprechenden chromosomalen Abberationen aufwiesen, ist es sehr wahrscheinlich, dass diese Fusionstranskripte durch trans-Spleißen entstehen. Während dieser Arbeit konnten durch inverse PCR, welche an unbehandelter cDNA gesunder Probanden durchgeführt wurde, intragenische trans-Spleiß-Produkte nachgewiesen werden. Interessanterweise weisen das MLL-Gen und seine fünf häufigsten Translokationspartner AF4, AF9, AF10, ELL und ENL ein großes Spektrum an trans-gespleißten RNAs auf. Nur in einem weiteren Mitglied der MLL-Familie (MLL3) konnte intragenisches trans-Spleißen nachgewiesen werden. Für verschiedene als Kontrolle verwendete Haushaltsgene konnte kein intragenisches trans-Spleißen nachgewiesen werden. Intergenische trans-Spleiß-Ereignisse konnten durch direkte PCR und RACEExperimente für die Gene MLL, ELL und ENL nachgewiesen werden. Bemerkenswerterweise entsprechen ein intragenisches trans-Spleiß-Produkt des MLL-Gens dem Transkript der chromosomalen Abberationen MLL-PTD und ein intergenisches trans-Spleiß-Produkt des MLL-Gens dem Transkript der chromosomalen Abberationen MLL•AF4. In Hefe konnte gezeigt werden, dass RNA als Vorlage für DNA-Reparaturen dienen kann. Somit lag der Schluß nahe, dass die oben genannten trans-gespleißten RNAs möglicherweise einen Einfluss auf die DNA-Reparatur haben. Dass RNA nicht nur in Hefen sondern auch in Menschen als Vorlage für DNA-Reparaturen dienen kann, konnte im Zuge dieser Arbeit durch mehrere in vitro Experimente mit Kernextrakten aus humanen Zelllinien bestätigt werden. Allerdings konnte keinerlei Einfluss von (trans-)gespleißter RNA auf die DNA-Reparatur in zahlreichen in vitro Experimenten nachgewiesen werden. Mit einem daraufhin etablierten in vivo System konnte ebenfalls ein Einfluss von (trans-) gespleißter RNA auf die DNA-Reparatur ausgeschlossen werden. Weiterhin konnten mit Hilfe der durchgeführten RACE-Experimente vorzeitige Polyadenylierungen von Transkripten in den Bruchpunktsregionen von MLL, AF4, AF9 und ENL identifiziert werden. Durch diese ungewöhnliche Termination der Transkription werden stark verkürzte Transkripte erzeugt, welche in kurze Proteinisoformen translatiert werden können. Ein Vergleich von 274 unterschiedlichen Bruchpunktsequenzen mit größeren direkten und indirekten Sequenzwiederholungen zwischen der Bruchpunktsregion von MLL und den Bruchpunktsregionen seiner häufigsten Translokationspartner wurde ebenfalls durchgeführt. Eine signifikante Korrelation zwischen den Sequenzwiederholungen und der Lokalisation der Bruchpunkte war jedoch nicht erkennbar. Bei diesem Vergleich fielen allerdings Häufungen von Bruchpunkten im MLL-Gen mit AF4, AF9 und ENL als Translokationspartner auf, wobei sich die Ursache für diese Häufungen auf Topoisomerase II Spaltstellen zurückführen ließ.
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The role of oncogenic Cbl mutants in Kit signaling and myeloid transformation
(2009)
- Acute myeloid leukemia (AML) is a hematopoietic cell disorder characterized by a block in differentiation and increased proliferation and survival of malignant blasts. Expansion of the malignant cell clone effects the normal production of blood cells and – if left untreated – leads to death. Receptor tyrosine kinases (RTKs) play an important role in the pathogenesis of AML, as they are either often mutated or overexpressed. In normal hematopoiesis, RTK signal termination is tightly controlled, and involves ubiquitination, internalization, endocytosis and degradation. Cbl proteins are E3 ligases and have been shown to ubiquitinate several activated RTKs, including Flt3 and Kit, targeting them for degradation. Recently, several Cbl mutations have been identified: Cbl-R420Q was identified in an AML patient and Cbl-70Z was identified in a mouse lymphoma model. In this thesis work, the role of these Cbl mutants in Kit signaling and in a mouse transplantation model was studied. Cbl mutants (Cbl-R420Q, Cbl-70Z) have the ability to transform the myeloid 32D cell line in cooperation with Kit WT. Cbl mutants along with Kit promoted interleukin-3 (IL3)-independent proliferation and enhanced the cell survival of 32D cells. In contrast, expression of the Cbl mutants alone did not confer IL3-independent growth. Stem cell factor (SCF, the Kit ligand) dependent growth was enhanced in the presence of Cbl mutants and Cbl mutants promoted colonogenic growth in the presence of Kit. Furthermore, Cbl mutants inhibited the ubiquitination of the activated Kit receptor. In addition, Cbl mutants inhibited the endocytosis of the activated Kit receptor. Retroviral expression of Cbl mutants in transplanted bone marrow induced a generalized mastocytosis, a myeloproliferative disease and, in rare care cases, myeloid leukemia. Splenomegaly was observed in the presence of Cbl mutants. Furthermore, mast cells with variable range of infiltration were noticed in all the vital organs (spleen, liver, bone marrow, lung, kidney, heart) of Cbl (mutant) transplanted mice. Almost all recipients of bone marrow cells transduced with Cbl mutants developed a lethal hematologic disorder with a mean latency of 341 days in the Cbl-R420Q group and 395 days in the Cbl-70Z group. This is the first published report on a hematological disease with Cbl mutants in a mouse model. Co-immunoprecipitation studies indicated that Cbl-70Z binds to Kit, even in the absence of Kit ligand. Cbl-R420Q also bound to Kit in the absence of SCF, albeit to a lesser extent. Association of Cbl mutants to Kit was enhanced in the presence of SCF. Signaling studies demonstrated the constitutive activation of Akt and Erk in the presence of Cbl mutants and Kit. In addition, Cbl mutants enhanced the SCF-dependent Kit, Akt and Erk