TY  - THES
A1  - Reimer, Anastasija
T1  - Search for novel antimicrobials against \(Neisseria\)  \(gonorrhoeae\) and \(Chlamydia\) \(trachomatis\)
T1  - Suche nach neuen Antimikrobiotika gegen \(Neisseria\)  \(gonorrhoeae\) und \(Chlamydia\) \(trachomatis\)
N2  - The obligate human pathogen Neisseria gonorrhoeae is responsible for the widespread sexually transmitted disease gonorrhoea, which in rare cases also leads to the development of disseminated gonococcal infection (DGI). DGI is mediated by PorBIA-expressing bacteria that invade host cells under low phosphate condition by interaction with the scavenger receptor-1 (SREC-I) expressed on the surface of endothelial cells. The interaction of PorBIA and SREC-I was analysed using different in vitro approaches, including surface plasmon resonance experiments that revealed a direct phosphate-independent high affinity interaction of SREC-I to PorBIA. However, the same binding affinity was also found for the other allele PorBIB, which indicates unspecific binding and suggests that the applied methods were unsuitable for this interaction analysis.
Since N. gonorrhoeae was recently classified as a “super-bug” due to a rising number of antibiotic-resistant strains, this study aimed to discover inhibitors against the PorBIA-mediated invasion of N. gonorrhoeae. Additionally, inhibitors were searched against the human pathogen Chlamydia trachomatis, which causes sexually transmitted infections as well as infections of the upper inner eyelid. 68 compounds, including plant-derived small molecules, extracts or pure compounds of marine sponges or sponge-associated bacteria and pipecolic acid derivatives, were screened using an automated microscopy based approach. No active substances against N. gonorrhoeae could be identified, while seven highly antichlamydial compounds were detected.
The pipecolic acid derivatives were synthesized as potential inhibitors of the virulence-associated “macrophage infectivity potentiator” (MIP), which exhibits a peptidyl prolyl cis-trans isomerase (PPIase) enzyme activity. This study investigated the role of C. trachomatis and N. gonorrhoeae MIP during infection. The two inhibitors PipN3 and PipN4 decreased the PPIase activity of recombinant chlamydial and neisserial MIP in a dose-dependent manner. Both compounds affected the chlamydial growth and development in epithelial cells. Furthermore, this work demonstrated the contribution of MIP to a prolonged survival of N. gonorrhoeae in the presence of neutrophils, which was significantly reduced in the presence of PipN3 and PipN4.
SF2446A2 was one of the compounds that had a severe effect on the growth and development of C. trachomatis. The analysis of the mode of action of SF2446A2 revealed an inhibitory effect of the compound on the mitochondrial respiration and mitochondrial ATP
production of the host cell. However, the chlamydial development was independent of proper functional mitochondria, which excluded the connection of the antichlamydial properties of SF2446A2 with its inhibition of the respiratory chain. Only the depletion of cellular ATP by blocking glycolysis and mitochondrial respiratory chain inhibited the chlamydial growth. A direct effect of SF2446A2 on C. trachomatis was assumed, since the growth of the bacteria N. gonorrhoeae and Staphylococcus aureus was also affected by the compound.
In summary, this study identified the severe antichlamydial activity of plant-derived naphthoquinones and the compounds derived from marine sponges or sponge-associated bacteria SF2446A2, ageloline A and gelliusterol E. Furthermore, the work points out the importance of the MIP proteins during infection and presents pipecolic acid derivatives as novel antimicrobials against N. gonorrhoeae and C. trachomatis.
N2  - Neisseria gonorrhoeae ist ein obligat humanpathogenes Bakterium, das für die weltweit verbreitete sexuell übertragbare Krankheit Gonorrhoe verantwortlich ist. In seltenen Fällen kann es auch zur Ausbildung der Disseminierten Gonokokken-Infektion (DGI) kommen, die mit der Expression des Gonokokken Oberflächenproteins PorBIA assoziiert ist. PorBIA-exprimierende Bakterien invadieren in die Wirtszelle unter phosphatfreien Bedingungen, was durch eine Interaktion mit dem zellulären Oberflächenrezeptor scavenger receptor-1 (SREC-I) vermittelt wird. Die direkte Interaktion zwischen PorBIA und SREC-I wurde mittels verschiedenster Methoden analysiert, einschließlich einer Oberflächenplasmonresonanz-analyse, die eine direkte Bindung von PorBIA zu SREC-I in einem phosphatunabhängigen Schritt aufzeigte. Allerdings wurde dieselbe Affinität auch zu PorBIB gefunden, was auf eine unspezifische Bindung hindeutet und dafür spricht, dass die verwendeten Methoden für diese Interaktionsanalyse ungeeignet sind.