activation. Cbl-70Z, in association with kinase-dead Kit (Kit-KD) or kinase-dead Flt3 (Flt3-KD), conferred IL3-independent growth and survival to the myeloid 32D cell line. Cbl-R420Q provided only a slight growth advantage in the presence of Kit-KD. As demonstrated by pharmacological inhibition studies, Akt activation was necessary for the transformation mediated by Cbl-70Z and Kit-KD / Flt3-KD. Cbl mutants enhanced the Src family kinases (SFKs) activity. The pharmacological inhibition of SFK activity inhibited the proliferation and colonogenic growth. Interaction was found between Cbl-70Z, SFKs and Kit-KD. The SFK member Fyn was identified to bind to Cbl. In addition, kinase activity of SFKs was necessary for binding to Cbl, since SFKs inhibition by PP-2 abolished the binding between the complex-binding partners. Dasatinib and PP-2, both SFK inhibitors, inhibited the Cbl and Akt phosphorylation indicating that Fyn acts upstream of Akt. Inhibition of Kit with imatinib reduced the proliferation of cells overexpressing Kit WT and Cbl-70Z much stronger compared with cells expressing Kit-KD and Cbl-70Z, but much less than the dual KIT/SFK inhibitor dasatinib. This indicated that Kit kinase activity was required but not essential. The data presented in this thesis work implies that both RTK and SFK inhibition may have to be targeted, in order to effectively prevent transformation. In summary, the present thesis work indicates an important role of Cbl, Kit and SFKs in myeloid transformation and deregulated signal transduction.
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Role of SOCS proteins in FLT3-ITD and BCR/ABL mediated leukemogenesis
(2010)
- Acute myeloid/lymphoid leukemia is a fatal hematological malignancy characterized by accumulation of nonfunctional, immature blasts, which interferes with the production of normal blood cells. Activating mutations of receptor tyrosine kinases are common genetic lesions in leukemia. FLT3-ITD is a frequent activating mutation found in AML patients, leading to uncontrolled proliferation of leukemic blasts. FLT3-ITD directly activates STAT5, leading to the induction of STAT5 target gene expression like PIM kinases and SOCS genes. STAT5 and PIM kinases have been shown to play a crucial role in the FLT3-ITD mediated transformation. On the other hand, the role of SOCS proteins in FLT3-ITD mediated transformation has not been studied to date. SOCS proteins are part of a negative feedback mechanism that controls Jak kinases downstream of cytokine receptors. One of the SOCS family members, SOCS1 has been reported to suppress oncogenecity of several activating kinases implicated in hematologic malignancies. In this thesis the role of these SOCS proteins in FLT3-ITD mediated transformation (in vitro) and leukemogenesis (in vivo) is systematically explored. Expression of FLT3-ITD in cell lines of myeloid (32D) and lymphoid (Ba/F3) origin, led to CIS, SOCS1 and SOCS2 expression. FLT3-ITD expression in primary murine bone marrow stem/progenitor cells led to a 59 fold induction of SOCS1 expression. Furthermore, FLT3-ITD positive AML cell lines (MV4-11, MOLM-13) show kinase dependent CIS, SOCS1, and SOCS3 expression. Importantly SOCS1 is highly expressed in AML patients with FLT3-ITD compared to healthy individuals. SOCS1 protein was expressed in FLT3-ITD transduced murine bone marrow stem cells and SOCS1 expression was abolished with kinase inhibition in MOLM-13 cell line. In conclusion, SOCS1 was highly regulated by FLT3-ITD in myeloid, lymphoid cell lines, in bone marrow stem/progenitors and in AML patient samples. SOCS1 co-expression did not affect FLT3-ITD mediated signaling and proliferation, but abolished IL-3 mediated proliferation and protected 32D cells from interferon-α and interferon-γ mediated growth inhibition. FLT3-ITD expressing 32D cells showed diminished STAT1 activation in response to interferons (α and γ). Alone, SOCS1 strongly inhibited cytokine induced colony formation of bone marrow stem and progenitors, but not FLT3-ITD induced colony formation. Most importantly, in the presence of growth inhibitory interferon-γ, SOCS1 co-expression with FLT3-ITD led to increased colony formation compared to FLT3-ITD alone. Taken together, FLT3-ITD induced and exogenously expressed SOCS1, shielded cells from external cytokines, signals, while not affecting FLT3-ITD induced proliferation/signaling. In further experiments the in vivo effects of SOCS1 were studied in a bone marrow transplantation model. SOCS1 bone marrow transplants were unable to engraft/proliferate in mice. FLT3-ITD was shown to induce a myeloproliferative disease. Both control (empty vector), SOCS1 transplanted mice were normal and did not show any disease phenotype. FLT3-ITD alone and SOCS1 co-expressing FLT3-ITD developed either myeloproliferative disease or acute lymphoblastic leukemia with equal distribution. SOCS1 co-expression with FLT3-ITD led to a decreased latency. Mice transplanted with FLT3-ITD alone and SOCS1 co-expressing FLT3-ITD displayed enlarged spleens, liver and hypercellular bone marrow indicating infiltration of leukemic cells. Mice were also anemic and showed decreased platelet counts. Importantly SOCS1 co-expression particularly shortened the latency of myeloproliferative disease but not of acute lymphoblastic leukemia. In summary, in the context of FLT3-ITD, SOCS1 acts as a ‘conditional oncogene’ and cooperates with FLT3-ITD in the development of myeloproliferative disease. With these data we propose the following model: FLT3-ITD induces SOCS gene expression, which shields cells against proliferation and differentiation signals from cytokines, while not affecting FLT3-ITD mediated proliferative signals. This leaves cells under the dictate of FLT3-ITD thereby contributing to leukemogenesis. Similar to FLT3-ITD, BCR/ABL (P190) (an oncogenic fusion kinase often found in acute lymphoblastic leukemia) induces SOCS gene expression in K562 and long-term cultured cells from patients with acute lymphoblastic leukemia. SOCS1 co-expression does not affect BCR/ABL mediated proliferation while abrogating IL-3 mediated proliferation. These findings suggest that SOCS proteins may play a general co-operative role in the context of oncogenes which aberrantly activate STAT3/5 independently of JAK kinases. This study reveals a novel molecular mechanism of FLT3-ITD mediated leukemogenesis and suggests SOCS genes as potential therapeutic targets.