N. gonorrheae wurde vor kurzem wegen der stetig steigenden Anzahl antibiotikaresistenter Stämme als „Superkeim“ bezeichnet. Aufgrund dessen wurden Inhibitoren gegen die PorBIA-vermittelte Invasion von N. gonorrhoeae, aber auch gegen Chlamydia trachomatis, den humanpathogenen Erreger von sexuell übertragbaren Infektionen und chronisch-follikulärer Bindehautentzündung, gesucht. 68 niedermolekulare Substanzen wurden mittels eines automatisierten Fluoreszenzmikroskopieverfahrens auf ihre inhibitorische Wirkung hin analysiert. Zu den getesteten Substanzen zählten pflanzenabstammende Stoffe, Isolate aus marinen Schwämmen oder Schwamm-assoziierten Bakterien, sowie Pipecolinsäure-Derivate. Gegen N. gonorrheae konnten keine Substanzen identifiziert werden, während sieben antichlamydiale Inhibitoren detektiert wurden. 
Pipecolinsäurederivate wurden synthetisiert als potentielle Inhibitoren des virulenz-assoziierten Proteins “macrophage infectivity potentiator” (MIP), das eine Peptidyl-Prolyl-cis-trans-Isomerase Aktivität besitzt. Diese Arbeit untersuchte die Rolle des MIP Proteins von N. gonorrhoeae und C. trachomatis während einer Infektion. Die zwei Inhibitoren PipN3 und PipN4 senkten die PPIase Aktivität des rekombinanten Chlamydien und Neisserien MIPs. Beide Substanzen beeinträchtigten das chlamydiale Wachstum und die Entwicklung in Epithelzellen. Ebenso konnte eine tragende Rolle des N. gonorrhoeae MIPs für das Überleben der Bakterien in Gegenwart von Neutrophilen aufgezeigt werden, das durch PipN3 und PipN4 inhibiert wurde. 
SF2446A2 war einer der Inhibitoren, der einen erheblichen Effekt auf das Wachstum und die Entwicklung von C. trachomatis aufgewiesen hat. Während der Analyse des Wirkmechanismus von SF2446A2 konnte eine Hemmung der mitochondrialen Atmungskette und eine Abnahme der mitochondrialen ATP Produktion in der Wirtszelle festgestellt werden. Allerdings war die Entwicklung von C. trachomatis unabhängig von der Funktionsfähigkeit der Mitochondrien. Eine Verbindung zwischen der antichlamydialen Wirkung von SF2446A2 und der Inhibierung der Mitochondrienatmungskette konnte damit ausgeschlossen werden. Nur das Reduzieren von zellulärem ATP durch Blockieren der Glykolyse und mitochondrialen Atmungskette verursachte eine Beeinträchtigung des Chlamydienwachstums. Eine direkte Auswirkung von SF2446A2 auf C. trachomatis wurde angenommen, da die Substanz auch das Wachstum von anderen Bakterien wie N. gonorrhoeae und Staphylococcus aureus inhibierte.
Zusammengefasst identifizierte diese Studie die antichlamydiale Aktivität pflanzenabstammender Naphthochinone und der Isolate aus marinen Schwämmen oder Schwamm-assoziierten Bakterien SF2446A2, ageloline A und gelliusterol E. Ebenso verdeutlicht die Arbeit die Bedeutung der MIP Proteine während der Infektion und legt Pipecolinsäurederivate als mögliche neue Antibiotika gegen N. gonorrhoeae und C. trachomatis nahe.
KW  - Neisseria gonorrhoeae
KW  - antibiotics
KW  - Chlamydia trachomatis
KW  - Antimikrobieller Wirkstoff
KW  - Pipecolinsäurederivate
KW  - Neisseria
KW  - Chlamydia
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-143168
ER  - 
TY  - THES
A1  - Reis, Helena
T1  - Characterization of telomere protein complexes in Trypanosoma brucei
T1  - Charakterisierung von telomerischen Proteinkomplexen in Trypanosoma brucei
N2  - African trypanosomiasis is a disease endemic to sub-Saharan Africa. It affects humans as well as wild and domestic animals. The human form of the disease is known as sleeping sickness and the animal form as nagana, which are usually fatal if left untreated. The cause of African trypanosomiasis is the unicellular parasite Trypanosoma brucei. During its life cycle, Trypanosoma brucei shuttles between a mammalian host and the tsetse fly vector. In the mammalian host the parasite multiplies as bloodstream form (BSF) extracellularly in the bloodstream or the lymphatic system. Survival of BSF parasites relies on immune evasion by antigenic variation of surface proteins because its extracellular lifestyle leads to direct exposure to immune responses. At any given time each BSF cell expresses a single type of variant surface glycoprotein (VSG) on its surface from a large repertoire. The active VSG is transcribed from one of 15 specialized subtelomeric domains, termed bloodstream expression sites (BESs). The remaining 14 BESs are silenced. This monoallelic expression and periodic switching of the expressed VSG enables to escape the immune response and to establish a persistent infection in the mammalian host. During developmental differentiation from BSF to the insect vector-resident procyclic form (PCF), the active BES is transcriptionally silenced to stop VSG transcription. Thus, all 15 BESs are inactive in the PCF cells as surface protein expression is developmentally regulated. 
Previous reports have shown that the telomere complex components TbTRF, TbRAP1 and TbTIF2 are involved in VSG transcriptional regulation. However, the precise nature of their contribution remains unclear. In addition, no information is available about the role of telomeres in the initiation and regulation of developmental BES silencing. To gain insights into the regulatory mechanisms of telomeres on VSG transcription and developmental repression it is therefore essential to identify the complete composition of the trypanosome telomere complex.
To this end, we used two complementary biochemical approaches and quantitative label-free interactomics to determine the composition of telomere protein complexes in T. brucei. Firstly, using a telomeric pull-down assay we found 17 potential telomere-binding proteins including the known telomere-binding proteins TbTRF and TbTIF2. Secondly, by performing a co-immunoprecipitation experiment to elucidate TbTRF interactions we co-purified five proteins. All of these five proteins were also enriched with telomeric DNA in the pull-down assay. 
To validate these data, I characterized one of the proteins found in both experiments (TelBP1). In BSF cells, TelBP1 co-localizes with TbTRF and interacts with already described telomere-binding proteins such as TbTRF, TbTIF2 and TbRAP1 indicating that TelBP1 is a novel component of the telomere complex in trypanosomes. Interestingly, protein interaction studies in PCF cells suggested a different telomere complex composition compared to BSF cells. In contrast to known members of the telomere complex, TelBP1 is dispensable for cell viability indicating that its function might be uncoupled from the known telomere-binding proteins. Overexpression of TelBP1 had also no effect on cell viability, but led to the discovery of two additional shorter isoforms of TelBP1. However, their source and function remained elusive. 
Although TelBP1 is not essential for cell viability, western blot analysis revealed a 4-fold upregulation of TelBP1 in the BSF stage compared to the PCF stage supporting the concept of a dynamic telomere complex composition. We observed that TelBP1 influences the kinetics of transcriptional BES silencing during developmental transition from BSF to PCF. Deletion of TelBP1 caused faster BES silencing compared to wild-type parasites. 
Taken together, TelBP1 function illustrates that developmental BES silencing is a fine-tuned process, which involves stage-specific changes in telomere complex formation.
N2  - Afrikanische Trypanosomiasis ist eine Krankheit, die in Afrika südlich der Sahara endemisch vorkommt und sowohl Menschen als auch Wild- und Haustiere betrifft. Die menschliche Form der Krankheit ist als Schlafkrankheit und die Tierform als Nagana bekannt. Ohne Behandlung verläuft die Krankheit in der Regel tödlich. Der einzellige Parasit Trypanosoma brucei ist die Ursache dieser Krankheit. Während seines Lebenszyklus bewegt sich der Parasit zwischen einem Säugetierwirt und einem Insektenvektor, der Tsetsefliege. Im Säugetierwirt vermehrt sich der Parasit als Blutstromform (BSF) extrazellulär im Blutkreislauf und im Lymphsystem. Das Fortbestehen der BSF-Parasiten im Wirt beruht auf einer Immunausweichstrategie durch antigene Variation der Oberflächenproteine. Diese Abwehrstrategie ist erforderlich, da der Parasit durch seinen extrazellulären Lebensstil direkt der Immunantwort ausgesetzt ist. Zu jedem Zeitpunkt wird nur ein variables Oberflächenprotein (VSG) auf der Zelloberfläche aus einem großen Repertoire exprimiert. Dabei wird das aktive VSG von einer von 15 spezialisierten telomerproximalen Transkriptionseinheiten transkribiert, den sogenannten Blutstromform Expression Sites (BESs). Die restlichen 14 BESs sind inaktiv. Diese monoallelische Expression und das periodische Wechseln des exprimierten VSG ermöglichen dem Parasiten der Immunantwort zu entgehen und eine persistente Infektion im Säugetierwirt zu etablieren. Während der Differenzierung von BSF zur Insektenvektor-residenten prozyklischen Form (PCF) wird die aktive BES transkriptionell herunter reguliert um die VSG-Transkription zu stoppen. Somit sind alle 15 BESs in PCF-Zellen inaktiv, da die Expression von Oberflächenproteinen stadienspezifisch reguliert ist. 