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Role of enhanced stem cell capacities in leukemogenesis
(2006)
- Unlimited self-renewal is an absolute prerequisite for any malignancy, and is the ultimate arbiter of the continuous growth and metastasis of tumors. It has been suggested that the self-renewal properties of a tumor are exclusively contained within a small population, i.e., the so-called cancer stem cells. Enhanced self-renewal potential plays a pivotal role in the development of leukemia. My data have shown that APL associated translocation products PML/RARalpha and PLZF/RARalpha increased the replating efficiency of mouse lin-/Sca1+ hematopoietic stem cells (HSCs). This effect is partly mediated by induction of gamma–catenin which is an important mediator of the Wnt signaling pathway and has been shown to be up regulated by the AML associated translocation products(AATPs). Suppression of gamma–catenin by siRNA can abrogate the increased replating efficiency induced by AATPs. Transduction of gamma–catenin in lin-/Sca1+ HSCs led to increased replating efficiency and the expression of stem cell markers Sca1 and c-kit. Additionally it induced accelerated cell cycle progression of mouse bone marrow HSCs. Transduction/transplantation mouse models have shown that ectopic expression of gamma–catenin in HSCs led to acute myeloid leukemia without maturation. These data suggest important roles of Wnt signaling pathway in the leukemogenesis induced by PML/RARalpha, PLZF/RARalpha and AML1/ETO. In contrast to AATPs, CML and Ph+-ALL associated translocation products p185(BCR-ABL) and p210(BCR-ABL) did not affect the self-renewal potential of hematopoietic stem/progenitor cells. However my studies indicated that their reciprocal translocation products p40(ABL/BCR) and p96(ABL/BCR) actually increased the replating efficiency of hematopoietic stem/progenitor cells. The effect is stronger when induced by p96(ABL/BCR) than by p40(ABL/BCR). It is very intriguing that p96(ABL/BCR) can activate Wnt signaling and up regulate the expression of HoxB4. Transduction/transplantation mouse model has shown that p40(ABL/BCR) and p96(ABL/BCR) both have their own leukemogenic potential. Given the fact that leukemic stem cells maintain the growth of tumor and are the origin of relapse, the cure of leukemia is dependent on the eradication of the leukemic stem cell and abrogation of aberrantly regulated self-renewal capability. Both t-RA and As2O3 have been shown to induce complete remission in APL patients with PML/RARalpha translocation product. However, t-RA as a single agent achieves completeremission (CR) but not complete molecular remissions (CMR). Therefore, virtually all patients will experience a relapse within a few months. In contrast to t-RA, As2O3 as a single agent is able to induce CR as well as CMR followed by long-term relapse-free survival in about 50% of APL patients even if relapsed after treatment with t-RA-containing chemotherapy regimens. Nothing is known about the mechanisms leading to the complete different clinical outcomes by the two compounds although both have been shown to induce differentiation of blast cells, proliferation arrest, induction of apoptosis and degradation of PML/RARalpha. We investigated the effect of t-RA and arsenic on PML/RARalpha-expressing cell population with stem cell capacity derived from the APL cell line NB4 as well as Sca1+/lin- murine bone marrow cells. We found that t-RA did not reduce the replating efficiency in PML/RARalpha- and PLZF/RARalpha-infected Sca1+/lincells whereas it selected small compact colonies representing very early progenitor cells. T-RA was unable to reduce the capacity to form colony forming units-spleen (CFU-S) of Sca1+/lin-cells expressing PML/RARalpha, additionally t-RA did not impair the capability of engraftment of NB4 cells in NOD/SCID mouse. On the contrary to t-RA, As2O3 abolished the aberrant self-renewal potential of Sca1+/lin- cells expressing PML/RARalpha. As2O3 not only abolished the replating efficiency of PML/RARalpha positive cells but also completely abrogated the ability of PML/RARalpha-positive HSC to produce CFU-S in vivo. On the contrary to As2O3, t-RA increased the absolute cell number and the percentage of cells in the side population with respect to the whole cell population in NB4 cells. Taken together these data suggest that arsenic but not all-trans retinoic acid overcomes the aberrant stem cell capacity of PML/RARalpha positive leukemic stem cells. My data prove for the first time that there is a direct relationship between the capacity of compounds to effectively target the LSC and their capacity to eradicate the leukemia, and, thereby, to induce complete molecular remission and long-term relapse-free survival. Thus, in order to increase the curative potential of leukemia therapies, future studies need to include the effect of given compounds on the stem cell compartment to determine their ability to eradicate the LSC.
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Regulation of the catalytic subunits of NADPH oxidase Nox1 and NOX4 in rat mesangial cells
(2005)
- The generation of O2- by NADPH oxidaes was mainly attributed to immune cells that kill invading bacteria or cancer cells. But importantly, in the past several years, several homologs of the catalytic subunit gp91phox (Nox2) of the phagocytic NADPH oxidase have been identified in non-immune cells and tissues. Superoxide production derived from NADPH oxidaes has been shown to play a role not only in host defense but also in defined signaling cascades mediating growth and apoptosis. The aim of this work was to study the expression and the regulation of the”new” Nox isoforms in rat renal mesangial cells (MC). In particular the following results were achieved. 1) mRNA’s for both Nox1 and Nox4 were detected by RT-PCR. 2) Nox1 mRNA levels were increased upon exposure to basic fibroblast growth factor (bFGF), platelet-derived growth factor (PDGF) and fetal calf serum (FCS) in a time- and dose-dependent manner. Exposure of MC to bFGF and FCS increased also basal production of reactive oxygen species (ROS) by MC. By contrast, Nox4 mRNA levels were not significantly affected by bFGF treatment, but were markedly down-regulated by PDGF and FCS. 3) To study the regulation of Nox1 on the protein level, an anti-Nox1 antibody was generated and characterized using affinity chromatography. Up-regulation of Nox1 expression by growth factors was confirmed also on the protein level. 4) Based on the already known cDNA sequence for Nox1, the transcriptional start site was determined by the “gene RACE” technique. 2547 bp of the genomic sequence of the 5´-flanking region of the Nox1 gene were cloned and sequenced using the „Genome-Walking“ method. To study the regulation of Nox1 transcription functional Nox1 promoter/luciferase fusions were be established. MC were transiently transfected with different promoter/luciferase constructs and stimulated with growth factors. By measuring luciferase activity it was determined that growth factors induced the Nox1 transcription and that the Nox1 core promoter is sufficient for the activation. 5) By measurement of superoxide radicals and analysis of Nox1 mRNA expression by quantitative RT-PCR (TaqMan) as well as protein level by Western blotting it could be shown that treatment of MC with NO donors inhibited the expression of Nox1 in a time- and dose-dependent manner. Moreover, using activators and inhibitors of the soluble guanylyl cyclase (sGC) it could be shown, that the activation of sGC mediates the effect of NO on Nox1 expression. However, NO had no inhibitory effect on Nox1 promoter activity. Experiments with the inhibitor of transcription, actinomycin D, suggest that NO-mediated regulation of Nox1 is triggered probably via post-transcriptional mechanisms. Nox4 is regulated on the mRNA levels in a similar manner as Nox1. 6) To analyze the sub-cellular localization of the Nox isoforms, coding sequences for Nox1 and Nox4 were fused together with green fluorescent protein into the pEGFP-N1 demonstrated that both isoforms are localized predominantly in the plasma membrane, but also in the perinuclear region and cytoplasm. However, the localization of Nox1 in the plasma membrane was more pronounced. 7) In addition to Nox1 and Nox4, mRNA of the newly identified NOXA1 that is a homolog of the p67phox subunit of NADPH oxidase was detected in MC by RT-PCR.