Frühere Veröffentlichungen haben gezeigt, dass die Proteine TbTRF, TbRAP1 und TbTIF2 des Telomerkomplexes an der Transkriptionsregulation von VSG-Genen beteiligt sind. Es ist jedoch unklar, wie genau sie zur Regulation beitragen. Darüber hinaus gibt es keine Informationen über die Rolle von Telomeren bei der Initiation und Regulation der BES-Inaktivierung während der Differenzierung. Um Einblicke in die regulatorischen Mechanismen von Telomeren auf die VSG-Transkription und differenzierungsbedingte Repression der aktiven BES zu gewinnen, ist es daher notwendig, die vollständige Zusammensetzung der Telomerkomplexe in Trypanosomen zu identifizieren.
Zu diesem Zweck wurden zwei komplementäre biochemische Ansätze und quantitative Massenspektrometrie genutzt um die Zusammensetzung von Telomerproteinkomplexen in T. brucei zu bestimmen. Zunächst wurden mittels einer Affinitätschromatographie mit TTAGGG-Oligonukleotiden 17 potentielle telomerbindende Proteine gefunden. Darunter waren auch die bereits bekannten telomerbindenden Proteine TbTRF und TbTIF2. Zweitens wurde mit Hilfe eines Co-Immunpräzipitationsexperiments um die Interaktionen von TbTRF aufzuklären, fünf Proteine aufgereinigt. Alle diese fünf Proteine wurden auch mit telomerischer DNA in der Affinitätschromatographie angereichert.
Um diese Daten zu validieren, wurde eines der in beiden Experimenten gefundenen Proteine (TelBP1) charakterisiert. In BSF-Zellen co-lokalisiert TelBP1 mit TbTRF und interagiert mit bereits beschriebenen telomerbindenden Proteinen wie TbTRF, TbTIF2 und TbRAP1. Dies deutet darauf, dass TelBP1 eine weitere Komponente des Telomerkomplexes in Trypanosomen ist. Interessanterweise deuteten Proteininteraktionsstudien in PCF-Zellen auf eine andere Zusammensetzung des Telomerkomplexes im Vergleich zu BSF-Zellen.
Im Gegensatz zu den bekannten Mitgliedern des Telomerkomplexes ist TelBP1 für das Zellwachstum nicht essentiell. Damit könnte die Funktion von TelBP1 von den bekannten telomerbindenden Proteinen entkoppelt sein. Die Überexpression von TelBP1 zeigte auch keinen Einfluss auf das Zellwachstum, führte aber zur Entdeckung von zwei weiteren kürzeren Isoformen von TelBP1. Ihr Ursprung und Funktion blieben jedoch ungeklärt. 
Obwohl TelBP1 für das Zellwachstum entbehrlich ist, zeigten Westernblot-Analysen eine 4-fache Hochregulierung von TelBP1 in BSF-Zellen im Vergleich zu PCF-Zellen. Die stadienspezifische Regulation von TelBP1 unterstützt damit das Konzept von einer dynamischen Zusammensetzung der Telomerkomplexe. Zudem wurde beobachtet, dass TelBP1 die Kinetik der Inaktivierung der aktiven BES während der Differenzierung von der BSF zur PCF beeinflusst. Die Deletion von TelBP1 führte zu einem schnelleren Abschalten der BES im Vergleich zu Wildtyp-Parasiten.
Zusammengefasst zeigt die Funktion von TelBP1, dass das Abschalten der aktiven BES während der Differenzierung ein fein abgestimmter Prozess ist, der stadienspezifische Veränderungen der Telomerkomplexe beinhaltet.
KW  - Trypanosoma brucei
KW  - Genexpression <Molekulargenetik>
KW  - Telomer
KW  - telomere-binding protein
KW  - chromatin remodeling
KW  - developmental differentiation
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-151323
ER  - 
TY  - THES
A1  - Ritter, Cathrin
T1  - Scientific basics for new immunotherapeutic approaches towards Merkel cell carcinoma
T1  - Grundlagen neuer immuntherapeutischer Ansätze gegen das Merkelzellkarzinom
N2  - Merkel cell carcinoma (MCC) is an aggressive neuroendocrine skin cancer that has been associated with the Merkel cell polyomavirus (MCPyV). Indeed, MCC is one of the cancers with the best-established viral carcinogenesis. Despite persistence of the virus in MCC cells and the subsequent expression of viral antigens, the majority of MCC tumors are able to escape the surveillance of the immune system. Therefore the aim of the here presented thesis was to scrutinize immune escape mechanisms operative in MCC. A better understanding of their underlying molecular processes should allow to improve immunotherapeutic treatment strategies for MCC patients. The manuscripts included in this thesis characterize three novel immune evasion strategies of MCC. 

I) the epigenetic silencing of the NKG2D ligands MICA and MICB via histone H3 hypoacetylation
II) reduced HLA class I surface expression via epigenetic silencing of the antigen processing machinery (APM)
III) the activation of the PI3K-AKT pathway in a mutation independent manner as potential immune escape strategy

MCC tumors and MCC cell lines were analyzed for their expression of MICA/B, HLA and components of the antigen processing machinery as well as for the activation of the PI3K-AKT pathway in situ and in vitro. These analysis reviled MICA and MICB, as well as HLA class I were not expressed or at least markedly reduced in ~80% of MCCs in situ. The PI3K-AKT pathway, that had only recently been demonstrated to play a significant role in tumor immune escape, was activated in almost 90% of MCCs in situ. To determine the underlying molecular mechanisms of these aberrations well characterized MCC cell lines were further analyzed in vitro. The fact that the PI3K-AKT pathway activation was due to oncogenic mutations in the PIK3CA or AKT1 gene in only 10% of MCCs, suggested an epigenetic regulation of this pathway in MCC. In line with this MICA/B as well as components of the APM were indeed silenced epigenetically via histone hypoacetylation in their respective promoter region. Notably MICA/B and HLA class I expression on the cell surface of MCC cells could be restored after treatment with HDAC inhibitors in combination with the Sp1 inhibitor Mithramycin A in all analyzed MCC cell lines in vitro and in a xenotransplantation mouse model in vivo. Moreover inhibition of HDACs increased immune recognition of MCC cell lines in a MICA/B and HLA class I dependent manner. 

Several studies have accumulated evidence that immunotherapy is a promising treatment option for MCC patients due to the exquisite immunogenicity of this malignancy. However, current immunotherapeutic interventions towards solid tumors like MCC have to account for the plentitude of tumor immune escape strategies, in order to increase response rates. The immune escape mechanisms of MCC described in this thesis can be reverted by HDAC inhibition, thus providing the rationale to combine ‘epigenetic priming’ with currently tested immunotherapeutic regimens.
N2  - Das Merkelzellkarzinom (MCC) ist ein aggressiver neuroendokriner Hautkrebs, der mit dem Merkelzell-Polyomavirus (MCPyV) assoziiert ist. Das MCC ist eine der Krebserkrankungen mit der am besten etablierten viralen Karzinogenese. Trotz der Anwesenheit des MCPyV in MCC-Zellen und der daraus einhergehenden Expression viraler Antigene sind die meisten MCC-Tumoren in der Lage der Überwachung durch das Immunsystem zu entgehen. Aus diesem Grund war das Ziel der hier vorliegenden Arbeit, neue im MCC operative „immune escape“ Mechanismen zu ermitteln. Ein besseres Verständnis der hierbei zugrunde liegenden Mechanismen, sollte es ermöglichen, immuntherapeutische Behandlungsstrategien für MCC-Patienten zu verbessern. Die  vorgestellten Manuskripte beschreiben drei neuartige „immune evasion“ Strategien des MCC:

I) die epigenetische Inaktivierung der NKG2D-Liganden MICA und MICB mittels Histone-H3-Hypoacetylierung
II) eine reduzierte HLA Klasse I-Oberflächenexpression aufgrund epigenetischer Inaktivierung der Antigenprozessierungsmaschinerie (APM)
III) die mutationsunabhängige Aktivierung des PI3K-AKT-Signalweges, als potentieller „immune escape“ Mechanismus 

MCC-Tumoren und MCC-Zelllinien wurden sowohl bezüglich der Expression von MICA/B, HLA Klasse I und Komponenten der APM als auch auf die Aktivierung des PI3K Signalweges in situ und in vitro untersucht. Diese Analysen zeigten, dass sowohl MICA und MICB als auch HLA Klasse I in ca. 80% der MCC-Tumoren in situ nicht, oder nur sehr reduziert, exprimiert wurden. Der PI3K-AKT-Signalweg, welcher erst kürzlich mit Tumor „immune escape“ in Verbindung gebracht wurde, war in fast 90% aller MCC-Tumoren in situ aktiviert. Um die zugrunde liegenden molekularen Mechanismen dieser Aberrationen zu entschlüsseln, wurden gut charakterisierte MCC-Zelllinien in vitro untersucht. Die Tatsache, dass der PI3K-AKT-Signalweg in nur 10% der MCCs auf Mutationen im PI3KA- oder AKT1-Gen zurückzuführen war, suggeriert eine epigenetische Regulation dieses Signalwegs. In Übereinstimmung hiermit waren sowohl MICA/B als auch Gene der APM epigenetisch mittels Histon-Hypoacetylierung in ihren jeweiligen Promoterregionen inaktiviert. Bemerkenswerterweise konnten in vitro und in einem Xenotransplantations-Mausmodell in vivo sowohl die MICA/B als auch die HLA Klasse I-Oberflächenexpression aller untersuchter MCC-Zelllinien durch die Behandlung mit HDAC-Inhibitoren in Kombination mit dem Sp1-Inhibitor Mithramycin A wieder hergestellt werden. Des Weiteren erhöhte die Inhibition von HDACs die MCC-Immunerkennung auf eine MICA/B und HLA Klasse I-abhängige Weise. 