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Novel approaches of molecular targeting in Philadelphia chromosome positive leukemia
(2009)
- In Philadelphia Chromosome (Ph) positive ALL and CML the fusion between BCR and ABL leads to the BCR/ABL fusion proteins, which induces the leukemic phenotype because of the constitutive activation of multiple signaling pathways down-stream to the aberrant BCR/ABL fusion tyrosine kinase. Targeted inhibition of BCR/ABL by ABL-kinase inhibitors induces apoptosis in BCR/ABL transformed cells and leads to complete remission in Ph positive leukemia patients. However, a large portion of patients with advanced Ph+ leukemia relapse and acquire resistance. Kinase domain (KD) mutations interfering with inhibitor binding represent the major mechanism of acquired resistance in patients with Ph+ leukemia. Tetramerization of BCR/ABL through the N-terminal coiled-coil region (CC) of BCR is essential for the ABL-kinase activation. Targeting the CC-domain forces BCR/ABL into a monomeric conformation, reduces its kinase activity and increases the sensitivity for Imatinib. Here we show that i.) targeting the tetramerization by a peptide representing the Helix-2 of the CC efficiently reduced the autophosphorylation of both WT BCR/ABL and its mutants; ii.) Helix-2 inhibited the transformation potential of BCR/ABL independently of the presence of mutations; iii.) Helix-2 efficiently cooperated with Imatinib as revealed by their effects on the transformation potential and the factor-independence related to BCR/ABL with the exception of mutant T315I. These findings suggest that BCR/ABL harboring the T315I mutation have a transformation potential which is at least partially independent from its kinase activity. Targeted inhibition of BCR/ABL by small molecule inhibitors reverses the transformation potential of BCR/ABL. We definitively proved that targeting the tetramerization of BCR/ABL mediated by the N-terminal coiled-coil domain (CC) using competitive peptides, representing the Helix-2 of the CC, represents a valid therapeutic approach for treating Ph+ leukemia. To further develop competitive peptides for targeting BCR/ABL, we created a membrane permeable Helix-2 peptide (MPH-2) by fusing the Helix-2 peptide with a peptide transduction tag. In this study, we report that the MPH-2: (i) interacted with BCR/ABL in vivo; (ii) efficiently inhibited the autophosphorylation of BCR/ABL; (iii) suppressed the growth and viability of Ph+ leukemic cells; and (iv) was efficiently transduced into mononuclear cells (MNC) in an in vivo mouse model. The T315I mutation confers resistance against all actually approved ABL-kinase inhibitors and competitive peptides. It seems not only to decrease affinity for kinase inhibitors but to confer additional features to the leukemogenic potential of BCR/ABL. To determine the role of T315I in resistance to the inhibition of oligomerization and in the leukemogenic potential of BCR/ABL, we investigated its influence on loss-of-function mutants with regard to the capacity to mediate factor-independence. Thus we studied the effects of T315I on BCR/ABL mutants lacking functional domains in the BCR portion indispensable for the oncogenic activity of BCR/ABL such as the N-terminal coiled coil (CC), the tyrosine phosphorylation site Y177 and the serine/threonine kinase domain (ST), as well as on the ABL portion of BCR/ABL (#ABL-T315I) with or without the inhibitory SH3 (delta SH3-ABL) domain. Here we report that i.) T315I restored the capacity to mediate factor independence of oligomerization_deficient p185BCR/ABL; ii.) resistance of p185-T315I against inhibition of the oligomerization depends on the phosphorylation at Y177; iii.) autophosphorylation at Y177 is not affected by the oligomerization inhibition, but phosphorylation at Y177 of endogenous BCR parallels the effects of T315I; iv.) the effects of T315I are associated with an intact ABL_kinase activity; v.) the presence of T315I is associated with an increased ABL_kinase activity also in mutants unable to induce Y177 phosphorylation of endogenous BCR; vi.) there is no direct relationship between the ABL-kinase activity and the capacity to mediate factor_independence induced by T315I as revealed by the #ABL-T315I mutant, which was unable to induce Y177 phosphorylation of BCR only in the presence of the SH3 domain. In contrast to its physiological counterpart c-ABL, the BCR/ABL kinase is constitutively activated, inducing the leukemic phenotype. The N-terminus of c-ABL (Cap region) contributes to the regulation of its kinase function. It is myristoylated, and the myristate residue binds to a hydrophobic pocket in the kinase domain known as the myristoyl binding pocket in a process called “capping”, which results in an auto-inhibited conformation. Because the cap region is replaced by the N-terminus of BCR, BCR/ABL “escapes” this auto-inhibition. Allosteric inhibition by myristate “mimics”, such as GNF-2, is able to inhibit unmutated BCR/ABL, but not the BCR/ABL that harbors the “gatekeeper” mutation T315I. Here we investigated the possibility of increasing the efficacy of allosteric inhibition by blocking BCR/ABL oligomerization. We demonstrate that inhibition of oligomerization was able not only to increase the efficacy of GNF-2 on unmutated BCR/ABL, but also to overcome the resistance of BCR/ABL-T315I to allosteric inhibition. These results strongly suggest that the response to allosteric inhibition by GNF-2 is inversely related to the degree of oligomerization of BCR/ABL. Taken together these data suggest that the inhibition of tetramerization inhibits BCR/ABL-mediated transformation and can contribute to overcome Imatinib-resistance. The study provides the first evidence that an efficient peptide transduction system facilitates the employ-ment of competitive peptides to target the oligomerization interface of BCR/ABL in vivo. Further the data show that T315I confers additional leukemogenic activity to BCR/ABL, which might explain the clinical behavior of patients with BCR/ABL -T315I-positive blasts. In summary, our observations establish a new approach for the molecular targeting of BCR/ABL and its resistant mutants represented by the combination of oligomerization and allosteric inhibitors.