Zahlreiche aktuelle Studien bestärken die Annahme, dass aufgrund der besonderen Immunogenität des MCC, die Immuntherapie eine aussichtsreiche Behandlungsoption für MCC-Patienten darstellt. Nichtsdestotrotz müssen die derzeitigen immuntherapeutischen Methoden zur Behandlung solider Tumore die Vielzahl von Tumor „immune escape“ Mechanismen mitberücksichtigen, um die Ansprechrate zu erhöhen. Die Tatsache, dass die hier beschriebenen „immune escape“ Mechanismen durch HDAC-Inhibition aufgehoben werden können, spricht für die Hypothese, dass eine Kombination von „epigenetischem Priming“ mit derzeitig untersuchten immuntherapeutischen Ansätzen sinnvoll ist.
KW  - Merkel-Zellkarzinom
KW  - Merkel cell carcinoma
KW  - Epigenetics
KW  - MICA
KW  - MICB
KW  - Tumor Immunology
KW  - Immune Escape
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-124162
ER  - 
TY  - JOUR
A1  - Ruf, Franziska
A1  - Fraunholz, Martin
A1  - Öchsner, Konrad
A1  - Kaderschabeck, Johann
A1  - Wegener, Christian
T1  - WEclMon - A simple and robust camera-based system to monitor Drosophila eclosion under optogenetic manipulation and natural conditions
JF  - PLoS ONE
N2  - Eclosion in flies and other insects is a circadian-gated behaviour under control of a central and a peripheral clock. It is not influenced by the motivational state of an animal, and thus presents an ideal paradigm to study the relation and signalling pathways between central and peripheral clocks, and downstream peptidergic regulatory systems. Little is known, however, about eclosion rhythmicity under natural conditions, and research into this direction is hampered by the physically closed design of current eclosion monitoring systems.
We describe a novel open eclosion monitoring system (WEclMon) that allows the puparia to come into direct contact with light, temperature and humidity. We demonstrate that the system can be used both in the laboratory and outdoors, and shows a performance similar to commercial closed funnel-type monitors. Data analysis is semi-automated based on a macro toolset for the open imaging software Fiji. Due to its open design, the WEclMon is also well suited for optogenetic experiments. A small screen to identify putative neuroendocrine signals mediating time from the central clock to initiate eclosion showed that optogenetic activation of ETH-, EH and myosuppressin neurons can induce precocious eclosion. Genetic ablation of myosuppressin-expressing neurons did, however, not affect eclosion rhythmicity.
KW  - chronobiology
KW  - infrared radiation
KW  - light pulses
KW  - molting
KW  - Drosophila melanogaster
KW  - optogenetics
KW  - eclosion
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-170755
VL  - 12
IS  - 6
ER  - 
TY  - JOUR
A1  - Ruppert, Manuela
A1  - Franz, Mirjam
A1  - Saratis, Anastasios
A1  - Escarcena, Laura Velo
A1  - Hendrich, Oliver
A1  - Gooi, Li Ming
A1  - Schwenkert, Isabell
A1  - Klebes, Ansgar
A1  - Scholz, Henrike
T1  - Hangover links nuclear RNA signaling to cAMP regulation via the phosphodiesterase 4d ortholog dunce
JF  - Cell Reports
N2  - The hangover gene defines a cellular stress pathway that is required for rapid ethanol tolerance in Drosophila melanogaster. To understand how cellular stress changes neuronal function, we analyzed Hangover function on a cellular and neuronal level. We provide evidence that Hangover acts as a nuclear RNA binding protein and we identified the phosphodiesterase 4d ortholog dunce as a target RNA. We generated a transcript-specific dunce mutant that is impaired not only in ethanol tolerance but also in the cellular stress response. At the neuronal level, Dunce and Hangover are required in the same neuron pair to regulate experience-dependent motor output. Within these neurons, two cyclic AMP (cAMP)-dependent mechanisms balance the degree of tolerance. The balance is achieved by feedback regulation of Hangover and dunce transcript levels. This study provides insight into how nuclear Hangover/RNA signaling is linked to the cytoplasmic regulation of cAMP levels and results in neuronal adaptation and behavioral changes.