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Nicht-viraler Faktor-IX-Gentransfer und die Entwicklung von Faktor-IX-Muteinen für neue therapeutische Strategien bei Hämophilie A und B
(2010)
- Die Hämophile ist eine X-chromosomal vererbbare Blutungserkrankung, die durch einen funktionellen Mangel der Gerinnungsaktoren Faktor VIII oder Faktor IX im Fall der Hämo-philie A oder Hämophilie B hervorgerufen wird. Der niedrige therapeutische Schwellenwert in der Behandlung der Hämophilie (Faktorenspiegel >1%) macht diese Krankheit zu einem idealen Zielobjekt in der Gentherapie. Eine schwerwiegende Komplikation in der Behandlung der Hämophilen besteht in der Entwicklung von neutralisierenden Antikörpern gegen das the-rapeutisch substituierte Protein. Akute Blutungen in solchen Hemmkörper-Patienten werden derzeit durch FVIII- und FIX-unabhängigen Bypass-Agenzien kontrolliert. Im Rahmen dieser Arbeit wurde nach einer erfolgten Optimierung eines nicht-viralen Ansatzes zur Transgenex-pression von FIX in der Leber der Maus dieses Gentransfersystem dazu verwendet, um eine Entwicklung von neuen, auf FIX basierenden, FVIII-Bypass-Strategien in vivo zu ermöglichen. Im ersten Teil der vorliegenden Arbeit wurden Plasmidvektoren und Vektorrückgrat-freie Minicircle-Konstrukte auf ihre Effizienz zur Expression des FIX-Transgens nach hydrodyna-misch basiertem Gentransfer in die Leber der Maus untersucht. Der Gentransfer der Mini-circle führte hierbei zu einer höheren Transgenexpression und einem geringeren Abfall der FIX-Antigen-Spiegel über die Zeit. Darüber hinaus war das FIX-Protein selbst bei den höchs-ten Expressionsleveln (700% des physiologischen Levels) völlig funktional aktiv. Der Abfall der Transgenexpression über die Zeit konnte größtenteils auf den Verlust des Vektors zurück-geführt werden. Ein signifikanter Silencing-Effekt konnte nur in den Plasmidvektor- und nicht in den Minicircle-behandelten Gruppen beobachtet werden. Diesbezüglich wurde nach 100 Tagen Persistenz der nicht-viralen Vektoren in der Mausleber eine signifikante Akkumulation an CpG-Methylierungen in regulatorischen Sequenzen des hAAT-Promoters im Plasmidvek-tor gegenüber den Minicirclen ermittelt. Außerdem konnte ebenfalls eine Demethylierung von Cytosin-Nukleotiden in bakteriellen Dcm-Sequenzmotiven über die Zeit beobachtet werden, die eine signifikant höhere Rate für das Minicircle-Konstrukt im hAAT-Promoter aufwies. Die erprobten nicht-viralen Vektoren versprechen somit eine ausreichende Effizienz, um eine Translation in den Menschen, z. B. über eine spezifische Behandlung von Lebersegmenten, möglich erscheinen zu lassen. Die Methylierungsanalyse von Promoterelementen auf Sequenzebene erbrachte zudem konkrete Ansätze zum Design von nicht-viralen Vektoren mit einer noch stabileren FIX-Expression. Im zweiten Teil dieser Arbeit wurde mit Hilfe eines Screening-Systems zur Aktivitätstestung von rekombinant exprimierten FIX-Varianten die Mutation K265T als die entscheidende Sub-stitution im 99-loop identifiziert, welche die FVIII-unabhängige Aktivität im FIX-Protein unter physiologischen Bedingungen begünstigt. Das Wildtyp- IX-Protein braucht hingegen FVIII um eine 106-fache Steigerung seiner proteolytischen Aktivität zu erreichen. Durch Kombination der Mutation K265T mit V181I und I383V konnte diese spezifische FVIII-Bypass-Aktivität in der resultierenden FIX-Variante (ITV) auf 15,6% (verglichen zu FIX in Anwesenheit von FVIII) gesteigert werden. Durch Inkubation der FIX-Varianten mit Plasma-proben aus Hemmkörper-Patienten konnte die Funktionalität der FIX-Varianten selbst in der Anwesenheit von inhibitorischen FVIII-Antikörpern demonstriert werden. Durch Untersu-chungen des Aktivierungszustands von FIX konnte zudem gezeigt werden, dass die im Rah-men dieser Arbeit generierten FIX-Varianten nicht voraktiviert sind und die messbare FVIII-Bypass-Aktivität FIX spezifisch ist. Darüber hinaus konnte hier erstmals eine hämostatische Effizienz von FIX-Varianten mit einer FVIII-unabhängigen Aktivität in einem relevanten Krankheitsmodel demonstriert werden. Diesbezüglich resultierte der nicht-virale Gentransfer der FIX-Varianten in FVIII-K.O.-Mäusen in einer dosisabhängigen Verkürzung der aPTT-basierenden Gerinnungszeit und in einer Reduktion des Blutverlustes im tail-clip-Assay in An- oder Abwesenheit von inhibitorischen FVIII-Antikörpern. Desweiteren konnte zudem mittels Vakzinierung von FIX-WT-tolerierten Mäusen mit den FIX-Varianten demonstriert werden, dass die hier eingeführten Mutationen keine hoch-immunogenen Epitope des FIX-Proteins betreffen. Schließlich konnte die Expression der FIX-Varianten in hämostatisch normalen Mäusen nicht mit der Entstehung von thromboembolischen Ereignissen selbst in einem intakten Gerinnungssystem assoziiert werden. Die hier beschriebenen FIX-Varianten könnten somit einen sicheren und effizienten Therapieansatz zur Behandlung der Hämophilie A mit inhibitorischen Antikörpern darstellen und hinsichtlich der Halbwertszeit und des möglichen throboembolischen Risikos zu einer wesentlichen Verbesserung der bereits verfügbaren Bypass-Strategien beitragen.