KW  - biology
KW  - hangover
KW  - dunce
KW  - Dunce isoforms
KW  - PDE4d
KW  - cellular stress
KW  - alcohol tolerance
KW  - Drosophila melanogaster
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-171950
VL  - 18
IS  - 2
ER  - 
TY  - JOUR
A1  - Römer, Daniela
A1  - Bollazzi, Martin
A1  - Roces, Flavio
T1  - Carbon dioxide sensing in an obligate insect-fungus symbiosis: CO\(_{2}\) preferences of leaf-cutting ants to rear their mutualistic fungus
JF  - PLoS ONE
N2  - Defense against biotic or abiotic stresses is one of the benefits of living in symbiosis. Leaf-cutting ants, which live in an obligate mutualism with a fungus, attenuate thermal and desiccation stress of their partner through behavioral responses, by choosing suitable places for fungus-rearing across the soil profile. The underground environment also presents hypoxic (low oxygen) and hypercapnic (high carbon dioxide) conditions, which can negatively influence the symbiont. Here, we investigated whether workers of the leaf-cutting ant Acromyrmex lundii use the CO\(_{2}\) concentration as an orientation cue when selecting a place to locate their fungus garden, and whether they show preferences for specific CO\(_{2}\) concentrations. We also evaluated whether levels preferred by workers for fungus-rearing differ from those selected for themselves. In the laboratory, CO\(_{2}\) preferences were assessed in binary choices between chambers with different CO\(_{2}\) concentrations, by quantifying number of workers in each chamber and amount of relocated fungus. Leaf-cutting ants used the CO\(_{2}\) concentration as a spatial cue when selecting places for fungus-rearing. A. lundii preferred intermediate CO\(_{2}\) levels, between 1 and 3%, as they would encounter at soil depths where their nest chambers are located. In addition, workers avoided both atmospheric and high CO\(_{2}\) levels as they would occur outside the nest and at deeper soil layers, respectively. In order to prevent fungus desiccation, however, workers relocated fungus to high CO\(_{2}\) levels, which were otherwise avoided. Workers’ CO\(_{2}\) preferences for themselves showed no clear-cut pattern. We suggest that workers avoid both atmospheric and high CO\(_{2}\) concentrations not because they are detrimental for themselves, but because of their consequences for the symbiotic partner. Whether the preferred CO\(_{2}\) concentrations are beneficial for symbiont growth remains to be investigated, as well as whether the observed preferences for fungus-rearing influences the ants’ decisions where to excavate new chambers across the soil profile.
KW  - fungi
KW  - nesting habits
KW  - carbon dioxide
KW  - ants
KW  - social systems
KW  - humidity
KW  - symbiosis
KW  - fungal physiology
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-159561
VL  - 12
IS  - 4
ER  - 
TY  - JOUR
A1  - Rössler, Wolfgang
A1  - Spaethe, Johannes
A1  - Groh, Claudia
T1  - Pitfalls of using confocal-microscopy based automated quantification of synaptic complexes in honeybee mushroom bodies (response to Peng and Yang 2016)
JF  - Scientific Reports
N2  - A recent study by Peng and Yang in Scientific Reports using confocal-microscopy based automated quantification of anti-synapsin labeled microglomeruli in the mushroom bodies of honeybee brains reports potentially incorrect numbers of microglomerular densities. Whereas several previous studies using visually supervised or automated counts from confocal images and analyses of serial 3D electron-microscopy data reported consistent numbers of synaptic complexes per volume, Peng and Yang revealed extremely low numbers differing by a factor of 18 or more from those obtained in visually supervised counts, and by a factor 22–180 from numbers in two other studies using automated counts. This extreme discrepancy is especially disturbing as close comparison of raw confocal images of anti-synapsin labeled whole-mount brain preparations are highly similar across these studies. We conclude that these discrepancies may reside in potential misapplication of confocal imaging followed by erroneous use of automated image analysis software. Consequently, the reported microglomerular densities during maturation and after manipulation by insecticides require validation by application of appropriate confocal imaging methods and analyses tools that rely on skilled observers. We suggest several improvements towards more reliable or standardized automated or semi-automated synapse counts in whole mount preparations of insect brains.
KW  - confocal-microscopy based automated quantification
KW  - mushroom bodies
KW  - honeybees
KW  - brain
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-170451
VL  - 7
IS  - 9786
ER  - 
TY  - JOUR
A1  - Sander, Bodo
A1  - Xu, Wenshan
A1  - Eilers, Martin
A1  - Popov, Nikita
A1  - Lorenz, Sonja
T1  - A conformational switch regulates the ubiquitin ligase HUWE1
JF  - eLife
N2  - The human ubiquitin ligase HUWE1 has key roles in tumorigenesis, yet it is unkown how its activity is regulated. We present the crystal structure of a C-terminal part of HUWE1, including the catalytic domain, and reveal an asymmetric auto-inhibited dimer. We show that HUWE1 dimerizes in solution and self-associates in cells, and that both occurs through the crystallographic dimer interface. We demonstrate that HUWE1 is inhibited in cells and that it can be activated by disruption of the dimer interface. We identify a conserved segment in HUWE1 that counteracts dimer formation by associating with the dimerization region intramolecularly. Our studies reveal, intriguingly, that the tumor suppressor p14ARF binds to this segment and may thus shift the conformational equilibrium of HUWE1 toward the inactive state. We propose a model, in which the activity of HUWE1 underlies conformational control in response to physiological cues—a mechanism that may be exploited for cancer therapy.