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Method developments in coupling gel electrophoresis with mass spectrometry
(2011)
- Proteomic analysis is the large-scale identification and characterization of proteins including post translational modifications. Proteomics encompasses a number of approaches including bottom-up and top-down workflows which are widely used independently and complementary as tools for the successful study of protein species. However, up to the present day these techniques have not been able to overcome every analytical limitation. Mass spectrometry has played a vital role alongside proteomics in providing the required analytical means of detecting protein amounts down to the atomole range. Soft ionization methods such as matrix assisted laser desorption/ionization (MALDI) and electrospray ionization (ESI) have permitted the transfer of peptides and intact proteins into the gas phase without extensive degradation. The introduction of recent developments in MALDI technology such as the highly sensitive 4-chloro-alpha-cyanocinnamic acid matrix (Cl-CCA) as well as the commercial availability of a MALDI-LTQ-Orbitrap which boosts peptide mass accuracy below 3 parts per million (ppm), have offered new prospective in protein analysis. The aim of the current study is to incorporate these new aspects and provide further advancements in gel-based as well as gel-free proteomic workflows. Peptides of proteolytically digested proteins are routinely analyzed by means of peptide mass fingerprinting (PMF) often combined with MS/MS analyses to complement and substantiate PMF results by peptide sequence information. The most widely used protease for enzymatic digestion is trypsin, since it exhibits a very specific cleavage behavior limited to C-terminal hydrolyses after basic amino acids. However, less specific enzymes such as chymotrypsin, elastase and pepsin have emerged as useful tools in the analysis of particular protein classes e.g. membrane, cereal, and phosphorylated proteins. In this work a comprehensive bottom-up proteomic investigation including in-solution and in-gel protein digestions of analytes covering small to large, acidic to basic, and hydrophobic to hydrophilic proteins in combination with a series of less specific enzymes are presented in order to show the superiority of the novel MALDI matrix Cl-CCA. The Cl-CCA matrix proved to be highly superior compared to standard α-cyano-4-hydroxycinnamic acid (CHCA) since an average detection of more than 2- to 3-fold peptide amount was possible depending on the used protease and, therefore, resulting in strongly increased sequence coverage. Additionally, protein identification of chymotrypsin and elastase in-gel digested protein standards was evaluated. The MALDI-LTQ-Orbitrap providing peptide mass accuracy below and up to 3 ppm in combination with Cl-CCA as matrix and newly optimized digestion conditions led to unambiguous protein identifications of all chymotryptic digests outperforming its tryptic counterparts in the case of hydrophobic bacteriorhodopsin and α-globin from hemoglobin A (α-HgbA). In addition, significantly higher sequence coverage and increased number of detected peptides was acquired. Moreover, a proposed workaround for elastase digestions was capable of providing a solution for successful identification results. Apart from digestions of singly separated proteins, solution isoelectic focusing (sIEF) was evaluated. OFFGEL fractionation is an efficient means of fractionating peptides and proteins according to their isoelectric point (pI) values through immobilized pH gel (IPG) strips after which samples are recovered in solution. Consequently, an issue of peptide recovery arises as a category of peptides relatively insoluble to the recovery solution should be present. A method was developed including the scraping of gel matrix from the IPG strips and peptide extraction using acetonitrile as organic solvent in combination with analytical techniques such as nLC-MALDI-MS/MS for peptide identification. The nature of the peptide species remaining in-gel was analysed and attributed to peptide solubility. A general trend in which a high percentage of neutral and hydrophobic peptides remaining entrapped in the IPG gel strip was observed. The present work also examines a new top-down proteomic workflow involving protein elution from cleavable gels containing the labile crosslinker ethylene-glycol-diacrylate (EDA). Protein amounts of as low as 100 ng loaded onto EDA gels were detected using MALDI-TOF MS in the linear acquisition mode. Proteins from 8.5 up to 78 kDa were successfully measured including a hydrophobic 15 kDa core protein attaining a GRAVY score of +0.079. Additionally, the method was compatible with one dimensional protein separation as well as for 2-D IEF/SDS-PAGE. Lastly, two methods for protein identification were tested and found to be compatible to the proposed technique.
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Leukämogenese durch die Translokation t(4;11) - Funktionelle Analyse der Translokationsprodukte MLL/AF4 und AF4/MLL
(2006)
- Das humane MLL-Gen (Mixed Lineage Leukemia) ist in chromosomale Translokationen mit mehr als 50 verschiedenen Partnergenen involviert. Alle diese Rearrangements sind mit akuter lymphatischer oder akuter myeloischer Leukämie assoziiert. Die reziproke Translokation t(4;11) ist ursächlich für die Entstehung einer akuten lymphatischen Leukämie, die gehäuft bei Kleinkindern auftritt. Die Prognose dieser aggressiven Leukämie ist sehr schlecht, da die leukämischen Blasten nahezu Therapie-resistent sind. Für einige MLL-Rearrangements konnte in Transduktions/Transplantations-Experimenten gezeigt werden, dass das MLL-Fusionsgen akute myeloische Leukämien in Mäusen induzieren kann. Aus diesem Grund steht immer noch das jeweilige MLL-Fusionsprotein im Mittelpunkt der Suche nach einem zugrunde liegenden Pathomechanismus. Die Versuche, ein Tiermodell mit dem MLL/AF4- Fusionsprodukt zu etablieren, blieben lange Zeit erfolglos. Erst Anfang dieses Jahres gelang es, durch eine knock-in Strategie, transgene Mäuse zu generieren, die das MLL/AF4 Translokationsprodukt tragen. Diese Mäuse entwickeln nach einer sehr langen Latenzzeit von bis zu 540 Tagen diffuse B-Zell-Lymphome. An der t(4;11) sind die Gene MLL auf Chromosom 11q23 und AF4 auf Chromosom 4q21 beteiligt. Die reziproke Translokation führt zur Entstehung von zwei Fusionsgenen (MLL/AF4 und AF4/MLL) mit intaktem Leserahmen. Wir nehmen an, dass beide Fusionsgene notwendig sind, um die Entartung der Zellen zu bewirken. Zum Einen ist der beschriebene Phänotyp der transgenen MLL/AF4 positiven Mäuse mit dem aggressiven Verlauf der t(4;11) Leukämie nicht vergleichbar, und zum Anderen findet man bei der Mehrzahl der Patienten mit einer t(4;11) beide Fusionstranskripte in den leukämischen Blasten. Um die Eigenschaften der Fusionsproteine AF4/MLL und MLL/AF4 zu untersuchen, wurden stabil transfizierte murine embryonale Fibroblasten-Linien etabliert, die entweder eines oder beide Fusionsgene regulierbar exprimierten. Mit Hilfe dieses in vitro Modells konnte man erstmals die Auswirkungen der gleichzeitigen Expression beider Fusionsgene auf das Verhalten der Zellen analysieren. Die Untersuchungen der Proliferation und der Apoptoseraten der verschiedenen transfizierten Zelllinien ergab, dass das AF4/MLL Fusionsprotein in den Zellen zu Wachstumstransformation führt, aber gleichzeitig die Zellen für den Zelltod durch bislang unbekannte Apoptosemechanismen sensitiviert. Das MLL/AF4 Translokationsprodukt war nicht in der Lage, eine Wachstumstransformation auszulösen. Vielmehr wurde deutlich, dass die Expression von MLL/AF4 die Proliferation der Zellen hemmt. Die Untersuchung der spezifischen Apoptoserate in den MLL/AF4 positiven Zellen ergab, dass die Zellen sowohl unter normalen Bedingungen als auch unter Stress-Konditionen Apoptose-resistent waren. Damit besitzen beide Fusionsproteine onkogene Eigenschaften. Da nur die mit AF4/MLL und MLL/AF4 transfizierten Zellen eine stark erhöhte Proliferation aufwiesen, im Wachstum transformiert waren und eine erhöhte Apoptoseresistenz zeigten, wurde deutlich, dass die Eigenschaften beider Fusionsproteine notwendig sind, um den vollständig transformierten Phänotyp auszulösen. Um die Veränderungen in den Zellen auf molekularer Ebene zu untersuchen, wurde mittels quantitativer PCR die Expression verschiedener Zellzyklus- und Apoptose-regulierender Gene untersucht. Dabei wurde deutlich, dass die Expression Zellzyklus- und Apoptose-regulierender Gene in allen drei Zellen verändert war. Genexpressionsprofil-Studien der Zellen ergaben schließlich, dass der Transkriptionsfaktor Nanog in den doppelt-transfizierten Zellen verstärkt exprimiert wurde. Nanog ist in die Aufrechterhaltung der Pluripotenz und des Selbsterneuerungspotenzials von embryonalen Stammzellen involviert. In dieser Arbeit konnte erstmals der Phänotyp einer Zelllinie beschrieben werden, die beide Fusionskonstrukte, AF4/MLL und MLL/AF4, stabil exprimierte. Dabei wurde deutlich, dass nur durch die Expression beider Fusionsgene ein Phänotyp erzeugt wird, der den Leukämoblasten sehr ähnlich ist. Die Expression von Nanog in diesen Zellen erklärt den Stammzell-Charakter der leukämischen Zellen.