KW  - Medicine
KW  - Structural Biology
KW  - Molecular Biophysics
KW  - HUWE1
KW  - HECT Ligase
KW  - Ubiquitin
KW  - P14ARF
KW  - X-Ray Chrystallography
KW  - Enzyme Regulation
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-171862
VL  - 6
ER  - 
TY  - JOUR
A1  - Sbirkov, Yordan
A1  - Kwok, Colin
A1  - Bhamra, Amandeep
A1  - Thompson, Andrew J.
A1  - Gil, Veronica
A1  - Zelent, Arthur
A1  - Petrie, Kevin
T1  - Semi-quantitative mass spectrometry in AML cells identifies new non-genomic targets of the EZH2 methyltransferase
JF  - International Journal of Molecular Sciences
N2  - Alterations to the gene encoding the EZH2 (KMT6A) methyltransferase, including both gain-of-function and loss-of-function, have been linked to a variety of haematological malignancies and solid tumours, suggesting a complex, context-dependent role of this methyltransferase. The successful implementation of molecularly targeted therapies against EZH2 requires a greater understanding of the potential mechanisms by which EZH2 contributes to cancer. One aspect of this effort is the mapping of EZH2 partner proteins and cellular targets. To this end we performed affinity-purification mass spectrometry in the FAB-M2 HL-60 acute myeloid leukaemia (AML) cell line before and after all-trans retinoic acid-induced differentiation. These studies identified new EZH2 interaction partners and potential non-histone substrates for EZH2-mediated methylation. Our results suggest that EZH2 is involved in the regulation of translation through interactions with a number of RNA binding proteins and by methylating key components of protein synthesis such as eEF1A1. Given that deregulated mRNA translation is a frequent feature of cancer and that eEF1A1 is highly expressed in many human tumours, these findings present new possibilities for the therapeutic targeting of EZH2 in AML.
KW  - acute myeloid leukaemia
KW  - EZH2
KW  - mass spectrometry
KW  - methylation
KW  - eEF1A1
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-285541
SN  - 1422-0067
VL  - 18
IS  - 7
ER  - 
TY  - JOUR
A1  - Scheiner, Ricarda
A1  - Entler, Brian V.
A1  - Barron, Andrew B.
A1  - Scholl, Christina
A1  - Thamm, Markus
T1  - The Effects of Fat Body Tyramine Level on Gustatory Responsiveness of Honeybees (Apis mellifera) Differ between Behavioral Castes
JF  - Frontiers in Systems Neuroscience
N2  - Division of labor is a hallmark of social insects. In the honeybee (Apis mellifera) each sterile female worker performs a series of social tasks. The most drastic changes in behavior occur when a nurse bee, who takes care of the brood and the queen in the hive, transitions to foraging behavior. Foragers provision the colony with pollen, nectar or water. Nurse bees and foragers differ in numerous behaviors, including responsiveness to gustatory stimuli. Differences in gustatory responsiveness, in turn, might be involved in regulating division of labor through differential sensory response thresholds. Biogenic amines are important modulators of behavior. Tyramine and octopamine have been shown to increase gustatory responsiveness in honeybees when injected into the thorax, thereby possibly triggering social organization. So far, most of the experiments investigating the role of amines on gustatory responsiveness have focused on the brain. The potential role of the fat body in regulating sensory responsiveness and division of labor has large been neglected. We here investigated the role of the fat body in modulating gustatory responsiveness through tyramine signaling in different social roles of honeybees. We quantified levels of tyramine, tyramine receptor gene expression and the effect of elevating fat body tyramine titers on gustatory responsiveness in both nurse bees and foragers. Our data suggest that elevating the tyramine titer in the fat body pharmacologically increases gustatory responsiveness in foragers, but not in nurse bees. This differential effect of tyramine on gustatory responsiveness correlates with a higher natural gustatory responsiveness of foragers, with a higher tyramine receptor (Amtar1) mRNA expression in fat bodies of foragers and with lower baseline tyramine titers in fat bodies of foragers compared to those of nurse bees. We suggest that differential tyramine signaling in the fat body has an important role in the plasticity of division of labor through changing gustatory responsiveness.
KW  - behavior
KW  - biogenic amines
KW  - division of labor
KW  - nurse bee
KW  - forager
KW  - PER
KW  - octopamine
KW  - insect
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-157874
VL  - 11
IS  - 55
ER  -